Patent Publication Number: US-2019185879-A1

Title: Plants comprising wheat g-type cytoplasmic male sterility restorer genes,  molecular markers and uses thereof

Description:
FIELD OF THE INVENTION 
     The present invention relates generally to the field of plant breeding and molecular biology and concerns a method for selecting or producing a cereal plant comprising a functional restorer gene for wheat G-type cytoplasmic male sterility, and nucleic acids for use therein. 
     BACKGROUND 
     Cytoplasmic male sterility (CMS) is a major trait of interest in cereals such as wheat in the context of commercial hybrid seed production (Kihara, 1951; Wilson and Ross, 1962; Lucken, 1987; Sage, 1976). The cytoplasms of  Triticum timopheevi  (G-type) and  Aegilops kotschyi  (K-type) are widely studied as inducers of male sterility in common wheat ( Triticum aestivum ), due to few deleterious effects (Kaul, 1988; Lucken, 1987; Mukai and Tsunewaki, 1979). 
     In hybrid seed production system using the G-type cytoplasm, fertility restoration is a critical problem. Most of the hexaploid wheats do not naturally contain fertility restoration genes (Ahmed et al., Genes Genet. Syst. 2001). In the complicated restoration system of  T. timopheevi , eight Rf genes are reported to restore the fertility against  T. timopheevii  cytoplasm, and their chromosome locations have been determined, namely, Rf1 (1A), Rf2 (7D), Rf3 (1B), Rf4 (6B), Rf5 (6D), Rf6 (5D), Rf7 (7B) and Rf8 (Tahir &amp; Tsunewaki, 1969; Yen et al., 1969; Bahl &amp; Maan, 1973; Du et al., 1991; Sihna et al., 2013). Ma et al. (1991) transferred an Rf gene from  Aegilops umbellulata  to wheat, the gene being located on chromosomes 6AS and 6BS (from Zhou et al., 2005). 
     Ma and Sorrels (Crop Science 1995) reported the linkage of Rf3 to RFLP markers Xbcd249 and Xcdo442 on chromosome 1 BS. 
     Kojima (Genes Genet Syst 1997) localized a fertility restorer gene from Chinese Spring termed Rf3 gene at a position 1.2 cM and 2.6 cM distant from RFLP markers Xcdo388 and Xabc156, respectively, although the authors were able to separate Rf3 from Xcdo388. It was estimated that that Rf3 could exist within a region of 500 Kbp of the adjacent RFLP markers. 
     Ahmed Talaat et al (Genes Genet. Syst., 2001) determined the close linkage of a major Rf QTL against G-type cytoplasm on chromosome 1B with RFLP marker XksuG9c, close to marker Xabc156 as reported by Kojima et al (supra). 
     Zhang et al., (Yi Chuan Xue Bao 2003) describe an Rf gene located on 1BS with a genetic distance of 5.1 cM to microsatellite marker Xgwm550. 
     Zhou et al (2005) describe Rf3 gene to be located either between SSR markers Xgwm582 and Xbarc207 or between Xbarc207 and Xgwm131 but very close to Xbarc207. Since the previously identified RFLP markers of Kojima, Ahmed and Ma &amp; Sorrels were not mapped in their mapping population, a linkage map including these RFLP markers could not be constructed to better estimate the distance between Rf3 and the identified SSR markers. 
     Accordingly, there remains the need for more accurate markers to identify and track Rf loci in breeding, which are particularly useful for hybrid seed production, and for improved methods for fertility restoration in wheat Thimopheevi cytoplasm. The present invention provides a contribution over the art by disclosing the functional Rf gene on chromosome 1B and by providing markers that are more tightly linked to the causal gene. 
    
    
     
       FIGURE LEGENDS 
         FIG. 1 : Seed set on the main head (ss_mh), as observed in two different locations (g, m). Number of plants (y-axis) per class of amount of seed (x-axis). 
         FIG. 2 : Profile plot for significance of marker-trait associations along chromosome 1B in −log 10(p) Indicative threshold=3.9. 
         FIG. 3 : (A)—Predicted gene structure for the identified PPR gene, displaying the 2 potential splice variants (SV1, SV2). @ indicates CDS, #5′ UTR, and *3′ UTR (B) amino acid sequence of identified PPR gene indicating the PPR motifs (alternatingly underlined and not underlined) including the 5th and 35th amino acid implied in RNA recognition (bold). Met→lie SNP at position 143 indicated by *. (C) Graphical representation of the structure of the PPR protein with PPR motifs. 
         FIG. 4 : (A) Overall alignment of the putative RNA recognition motif of the identified PPR protein with ORF256. (B) Close-up showing nucleotide alignment. 
         FIG. 5 : Mean normalized expression levels of Rf3-PPR in tissues of Rf3 restorer and wild-type (non-restorer) F4 progeny of a cross between ‘Resource-5’ and a CMS line. Rf3-containing progeny were identified following KASP genotyping with fine-mapping markers and phenotyped to confirm restoration of fertility 
     
    
    
     DETAILED DESCRIPTION 
     The present invention describes the identification of a functional restorer (Rf) locus and gene for wheat G-type cytoplasmic male sterility (i.e.,  T. timopheevi  cytoplasm) located on chromosome 1B (short arm 1BS), as well as markers associated therewith. Said markers can be used in marker-assisted selection (MAS) of cereal plants, such as wheat, comprising said functional restorer genes located on chromosomes 1B. The identification of the genes and markers are therefore extremely useful in methods for hybrid seed production, as they can be used e.g. in a method for restoring fertility in progeny of a plant possessing G-type cytoplasmic male sterility, thereby producing fertile progeny plants from a G-type cytoplasmic male sterile parent plant. Likewise, the present disclosure also allows identifying plants lacking the desired allele, so that non-restorer plants can be identified and, e.g., eliminated from subsequent crosses. 
     One advantage of marker-assisted selection over field evaluations for fertility restoration is that MAS can be done at any time of year regardless of the growing season. Moreover, environmental effects are irrelevant to marker-assisted selection. 
     When a population is segregating for multiple loci affecting one or multiple traits, e.g., multiple loci involved in fertility restoration or multiple loci each involved in fertility restoration of different cytoplasmic male sterility (CMS) systems or loci affecting distinct traits (for example fertility and disease resistance) the efficiency of MAS compared to phenotypic screening becomes even greater because all the loci can be processed in the lab together from a single sample of DNA. Any one or more of the markers and/or marker alleles, e.g., two or more, up to and including all of the established markers, can be assayed simultaneously. 
     Another use of MAS in plant breeding is to assist the recovery of the recurrent parent genotype by backcross breeding. Backcross breeding is the process of crossing a progeny back to one of its parents. Backcrossing is usually done for the purpose of introgressing one or a few loci from a donor parent into an otherwise desirable genetic background from the recurrent parent. The more cycles of backcrossing that are done, the greater the genetic contribution of the recurrent parent to the resulting variety. This is often necessary, because donor parent plants may be otherwise undesirable, i.e., due to low yield, low fecundity or the like. In contrast, varieties which are the result of intensive breeding programs may have excellent yield, fecundity or the like, merely being deficient in one desired trait such as fertility restoration. As a skilled worker understands, backcrossing can be done to select for or against a trait. For example, in the present invention, one can select a restorer gene for breeding a restorer line or one select against a restorer gene for breeding a maintainer (female pool). 
     The presently described Rf locus on chromosome 1B was mapped to a segment along the chromosome 1B, in an interval of about 15.8 cM, said interval being flanked by markers of SEQ ID NO 2 and SEQ ID NO 8. 
     Thus, in a first aspect, a method is provided for selecting a cereal plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility or for producing a cereal plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility, comprising the steps of:
         (a) Identifying at least one cereal plant comprising at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B; and   (b) Selecting the plant comprising said at least one marker allele, wherein said plant comprises said functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B   wherein said at least one marker allele localises within an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 2 and SEQ ID NO 8.       

     In a second aspect, a method is provided for restoring fertility in a progeny of a G-type cytoplasmic male sterile cereal plant OR for producing a fertile progeny plant from a G-type cytoplasmic male sterile cereal parent plant, comprising the steps of
         (a) Providing a population of progeny plants obtained from crossing a female cereal parent plant with a male cereal parent plant, wherein the female parent plant is a G-type cytoplasmic male sterile cereal plant, and wherein the male parent plant comprises a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B;   (b) Identifying in said population a fertile progeny plant comprising at least one marker allele linked to said functional restorer gene allele for wheat G-type cytoplasmic male sterility, wherein said progeny plant comprises said functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B; and optionally   (c) Selecting said fertile progeny plant; and optionally   (d) Propagating the fertile progeny plant,   wherein said at least one marker allele localises within an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 2 and SEQ ID NO 8.       

     Male sterility in connection with the present invention refers to the failure or partial failure of plants to produce functional pollen or male gametes. This can be due to natural or artificially introduced genetic predispositions or to human intervention on the plant in the field. Male fertile on the other hand relates to plants capable of producing normal functional pollen and male gametes. Male sterility/fertility can be reflected in seed set upon selfing, e.g. by bagging heads to induce self-fertilization. Likewise, fertility restoration can also be described in terms of seed set upon crossing a male sterile plant with a plant carrying a functional restorer gene, when compared to seed set resulting from crossing (or selfing) fully fertile plants. 
     A male parent or pollen parent, is a parent plant that provides the male gametes (pollen) for fertilization, while a female parent or seed parent is the plant that provides the female gametes for fertilization, said female plant being the one bearing the seeds. 
     Cytoplasmic male sterility or “CMS” refers to cytoplasmic-based and maternally-inherited male sterility. CMS is total or partial male sterility in plants as the result of specific nuclear and mitochondrial interactions and is maternally inherited via the cytoplasm. Male sterility is the failure of plants to produce functional anthers, pollen, or male gametes although CMS plants still produce viable female gametes. Cytoplasmic male sterility is used in agriculture to facilitate the production of hybrid seed. 
     “Wheat G-type cytoplasmic male sterility”, as used herein refers to the cytoplasm of  Triticum timopheevi  that can confer male sterility when introduced into common wheat (i.e.  Triticum aestivum ), thereby resulting in a plant carrying common wheat nuclear genes but cytoplasm from  Triticum timopheevii  that is male sterile. The cytoplasm of  Triticum timopheevi  (G-type) as inducers of male sterility in common wheat have been extensively studied (Wilson and Ross, Genes Genet. Syst. 1962; Kaul, Male sterility in higher plants. Springer Verlag, Berlin. 1988; Lucken, Hybrid wheat. In Wheat and wheat improvement. Edited by E. G. Heyne. American Society of Agronomy, Madison, Wis, 1987; Mukai and Tsunewaki, Theor. Appl. Genet. 54, 1979; Tsunewaki, Jpn. Soc. Prom. Sci. 1980; Tsunewaki et al., Genes Genet. Syst. 71, 1996). The origin of the CMS phenotype conferred by  T. timopheevi  cytoplasm is with a novel chimeric gene termed orf256, which is upstream of coxl sequences and is cotranscribed with an apparently normal cox1 gene. Antisera prepared against polypeptide sequences predicted from orf256 recognized a 7-kDa protein present in the CMS line but not in the parental or restored lines (Song and Hedgcoth, Genome 37(2), 1994; Hedgcoth et al., Curr. Genet. 41, 357-365, 2002). 
     As used herein “a functional restorer gene allele for wheat G-type cytoplasmic male sterility” or “a functional restorer locus for wheat G-type cytoplasmic male sterility” or a “restorer QTL for wheat G-type cytoplasmic male sterility” indicates an allele that has the capacity to restore fertility in the progeny of a cross with a G-type cytoplasmic male sterility (“CMS”) line, i.e., a line carrying common wheat nuclear genes but cytoplasm from  Triticum timopheevii . Restoration against G-type cytoplasm has e.g. been described by Robertson and Curtis (Crop Sci. 9, 1967), Yen et al. (Can. J. Genet. Cytol. 11, 1969), Bahl and Maan (Crop Sci. 13, 1973), Talaat et al. (Egypt. J. Genet. 2, 195-205, 1973) Zhang et al., (2003, supra) Ma and Sorrels (1995, supra), Kojima (1997, supra), Ahmed Talaat et al (2001, supra), Zhou et al (2005, supra). Such restorer genes or alleles are also referred to as Rf genes and Rf alleles. 
     The term “maintainer” refers to a plant that when crossed with the CMS plant does not restore fertility, and maintains sterility in the progeny. The maintainer is used to propagate the CMS line, and may also be referred to as a non-restorer line. Maintainer lines have the same nuclear genes as the sterile one (i.e. do not contain functional Rf genes), but differ in the composition of cytoplasmic factors that cause male sterility in plants i.e. maintainers have “fertile” cytoplasm. Therefore when a male sterile line is crossed with its maintainer progeny with the same male sterile genotype will be obtained. 
     The term “cereal” relates to members of the monocotyledonous family Poaceae which are cultivated for the edible components of their grain. These grains are composed of endosperm, germ and bran. Maize, wheat and rice together account for more than 80% of the worldwide grain production. Other members of the cereal family comprise rye, oats, barley, triticale, sorghum, wild rice, spelt, einkorn, emmer, durum wheat and kamut. 
     In one embodiment, a cereal plant according to the invention is a cereal plant that comprises at least a B genome or related genome, such as wheat ( Triticum aestivum ; ABD), spelt ( Triticum spelta ; ABD) durum ( T. turgidum ; AB), barley ( Hordeum vulgare ; H) and rye ( Secale cereale ; R). In a specific embodiment, the cereal plant according to the invention is wheat ( Triticum aestivum ; ABD). 
     A “molecular marker” or “marker” or “marker nucleic acid” or “genetic marker”, as used herein, refers to a polymorphic locus, i.e. a polymorphic nucleotide (a so-called single nucleotide polymorphism or SNP) or a polymorphic DNA sequence at a specific locus. A marker refers to a measurable, genetic characteristic with a fixed position in the genome, which is normally inherited in a Mendelian fashion, and which can be used for mapping of a trait of interest or to identify certain individuals with a certain trait of interest. A marker thus refers to a gene or nucleotide sequence that can be used to identify plants having a particular allele, e.g., the presently described Rf alleles on chromosome 1B. A marker may be described as a variation at a given genomic locus. It may be a short DNA sequence, such as a sequence surrounding a single base-pair change (single nucleotide polymorphism, or “SNP”), or a long one, for example, a microsatellite/simple sequence repeat (“SSR”). A molecular marker may also include ‘Indels’ which refers to the insertion or the deletion of bases or a combination of both in the DNA of an organism, and which can be used as molecular markers. 
     The term “marker genotype” refers to the combination of marker alleles present at a polymorphic locus on each chromosome of the chromosome pair. The term “marker allele” refers to the version of the marker that is present in a particular plant at one of the chromosomes. Typically, a marker can exist as or can be said to have or to comprise two marker alleles. The term “haplotype”, as used herein, refers to a specific combination of marker alleles as present within a certain plant or group of (related) plants. See also the below definitions of a SNP (marker) genotype and SNP (marker) allele. 
     A “marker context” or “marker context sequence”, as used herein, refers to 50-150 bp upstream of a marker, such as a SNP marker, and/or 50-150 bp downstream of such a marker. The marker context of the herein described (SNP) markers is given in the sequence listing, flanking the SNP position. The upstream and downstream sequences of a (SNP) marker can also be referred to as (upstream and/or downstream) flanking sequences. 
     Identifying a cereal plant comprising at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B can be accomplished using a molecular marker assay that detects the presence of at least one such marker allele, e.g. the marker alleles described herein that are linked to the functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B. This can involve obtaining or providing a biological sample, i.e. plant material, or providing genomic DNA of a plant, and analyzing the genomic DNA of the material for the presence of at least one of said marker alleles (or the marker genotype for at least one of such markers). In this method also other molecular marker tests described elsewhere herein can be used. 
     As will be well known to a person skilled in the art, markers and marker assays include for example Restriction Fragment Length Polymorphisms (RFLPs), Random Amplified Polymorphic DNA&#39;s (RAPDs), Amplified Fragment Length Polymorphism&#39;s (AFLPs), DAF, Sequence Characterized Amplified Regions (SCARs), microsatellite or Simple Sequence Repeat markers (SSRs), Sequence Characterized Amplified Regions (SCARs), single-nucleotide polymorphisms (SNPs), KBioscience Competitive Allele-Specific PCR (KASPar), as inter alia described in Jonah et al. (Global Journal of Science Frontier Research 11:5, 2011) and Lateef (Journal of Biosciences and Medicines, 2015, 3, 7-18). 
     As used herein, the term “single nucleotide polymorphism” (SNP) may refer to a DNA sequence variation occurring when a single nucleotide in the genome (or other shared sequence) differs between members of a species or paired chromosomes in an individual. [0057] Within a population, SNPs can be assigned a minor allele frequency the lowest allele frequency at a locus that is observed in a particular population. This is simply the lesser of the two allele frequencies for single-nucleotide polymorphisms. There are variations between various populations, so a SNP allele that is common in one geographical group or variety may be much rarer in another. 
     Single nucleotide polymorphisms may fall within coding sequences of genes, non-coding regions of genes, or in the intergenic regions between genes. SNPs within a coding sequence will not necessarily change the amino acid sequence of the protein that is produced, due to degeneracy of the genetic code. A SNP in which both forms lead to the same polypeptide sequence is termed “synonymous” (sometimes referred to a silent mutation). If a different polypeptide sequence is produced, they are termed “non-synonymous.” A non-synonymous change may either be mis-sense or nonsense, where a mis-sense change results in a different amino acid and a nonsense change results in a premature stop codon. SNPs that are not in protein-coding regions may still have consequences for e.g. gene splicing, transcription factor binding, or the sequence of non-coding RNA (e.g. affecting transcript stability, translation). SNPs are usually biallelic and thus easily assayed in plants and animals. 
     A particularly useful assays for detection of SNP markers is for example KBioscience Competitive Allele-Specific PCR (KASP, see www.kpbioscience.co.uk), For developing the KASP-assay 70 base pairs upstream and 70 basepairs downstream of the SNP are selected and two allele-specific forward primers and one allele specific reverse primer is designed. See e.g. Allen et al. 2011, Plant Biotechnology J. 9, 1086-1099, especially p 1097-1098 for KASP assay method. 
     The terms “linked to” or “linkage”, as used herein, refers to a measurable probability that genes or markers located on a given chromosome are being passed on together to individuals in the next generation. Thus, the term “linked” may refer to one or more genes or markers that are passed together with a gene with a probability greater than 0.5 (which is expected from independent assortment where markers/genes are located on different chromosomes). Because the proximity of two genes or markers on a chromosome is directly related to the probability that the genes or markers will be passed together to individuals in the next generation, the term “linked” may also refer herein to one or more genes or markers that are located within about 50 centimorgan (cM) or less of one another on the same chromosome. Genetic linkage is usually expressed in terms of cM. Centimorgan is a unit of recombinant frequency for measuring genetic linkage, defined as that distance between genes or markers for which one product of meiosis in 100 is recombinant, or in other words, the centimorgan is equal to a 1% chance that a marker at one genetic locus on a chromosome will be separated from a marker at a second locus due to crossing over in a single generation. It is often used to infer distance along a chromosome. The number of basepairs to which cM correspond varies widely across the genome (different regions of a chromosome have different propensities towards crossover) and the species (i.e. the total size of the genome). 
     The presently described Rf locus on chromosome 1B was mapped to a segment at chromosome 1B, in an interval of about 15.8 cM, said interval being flanked by markers of SEQ ID NO 2 and SEQ ID NO 8. These and any marker located in between can be said to comprise an allele that is linked to functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B Thus, in this respect, the term linked can be a separation of about 15.8 cM, or less such as about 12.5 cm, about 10 cM, 7.5 cM, about 6 cM, about 5 cM, about 4 cM, about 3 cM, about 2.5 cM, about 2 cM, or even less. Particular examples of markers comprising an allele linked to the functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B are specified in table 1. The peak marker was the marker of SEQ ID NO. 6. 
     Further finemapping narrowed the 1B region to an interval of about 1.25 cM (from 6.8 to 8.05 cM), comprising the markers as represented by SEQ ID NO. 11, SEQ ID NO. 12, SEQ ID NO. 12 and SEQ ID NO. 14. These and any further marker located in said interval can be said to comprise an allele that is “tightly linked” to the functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B. Thus, the term “tightly linked” as used herein can be a separation of about 1.25 cM, or even less, such as about about, 1.0 cM, about 0.95 cM, about 0.9 cM, about 0.85 cM, about 0.8 cM, about 0.75 cM, about 0.5 cM, about 0.4 cM, about 0.3 cM, about 0.25 cM, about 0.20 cM, about 0.15 cM, about 0.10 cM, or even less. Particular examples of markers comprising an allele tightly linked to the functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B are given in table 2. The marker closest to the peak was SEQ ID NO. 13. 
     Furthermore, a G/C SNP was identified at a position corresponding to nucleotide position 429 of SEQ ID NO 16, where a G is present at nucleotide position 429 of SEQ ID NO: 16 and the corresponding C is present at nucleotide position 429 of SEQ ID NO. 18. 
     Thus, said at least one marker allele linked to said functional restorer gene allele located on chromosome 1B can be selected from any one of:
         a. a T at SEQ ID NO: 2;   b. a C at SEQ ID NO: 3;   c. a T at SEQ ID NO: 4;   d. a T at SEQ ID NO: 5;   e. an A at SEQ ID NO: 6;   f. an A at SEQ ID NO: 7;   g. a G at SEQ ID NO: 8;   h. a C at SEQ ID NO: 11;   i. an A at SEQ ID NO: 12,   j. a T at SEQ ID NO: 13;   k. a T at SEQ ID NO: 14,   l. a C at SEQ ID NO: 16/SEQ ID NO: 18
 
or any combination thereof.
       

     As used herein, “a T at SEQ ID NO: 2” or “a C at SEQ ID NO. 3” and the like, refers to a T or a C etc being present at a position corresponding to the position of the SNP in said SEQ ID NO, as e.g. indicated in table 1 or 2. This can for example be determined by alignment of the genomic sequence with said SEQ ID NO. Thus, “a T at SEQ ID NO: 2” means “a T at a position corresponding to position 51 of SEQ ID NO: 2”, etc. Likewise, whether e.g. C is present at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16 (or of SEQ ID NO. 18) can also be determined by alignment of SEQ ID NO. 16 or SEQ ID NO. 18, or a fragment thereof (such as a fragment of at least about 20 nt, such as about 20-100 nt, or of about 20-200 nt, comprising said C at the position corresponding to nucleotide position 429 of SEQ ID NO 16 or SEQ ID NO. 18) to the genomic sequence. 
     In a further embodiment, said at least one marker allele localises to an interval from 6.8 to 8.05 cM on chromosome 1B. Said 1.25 cM interval comprises the markers of SEQ ID NO. 11, SEQ ID NO. 12, SEQ ID NO. 13 and SEQ ID NO. 14 at the positions as indicated in table 2. Said interval also comprises a SNP marker at a position corresponding to nucleotide position 429 of SEQ ID NO: 16/SEQ ID NO. 18. 
     For example, said at least one marker allele linked to said functional restorer gene allele can be selected from any one of:
         a. a C at SEQ ID NO: 11;   b. an A at SEQ ID NO: 12,   c. a T at SEQ ID NO: 13;   d. a T at SEQ ID NO: 14,   e. a C at SEQ ID NO: 16/SEQ ID NO. 18,
 
or any combination thereof.
       

     In an even further embodiment, said at least one marker allele linked to said functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B localises to an interval of 0.95 cM (from 7.1 to 8.05 cM) on chromosome 1B flanked by and comprising the marker pair of SEQ ID NO. 11 and SEQ ID NO. 14. 
     In a particular embodiment, said at least one marker allele linked to said functional restorer gene allele is a T at SEQ ID NO. 13. 
     In a further embodiment, said at least one marker allele linked to said functional restorer gene allele is a C at SEQ ID NO. 16/SEQ ID NO. 18. 
     The term “interval” refers to a continuous linear span of chromosomal DNA with termini defined by map position and/or markers. For example, the interval comprising and flanked by the marker pair of SEQ ID NO: 11 and SEQ ID NO: 14. comprises the specifically mentioned flanking markers and the markers located in between, e.g. SEQ ID NO: 12 and 13 as listed in table 2 below. The interval comprising and flanked by the marker pair of SEQ ID NO: 2 and SEQ ID NO: 8 comprises the markers of SEQ ID NO: 3 to 7 as well as the markers of SEQ ID NO: 11-14, as well as the marker of SEQ ID NO. 16/18. Accordingly, a flanking marker as used herein, is a marker that defines one of the termini of an interval (and is included in that interval). It will be clear that any of such intervals may comprise further markers not specifically mentioned herein. 
     The position of the chromosomal segments identified, and the markers thereof, when expressed as recombination frequencies or map units, are provided herein as a matter of general information. The embodiments described herein were obtained using particular wheat populations. Accordingly, the positions of particular segments and markers as map units are expressed with reference to the used populations. It is expected that numbers given for particular segments and markers as map units may vary from cultivar to cultivar and are not part of the essential definition of the DNA segments and markers, which DNA segments and markers are otherwise described, for example, by nucleotide sequence. 
     A locus (plural loci), as used herein refers to a certain place or position on the genome, e.g. on a chromosome or chromosome arm, where for example a gene or genetic marker is found. A QTL (quantitative trait locus), as used herein, and refers to a position on the genome that corresponds to a measurable characteristic, i.e. a trait, such as the presently described Rf loci. 
     As used herein, the term “allele(s)”, such as of a gene, means any of one or more alternative forms of a gene at a particular locus. In a diploid cell of an organism, alleles of a given gene are located at a specific location or locus (loci plural) on a chromosome. One allele is present on each chromosome of the pair of homologous chromosomes or possibly on homeologous chromosomes. 
     As used herein, the term “homologous chromosomes” means chromosomes that contain information for the same biological features and contain the same genes at the same loci but possibly different alleles of those genes. Homologous chromosomes are chromosomes that pair during meiosis. “Non-homologous chromosomes”, representing all the biological features of an organism, form a set, and the number of sets in a cell is called ploidy. Diploid organisms contain two sets of non-homologous chromosomes, wherein each homologous chromosome is inherited from a different parent. In tetraploid species, two sets of diploid genomes exist, whereby the chromosomes of the two genomes are referred to as “homeologous chromosomes” (and similarly, the loci or genes of the two genomes are referred to as homeologous loci or genes). Likewise, hexaploid species have three sets of diploid genomes, etc. A diploid, tetraploid or hexaploid plant species may comprise a large number of different alleles at a particular locus. The ploidy levels of domesticated wheat species range from diploid ( Triticum monococcum,  2n=14, AA), tetraploid ( T. turgidum,  2n=28, AABB) to hexaploid ( T. aestivum,  2n=42, AABBDD). 
     As used herein, the term “heterozygous” means a genetic condition existing when two different alleles reside at a specific locus, but are positioned individually on corresponding pairs of homologous chromosomes in the cell. Conversely, as used herein, the term “homozygous” means a genetic condition existing when two identical alleles reside at a specific locus, but are positioned individually on corresponding pairs of homologous chromosomes in the cell. 
     An allele of a particular gene or locus can have a particular penetrance, i.e. it can be dominant, partially dominant, co-dominant, partially recessive or recessive. A dominant allele is a variant of a particular locus or gene that when present in heterozygous form in an organism results in the same phenotype as when present in homozygous form. A recessive allele on the other hand is a variant of an allele that in heterozygous form is overruled by the dominant allele thus resulting in the phenotype conferred by the dominant allele, while only in homozygous form leads to the recessive phenotype. Partially dominant, co-dominant or partially recessive refers to the situation where the heterozygote displays a phenotype that is an intermediate between the phenotype of an organism homozygous for the one allele and an organism homozygous for the other allele of a particular locus or gene. This intermediate phenotype is a demonstration of partial or incomplete dominance or penetrance. When partial dominance occurs, a range of phenotypes is usually observed among the offspring. The same applies to partially recessive alleles. 
     Cytoplasmic male-sterililty is caused by one or more mutations in the mitochondrial genome (termed “sterile cytoplasm”) and is inherited as a dominant, maternally transmitted trait. For cytoplasmic male sterility to be used in hybrid seed production, the seed parent must contain a sterile cytoplasm and the pollen parent must contain (nuclear) restorer genes (Rf genes) to restore the fertility of the hybrid plants grown from the hybrid seed. Accordingly, also such Rf genes preferably are at least partially dominant, most preferably dominant, in order to have sufficient restoring ability in offspring. 
     A chromosomal interval flanked by the above mentioned markers, are for example the markers as listed in Table 1-2 below between the specifically mentioned markers, or other markers that are not explicitly shown, but which are also flanked by the marker pairs mentioned. The skilled person can easily identify new markers in the genomic region or subgenomic region being flanked by any of the marker pairs listed above. Such markers need not to be SNP markers, but can be any type of genotypic or phenotypic marker mapped to that genomic or subgenomic region. Preferably such markers are genetically and physically linked to the presently described Rf loci as present in (and as derivable from) at least Accession number PI 583676 (USDA National Small Grains Collection), but preferably also as present in other cereals comprising the Rf 1B locus. In other words, the markers are preferably indicative of the presence of the Rf locus in a non-source specific manner. 
     In a further embodiment, at least two, three, four, or more marker alleles linked to said functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B can be used, such as, at least two, three, four, or more marker nucleic acids selected from any one of SEQ IN NO. 2, SEQ ID NO. 3, SEQ ID NO. 4, SEQ ID NO. 5, SEQ ID NO. 6, SEQ ID NO. 7, SEQ ID NO. 8, SEQ ID NO. 11, SEQ ID NO. 12, SEQ ID NO. 13, SEQ ID NO. 14, SEQ ID NO. 16/18. 
     In a further embodiment, at least two, three, four, or more contiguous marker alleles linked to said functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B may be used. A contiguous marker, as used herein is a nucleotide sequence located “upstream” or “downstream” of another marker, depending on whether the contiguous nucleotide sequence from the chromosome is on the 5′ or the 3′ side of the original marker, as conventionally understood, e.g. in the order as listed in table 1 or 2. 
     Integration of the fine map with partial genome sequences identified scaffold as represented by SEQ ID NO. 15 as harboring the functional restorer gene allele. Thus, in any of the herein described embodiments or aspects, the functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B may localize to the genome scaffold as represented by SEQ ID NO. 15. 
     A “contig”, as used herein refers to set of overlapping DNA segments that together represent a consensus region of DNA. In bottom-up sequencing projects, a contig refers to overlapping sequence data (reads); in top-down sequencing projects, contig refers to the overlapping clones that form a physical map of the genome that is used to guide sequencing and assembly. Contigs can thus refer both to overlapping DNA sequence and to overlapping physical segments (fragments) contained in clones depending on the context. 
     A “scaffold” as, used herein, refers to overlapping DNA contigs that together represent a consensus region of DNA. 
     In a further embodiment, said functional restorer gene allele is a functional allele of a gene encoding a pentatricopeptide repeat (PPR) protein (i.e. a PPR gene) localising within any of the above intervals or to said scaffold. 
     PPR proteins are classified based on their domain architecture. P-class PPR proteins possess the canonical 35 amino acid motif and normally lack additional domains. Members of this class have functions in most aspects of organelle gene expression. PLS-class PPR proteins have three different types of PPR motifs, which vary in length; P (35 amino acids), L (long, 35-36 amino acids) and S (short, ˜31 amino acids), and members of this class are thought to mainly function in RNA editing. Subtypes of the PLS class are categorized based on the additional C-terminal domains they possess (reviewed by Manna et al., 2015, Biochimie 113, p 93-99, incorporated herein by reference). 
     Most fertility restoration (Rf) genes come from a small clade of genes encoding pentatricopeptide repeat (PPR) proteins (Fuji et al., 2011, PNAS 108(4), 1723-1728—herein incorporated by reference). PPR genes functioning as fertility restoration (Rf) genes are referred to in Fuji (supra) as Rf-PPR genes. Rf-PPR genes are usually present in clusters of similar Rf-PPR-like genes, which show a number of characteristic features compared with other PPR genes. They are comprised primarily of tandem arrays of 15-20 PPR motifs, each composed of 35 amino acids. 
     Most Rf PPR genes belong to the P-class PPR subfamily, although also PLS-class PPR Rf genes have been identified, and are characterized by the presence of tandem arrays of 15 to 20 PPR motifs each composed of 35 amino acid residues. High substitution rates observed for particular amino acids within otherwise very conserved PPR motifs, indicating diversifying selection, prompted the conclusion that these residues might be directly involved in binding to RNA targets. This has led to the development of a “PPR code” which allows the prediction of RNA targets of naturally occurring PPR proteins as well as the design of synthetic PPR proteins that can bind RNA molecules of interest, whereby sequence specificity is ensured by distinct patterns of hydrogen bonding between each RNA base and the amino acid side chains at positions 5 and 35 in the aligned PPR motif (Melonek et al., 2016, Nat Sci Report 6:35152, Barkan et al., 2012, PLoS Genet 8(8): e1002910, both incorporated herein by reference). 
     Accordingly, a functional allele of a PPR gene, as used herein, refers to an allele of a PPR gene that is a functional restorer gene allele for wheat G-type cytoplasmic male sterility as described herein, i.e. that when expressed in a (sexually compatible) cereal plant has the capacity to restore fertility in the progeny of a cross with a G-type cytoplasmic male sterile cereal plant. Such a functional allele of a PPR gene is also referred to as a PPR-Rf gene (or Rf-PPR gene), which in turn encodes a PPR-Rf (or Rf-PPR) protein. 
     In one embodiment, said functional restorer gene allele encodes a polypeptide, such as a PPR protein that has the capacity to (specifically) bind to the CMS ORF256 (SEQ ID NO. 24). Bind to or specifically bind to or (specifically) recognize, as used herein, means that according to the above described PPR code, the PPR protein contains a number of PPR motifs with specific residues at positions 5 and 35 and which are ordered in such a way so as to be able to bind to a target mRNA, in this case the ORF256 mRNA, in a sequence-specific or sequence-preferential manner. 
     For example, the functional restorer gene allele can encode a PPR protein containing PPR motifs with specific residues at the above indicated positions so as to recognize the target sequence ATTTTGCACTTTTGTAT of ORF256 (nt 139-154 of SEQ ID NO. 24). In one example, the predicted recognition sequence can be AUUUKCASNCNYACGU (SEQ ID NO. 23). 
     The functional restorer gene allele can for example encode a PPR protein having a mutation (with respect to SEQ ID NO. 17) that affects mRNA or protein stablility, for example that increases mRNA or protein stability, thereby resulting in an increased expression of the PPR protein, especially during early pollen development and meisosis, such as in anther or, more specifically, tapetum, or developing microspore. 
     The functional restorer gene allele can also encode a PPR protein having a mutation (with respect to SEQ ID NO. 17) in an α-helical domain of an PPR motif, such as a mutation that affects hairpin formation between two of the α-helices making up a PPR motif. 
     The functional restorer gene allele can also encode a PPR protein having a mutation (with respect to SEQ ID NO. 17) that affects dimerization of the PPR protein. It has e.g. been found that ‘Thylakoid assembly 8’ (THA8) protein is a pentatricopeptide repeat (PPR) RNA-binding protein required for the splicing of the transcript of ycf3, a gene involved in chloroplast thylakoid-membrane biogenesis. THA8 forms an assymetic dimer once bound to single stranded RNA, with the bound RNA at the dimer interface. This dimer complex formation is mediated by the N-terminal PPR motifs 1 and 2 and the C-terminal motifs 4 and 5 (Ke et al., 2013, Nature Structural &amp; Molecular Biology, 20, 1377-1382). 
     In one embodiment, the functional restorer gene allele encodes a PPR protein having a mutation (with respect to SEQ ID NO. 17) in the 6 th  PPR motif (or in the 13 th  when counting from the C-terminus). 
     In a further embodiment, said functional restorer gene allele is a functional allele of the PPR gene encoded by the nucleic acid sequence of SEQ ID NO. 16, SEQ ID NO 20, SEQ ID NO 21, SEQ ID NO. 22, or the polypeptide sequence of SEQ ID NO. 17. For example, said functional restorer gene allele can comprise or encode a sequence that is substantially identical to SEQ ID NO. 16, SEQ ID NO. 17, SEQ ID NO. 18, SEQ ID NO 21, SEQ ID NO. 22, as defined herein, such as at least 85%, 85.5%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99% or 99.5% identical to SEQ ID NO. 16, SEQ ID NO. 17, SEQ ID NO. 18, SEQ ID NO 21, SEQ ID NO. 22. 
     In a further embodiment, said functional restorer gene allele is a functional restorer gene allele as present in (and as derivable from) at least Accession number PI 583676 (USDA National Small Grains Collection, also known as Dekalb 582M and registered as US PVP 7400045). 
     In a further embodiment, said functional restorer gene allele comprises a C at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16 or wherein said functional restorer gene allele comprises an I at the amino acid position corresponding to position 143 of SEQ ID NO. 17. 
     In an even further embodiment, said functional restorer gene allele comprises the nucleotide sequence of SEQ ID NO. 18, SEQ ID NO 20, SEQ ID NO 21, SEQ ID NO. 22 or encodes the polypeptide of SEQ ID NO. 19. 
     It will be clear that when reference herein is made to a certain SNP genotype or SNP allele (or marker genotype or marker allele) in a specific genomic sequence (selected e.g. from SEQ ID NO: 1 to SEQ ID NO: 14, or from SEQ ID NO. 16, SEQ ID NO. 18 or fragments thereof), this encompasses also the SNP genotype or allele in variants of the genomic sequence, i.e. the SNP genotype or allele in a genomic sequence that are homologous, e.g. comprising at least 90%, 95%, 98%, 99% (substantial) sequence identity or more to the sequence referred to (selected e.g. from SEQ ID NO: 1 to SEQ ID NO: 14, or to SEQ ID NO. 16, SEQ ID NO. 18 or fragments thereof). Thus any reference herein to any one of SEQ ID NO: 1 to 14 (and SEQ ID NO. 16, SEQ ID NO. 18 or fragments thereof) in one aspect also encompasses a variant of any one of SEQ ID NO: 1 to 14 (and SEQ ID NO. 16, SEQ ID NO. 18 or fragments thereof), said variant (homologous sequence) comprising at least 85%, 90%, 95%, 98%, 99% sequence identity or more to said sequence (using e.g. the program ‘Needle’), but comprising said SNP (marker) genotype or allele. 
     The SNP genotype refers to two nucleotides, and genomic sequences comprising one of these two nucleotides, one on each chromosome of the chromosome pair. So a plant having e.g. a AA genotype for SEQ ID NO. 6 has an identical nucleotide (A) on both chromosomes at the position corresponding to nucleotide 32 of SEQ ID NO: 6, while a plant having an AG genotype for SEQ ID NO. 6 has one chromosome with an A at the position corresponding to nucleotide 32 of SEQ ID NO: 6 and one chromosome with a G at said nucleotide position. Accordingly, a SNP allele refers to one of the two nucleotides of the SNP genotype as present on a chromosomes. 
     Based on the present disclosure, the skilled person can easily identify any further Rf specific marker or marker alleles as listed above. This can for example be done by sequencing genomic regions in-between any of the markers mentioned herein or by mapping new markers to a region in between any of the marker intervals or sub-intervals listed above. Preferably, but not necessarily, such markers are common markers, i.e. they are present on chromosome 1B of more than one Rf source. 
     The invention further describes a method for producing a cereal (e.g. wheat) plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility, comprising the steps of
         a. crossing a first cereal plant comprising a functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B, with a second plant (wherein said first plant comprises at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B as described herein, and hence is identifiable using the methods described herein)   b. identifying (and optionally selecting) a progeny plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B according to any of the methods described herein, by identifying a progeny plant comprising at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B as described herein (wherein said progeny plant comprises said functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B).       

     Also provided is a method for producing a cereal plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, comprising the steps of
         a. crossing a first cereal plant homozygous for a functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B with a second cereal plant (wherein said first cereal plant comprises at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B as described herein, preferably wherein said plant is homozygous for said at least one marker allele)   b. obtaining a progeny plant, wherein said progeny plant comprises a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B (wherein said progeny plant comprises at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B as described herein, and hence is identifiable using the methods described herein).       

     Said second plant can be a plant not comprising a functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B. 
     In an even further embodiment, the invention provides a method for producing F1 hybrid seeds or F1 hybrid plants, comprising the steps of:
         a. Providing a male cereal (e.g. wheat) parent plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B;   b. Crossing said male parent plant with a female cereal (e.g. wheat) parent plant, wherein the female parent plant is a G-type cytoplasmic male sterile cereal plant;   c. Optionally collecting hybrid seeds from said cross.       

     The F1 hybrid seeds and plants preferably comprise at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B as described herein, and the F1 plants grown from the seeds are therefore fertile. Preferably, the male parent plant is thus homozygous for said a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B and hence is also homozygous for said at least one marker allele. 
     In the above method, the male parent plant used for crossing can be selected using any of the herein described methods for selecting a cereal plant comprising a functional restorer gene for wheat G-type cytoplasmic male sterility. Accordingly, the male parent plant comprises at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, preferably in homozygous form. 
     The invention also provides cereal plants, such as wheat plants, obtained by any of the above methods, said cereal plant comprising at least one marker allele linked to the functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B. 
     Said at least one marker allele linked to the functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B may localize to the same chromosomal intervals or contigs and can be selected from the same groups as described above for the other embodiments and aspect. 
     Also described is a cereal plant, plant part, plant cell or seed comprising at least one functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, said plant comprising at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, wherein said at least one marker allele localises within an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 2 and SEQ ID NO 8, preferably wherein said plant comprises at least one of (such as one, two, three, four five, six, seven, eight, nine, ten or all of):
         a. a T at SEQ ID NO: 2;   b. a C at SEQ ID NO: 3;   c. a T at SEQ ID NO: 4;   d. a T at SEQ ID NO: 5;   e. an A at SEQ ID NO: 6;   f. an A at SEQ ID NO: 7;   g. a G at SEQ ID NO: 8;   h. a C at SEQ ID NO: 11;   i. an A at SEQ ID NO: 12,   j. a T at SEQ ID NO: 13;   k. a T at SEQ ID NO: 14,   l. a C at SEQ ID NO: 16/SEQ ID NO. 18       

     said plant not comprising any one or all of
         m. an A at SEQ ID NO: 1;   n. a T at SEQ ID NO: 9.       

     Also described is cereal plant, plant part, plant cell or seed comprising at least one functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, said plant comprising at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, wherein said at least one marker allele localises within an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 11 and SEQ ID NO 14, preferably wherein said plant comprises at least one of (such as one, two, three or all of):
         a. a C at SEQ ID NO: 11;   b. an A at SEQ ID NO: 12,   c. a T at SEQ ID NO: 13;   d. a T at SEQ ID NO: 14,   e. a C at SEQ ID NO: 16/SEQ ID NO. 18
 
said plant not comprising any one or all of
   f. a T at SEQ ID NO: 2;   g. an A at SEQ ID NO: 8.       

     Also described are a cereal plant, plant part, plant cell or seed comprising at least one functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, said plant comprising at least one marker allele linked to a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B wherein said at least one marker allele localises within an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 11 and SEQ ID NO 14, preferably wherein said plant comprises at least one of (such as one, two, three or all of):
         a. a C at SEQ ID NO: 11;   b. an A at SEQ ID NO: 12,   c. a T at SEQ ID NO: 13;   d. a T at SEQ ID NO: 14,   e. a C at SEQ ID NO: 16/SEQ ID NO. 18       

     said plant not comprising any one or all of
         f. a T at SEQ ID NO: 10;   g. a T at SEQ ID NO: 5.       

     In a further embodiment, any of the above plants plant part, plant cell or seeds comprises a T at SEQ ID NO. 13. In a further embodiment, said plant comprising a T at SEQ ID NO 13, does not comprise any one or all of: a C at SEQ ID NO: 11; an A at SEQ ID NO: 12; a T at SEQ ID NO: 14. 
     Any of the above plants, plant part, plant cell or seeds may also comprise a C at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16/SEQ ID NO. 18. In particular, the invention provides a plant comprising a C at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16/18, said plant not comprising any one or all of a C at SEQ ID NO: 11, an A at SEQ ID NO: 12, a T at SEQ ID NO: 13, a T at SEQ ID NO: 14. 
     Also provided are plant parts, plant cells and seed from the cereal plants according to the invention comprising said at least one marker allele and said functional restorer gene allele. The plants, plant parts, plant cells and seeds of the invention may also be hybrid plants, plant parts, plant cells or seeds. 
     Also provided is a method to determine the presence or absence or zygosity status of a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B in a biological sample of a cereal plant, comprising providing genomic DNA from said biological sample, and analysing said DNA for the presence or absence or zygosity status of at least one marker allele linked to a functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B a described herein. It will be clear that the presence can be determined using a marker allele linked to the functional restorer gene as described herein, whereas the absence can (additionally) be determined by detecting the presence of the other, non-restoring allele. The zygosity status, i.e. whether the plant is homozygous for the restorer allele, homozygous for the non-restorer allele or heterozygous (i.e. the Rf genotype), can be determined by detecting the presence or absence of a marker allele linked to the functional restorer gene and by detecting the presence of the other, non-restoring allele, but depending on the parental origin it can also be sufficient to determine the presence or absence of only one of the alleles to be able to deduce the complete genotype (zygosity status) of the plant. 
     Also provided is a method for the identification and/or selection of a cereal (e.g. wheat) plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility comprising the steps of
         a. Identifying or detecting in said plant the presence of a C at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16/18; or   b. and optionally selecting said plant having a C at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16/18.       

     Also provided is a method for the identification and/or selection of a cereal (e.g. wheat) plant comprising a functional restorer gene allele for wheat G-type cytoplasmic male sterility comprising the steps of
         a. Identifying or detecting in said plant the presence of the nucleic acid or the polypeptide encoding a functional restorer gene for wheat G-type cytoplasmic male sterility as described herein   b. and optionally selecting said plant comprising said nucleic acid or polypeptide.       

     Likewise, identifying or detecting can involve obtaining a biological sample (e.g. protein) or genomic DNA and determining the presence of the nucleic acid or polypeptide according to methods well known in the art, such as hybridization, PCR, Rt-PCR, Southern blotting, Southern-by-sequencing, SNP detection methods (e.g. as described herein), western blotting, elisa etc, e.g. based on the sequences provided herein. 
     The invention also provides the use of at least one marker comprising an allele linked to the functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B for the identification of at least one further marker comprising an allele linked to said functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B. Such markers are also genetically linked or tightly linked to the restorer gene, and are also within the scope of the invention. Markers can be identified by any of a variety of genetic or physical mapping techniques. Methods of determining whether markers are genetically linked to a restore gene are known to those of skill in the art and include, for example, interval mapping (Lander and Botstein, (1989) Genetics 121:185), regression mapping (Haley and Knott, (1992) Heredity 69:315) or MQM mapping (Jansen, (1994) Genetics 138:871), rMQM mapping. In addition, such physical mapping techniques as chromosome walking, contig mapping and assembly, amplicon resequencing, transcriptome sequencing, targeted capture and sequencing, next generation sequencing and the like, can be employed to identify and isolate additional sequences useful as markers in the context of the present invention. 
     The invention further provides the use of at least one marker allele linked to a functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B as described herein for the identification of a plant a comprising said functional restorer gene for wheat G-type cytoplasmic male sterility. 
     Also provided is the use of a plant obtained by any of the methods as described herein and comprising at least one marker allele linked to a functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B as described herein, for restoring fertility in a progeny of a G-type cytoplasmic male sterile cereal plant, such as a wheat plant, or for producing a population of hybrid cereal plants, such as a wheat plants or for producing hybrid seed. 
     Further provided is a method for identifying a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B, comprising the steps of
         a. Providing a population of F2 plants resulting from selfing of a population of F1 plants obtained by crossing a female cereal parent plant with a male cereal parent plant, wherein the female parent plant is a G-type cytoplasmic male sterile cereal plant, and wherein the male parent plant comprises a functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B.   b. Classifying the fertility of a plurality of said F2 plants.   c. Determining the nucleotide sequence of at least part of the region of chromosome 1B comprising and flanked by the markers of SEQ ID NO 2 and SEQ ID NO 8 of genomic DNA isolated from each of said plurality of F2 plants.   d. Identifying the coding sequence within said region having the highest association to the phenotype of restored fertility, wherein the identified coding sequence is the functional restorer gene allele for wheat G-type cytoplasmic male sterility located on chromosome 1B.       

     In any of the above described methods or uses, the markers and marker alleles can localize to the same chromosomal intervals and can be selected from the same groups as described above for the other embodiments and aspect. 
     Also provided are any of the markers comprising an allele linked to the functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B, as described herein. 
     Also provided herein is a chromosome fragment, which comprises a functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B, as described throughout the specification. In one aspect the chromosome fragment is isolated from its natural environment. In another aspect it is in a plant cell, especially in a cereal cell, especially in a wheat cell. Also an isolated part of the chromosome fragment comprising the functional restorer gene for wheat G-type cytoplasmic male sterility located on chromosome 1B is provided herein. Such a chromosome fragment can for example be a contig or a scaffold, such as corresponding to SEQ ID NO. 16. 
     Further provided is a recombinant nucleic acid molecule, especially a recombinant DNA molecule, which comprises a functional restorer gene according to the invention. In one aspect the functional restorer gene is detectable by one or more of the molecular marker assays described herein. Also a DNA vector is provided comprising the recombinant DNA. The recombinant DNA molecule or DNA vector may be an isolated nucleic acid molecule. The DNA comprising the functional restorer gene may be in a microorganism, such as a bacterium (e.g.  Agrobacterium  or  E. coli ). 
     Thus, in one embodiment, the invention provides an (isolated) nucleic acid molecule encoding a functional restorer gene allele for wheat G-type cytoplasmic male sterility, wherein said functional restorer gene allele localises within an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 2 and SEQ ID NO 8. Thus, the (isolated) nucleic acid molecule encodes or comprises a functional restorer gene allele for wheat G-type cytoplasmic male sterility that is derivable or derived from an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 2 and SEQ ID NO 8. Said functional restorer gene allele can be identified and hence is identifiable using any of the markers and marker alleles linked to said functional restorer gene allele as described herein. 
     In a further embodiment, said functional restorer gene allele encoded by said (isolated) nucleic acid molecule localizes within an interval on chromosome 1B comprising and flanked by the markers of SEQ ID NO 11 and SEQ ID NO 14. 
     In a further embodiment, said functional restorer gene allele encoded by said (isolated) nucleic acid molecule localizes to the contig as represented by SEQ ID NO 15. 
     In a further embodiment, said functional restorer gene allele encoded by said (isolated) nucleic acid molecule can be a functional allele of a PPR gene localising within any of said intervals or to said contig. 
     In one embodiment, said (isolated) nucleic acid encoding said functional restorer gene allele encodes a(n) (isolated) polypeptide, such as a PPR protein, that has the capacity to (specifically) bind to the CMS ORF256 (SEQ ID NO. 24). Bind to or specifically bind to or (specifically) recognize, as used herein, means that according to the above described PPR code, the PPR protein contains a number of PPR motifs with specific residues at positions 5 and 35 and which are ordered in such a way so as to be able to bind to a target mRNA, in this case the ORF256 mRNA, in a sequence-specific or sequence-preferential manner. 
     For example, the functional restorer gene allele can encode a(n) (isolated) PPR protein containing PPR motifs with specific residues at the above indicated positions so as to recognize the target sequence ATTTTGCACTTTTGTAT of ORF256 (nt 139-154 of SEQ ID NO. 24). In one example, the predicted recognition sequence can be AUUUKCASNCNYACGU (SEQ ID NO. 23). 
     The functional restorer gene allele can for example have a mutation (with respect to SEQ ID NO. 16 or) that affects mRNA stability or can encode a PPR protein having a mutation (with respect to SEQ ID NO. 17, 20 or 21) that affects protein stability, for example that increases mRNA or protein stability (or prevents degradation), thereby resulting in an increased expression of the PPR protein, especially during early pollen development and meiosis, such as in anther or, more specifically, tapetum, or developing microspore. 
     The functional restorer gene allele can also encode a PPR protein having a mutation (with respect to SEQ ID NO. 17) in an α-helical domain of a PPR motif, such as a mutation that affects hairpin formation between two of the α-helices making up a PPR motif. 
     The functional restorer gene allele can also encode a PPR protein having a mutation (with respect to SEQ ID NO. 17) that affects dimerization of the PPR protein. It has e.g. been found that ‘Thylakoid assembly 8’ (THA8) protein is a pentatricopeptide repeat (PPR) RNA-binding protein required for the splicing of the transcript of ycf3, a gene involved in chloroplast thylakoid-membrane biogenesis. THA8 forms an asymmetric dimer once bound to single stranded RNA, with the bound RNA at the dimer interface. This dimer complex formation is mediated by the N-terminal PPR motifs 1 and 2 and the C-terminal motifs 4 and 5 (Ke et al., 2013, Nature Structural &amp; Molecular Biology, 20, 1377-1382). 
     In one embodiment, the functional restorer gene allele encodes a PPR protein having a mutation (with respect to SEQ ID NO. 17) in the 13 th  PPR motif when counting from the C-terminus). 
     The functional restorer gene allele can also encode a PPR protein which when expressed is targeted to the mitochondrion. This can e.g. be accomplished by the presence of a (plant-functional) mitochondrial targeting sequence or mitochondrial signal peptide, or mitochondrial transit peptide. A mitochondrial targeting signal is a 10-70 amino acid long peptide that directs a newly synthesized protein to the mitochondria, typically found at the N-terminus. Mitochondrial transit peptides are rich in positively charged amino acids but usually lack negative charges. They have the potential to form amphipathic α-helices in nonaqueous environments, such as membranes. Mitochondrial targeting signals can contain additional signals that subsequently target the protein to different regions of the mitochondria, such as the mitochondrial matrix. Like signal peptides, mitochondrial targeting signals are cleaved once targeting is complete. Mitochondrial Transit peptides are e.g. described in Shewry and Gutteridge (1992, Plant Protein Engineering, 143-146, and references therein), Sjoling and Glaser (Trends Plant Sci Volume 3, Issue 4, 1 Apr. 1998, Pages 136-140), Pfanner (2000, Current Biol, Volume 10, Issue 11), Huang et al (2009, Plant Phys 150(3): 1272-1285), Chen et al. (1996, PNAS, Vol. 93, pp. 11763-11768), Fuji et al. (Plant J 2016). 
     In a further embodiment, said functional restorer gene allele is a functional allele of the PPR gene encoded by the nucleic acid sequence of SEQ ID NO. 16, SEQ ID NO 20, SEQ ID NO 21, SEQ ID NO. 22, or the polypeptide sequence of SEQ ID NO. 17. For example, said functional restorer gene allele can comprise or encode a sequence that is substantially identical to SEQ ID NO. 16, SEQ ID NO. 17, SEQ ID NO. 18, SEQ ID NO. 19, SEQ ID NO 21, SEQ ID NO. 22, as defined herein, such as at least 85%, 85.5%, 86%, 87%, 88%, 89%, 90%, 91%, 92%, 93%, 94%, 95%, 96%, 97%, 98%, 99% or 99.5% identical to SEQ ID NO. 16, SEQ ID NO. 17, SEQ ID NO. 18, SEQ ID NO. 19, SEQ ID NO 21, SEQ ID NO. 22. 
     In a further embodiment, said functional restorer gene allele encoded by said (isolated) nucleic acid molecule is a functional allele of a PPR gene encoded by SEQ ID NO. 16 or a PPR gene encoding the polypeptide of SEQ ID NO. 17. 
     In a further embodiment, said functional restorer gene allele encoded by said (isolated) nucleic acid molecule comprises a C at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16 or wherein said functional restorer gene allele comprises an I at the amino acid position corresponding to position 143 of SEQ ID NO. 17. 
     In an even further embodiment, said functional restorer gene allele encoded by said (isolated) nucleic acid molecule comprises the nucleotide sequence of SEQ ID NO. 18 or encodes the polypeptide of SEQ ID NO. 19. 
     In an even further embodiment, said functional restorer gene allele comprises the nucleotide sequence of SEQ ID NO. 18, SEQ ID NO 20, SEQ ID NO 21, SEQ ID NO. 22 or encodes the polypeptide of SEQ ID NO. 19. 
     In a further embodiment, said functional restorer gene allele encoded by said (isolated) nucleic acid molecule is obtainable from USDA accession number PI 583676. 
     Also provided is a(n) (isolated) polypeptide encoded by the nucleic acid molecule as described above (said polypeptide encoding a functional restorer protein for wheat G-type cytoplasmic male sterility). 
     The functional restorer gene allele may also be cloned and a chimeric gene may be made, e.g. by operably linking a plant expressible promoter to the functional restorer gene allele and optionally a 3′ end region involved in transcription termination and polyadenylation functional in plants. Such a chimeric gene may be introduced into a plant cell, and the plant cell may be regenerated into a whole plant to produce a transgenic plant. In one aspect the transgenic plant is a cereal plant, such as a wheat plant, according to any method well known in the art. 
     Thus, in a particular embodiment a chimeric gene is provided comprising a(n) (isolated) nucleic acid molecule encoding the functional restorer gene allele as described above, operably linked to a heterologous plant-expressible promoter and optionally a 3′ termination and polyadenylation region. 
     The use of such a (isolated or extracted) nucleic acid molecule and/or of such a chimeric gene and/or of such a chromosome fragment for generating plant cells and plants comprising a functional restorer gene allele is encompassed herein. In one aspect it may be used to generate transgenic cereal (e.g. wheat) cells, plants and plant parts or seeds comprising the functional restorer gene allele and the plant having the capacity to restore fertility against wheat G-type cytoplasmic male sterility as described above. 
     A host or host cell, such as a (cereal_plant cell or (cereal) plant or seed thereof, such as a wheat plant cell or plant or seed thereof, comprising the (isolated) nucleic acid molecule, (isolated) polypeptide, or the chimeric gene as described above is provided, wherein preferably said polypeptide, said nucleic acid, or said chimeric gene in each case is heterologous with respect to said plant cell or plant or seed. The host cell can e.g also be a bacterium, such as  E. coli  or  Agrobacterium  ( tumefaciens ). 
     Thus, also provided is a method for producing a cereal plant cell or plant or seed thereof, such as a wheat plant cell or plant or seed thereof, comprising a functional restorer gene for wheat G-type cytoplasmic male sterility, or for increasing restoration capacity for wheat G-type cytoplasmic male sterility (“CMS”) in a cereal plant, such as a wheat plant, comprising the steps of providing said plant cell or plant with the (recombinant) chromosome fragment or the (isolated) nucleic acid molecule or the chimeric gene as described herein wherein said providing comprises transformation, crossing, backcrossing, genome editing or mutagenesis. Restoration capacity, as used herein, means the capacity of a plant to restore fertility in the progeny of a cross with a G-type cytoplasmic male sterility (“CMS”) line. Preferably, said plant expresses or has increased expression of the polypeptide according to the invention. Preferably, said (increase in) expression is at least during (the early phases of) pollen development and meiosis, such as in anther or, more specifically, tapetum, or developing microspores (where said plant did not express or to a lesser extent expressed the polypeptide prior to the providing step). 
     Thus, also provided is a method for producing a cereal plant cell or plant or seed thereof, such as a wheat plant cell or plant or seed thereof, comprising a functional restorer gene for wheat G-type cytoplasmic male sterility, or for increasing restoration capacity for wheat G-type cytoplasmic male sterility (“CMS”) in a cereal plant, such as a wheat plant, comprising the steps of increasing the expression of the (isolated) polypeptide as described herein in said plant cell or plant or seed. Preferably, said (increase in) expression is at least during (the early phases of) pollen development and meiosis, such as in anther or, more specifically, tapetum, or developing microspores. Prior to the providing step said plant did not express or to a lesser extent expressed the polypeptide and/or did not have or to a lesser extent had restoration capacity for wheat G-type cytoplasmic male sterility (“CMS”)). 
     Increasing the expression can be done by providing the plant with the (recombinant) chromosome fragment or the (isolated) nucleic acid molecule or the chimeric gene as described herein, whereby the nucleic acid encoding the functional restorer gene allele is under the control of appropriate regulatory elements such as a promoter driving expression in the desired tissues/cells, but also by providing the plant with transcription factors that e.g. (specifically) recognise the promoter region and promote transcription, such as TALeffectors, dCas, dCpf1 etc coupled to transcriptional enhancers. 
     Further described is a method for converting a cereal plant, such as a wheat plant, not having the capacity to restore fertility in the progeny of a cross with a G-type cytoplasmic male sterility (“CMS”) line (a non-restorer plant) into a plant having the capacity to restore fertility in the progeny of a cross with a G-type cytoplasmic male sterility (“CMS”) line (a restorer plant), comprising the steps of modifying the genome of said plant to comprise the (isolated) nucleic acid molecule or the chimeric gene encoding a functional restorer gene allele for wheat G-type cytoplasmic male sterility as described herein wherein said modifying comprises transformation, crossing, backcrossing, genome editing or mutagenesis. Preferably, said plant expresses the polypeptide according to the invention, particularly at least during (the early phases of) pollen development and meiosis, such as in anther or, more specifically, tapetum, or developing microspores. Prior to said modification said plant did not express or to a lesser extent expressed the polypeptide and/or did not have or to a lesser extent had restoration capacity for wheat G-type cytoplasmic male sterility (“CMS”)). 
     Thus, also provided is a method for converting a non-restoring cereal plant, such as a wheat plant, into a restoring plant for wheat G-type cytoplasmic male sterility (“CMS”), or for increasing restoration capacity for wheat G-type cytoplasmic male sterility (“CMS”) in a cereal plant, such as a wheat plant, comprising the steps of modifying the genome of said plant to increase the expression of a polypeptide according to the invention in said plant. Preferably, said (increase in) expression is at least during (the early phases of) pollen development and meiosis, such as in anther or, more specifically, tapetum, or developing microspores. Prior to said modification said plant did not express or to a lesser extent expressed the polypeptide and/or did not have or to a lesser extent had restoration capacity for wheat G-type cytoplasmic male sterility (“CMS”)). 
     Modifying the genome to increase expression of the polypeptide can for example be done by modifying the native promoter to include regulatory elements that increase transcription, such as certain enhancer element, but also by inactivating or removing certain negative regulatory elements, such as repressor elements or target sites for miRNAs or lncRNAs. The Rf3 5′/upstream region including the promoter is included in SEQ ID NO 22, e.g. as represented by nt 8357-12518 or fragments thereof. 
     Also described is a plant cell or plant, preferably a cereal plant cell or cereal plant or seed thereof, such as a wheat plant cell or plant or seed thereof, produced according to any of the above methods, preferably wherein said plant has an increased restoration capacity for wheat G-type cytoplasmic male sterility (“CMS”) compared to said plant prior to the providing step or the modification step. Use of such a plant obtained according to the above methods to restore fertility in the progeny of a cross with a G-type cytoplasmic male sterility (“CMS”) plant or to produce hybrid plants or hybrid seed is also described. Such a plant cell, plant or seed can be a hybrid plant cell, plant or seed. 
     Genome editing, as used herein, refers to the targeted modification of genomic DNA using sequence-specific enzymes (such as endonuclease, nickases, base conversion enzymes) and/or donor nucleic acids (e.g. dsDNA, oligo&#39;s) to introduce desired changes in the DNA. Sequence-specific nucleases that can be programmed to recognize specific DNA sequences include meganucleases (MGNs), zinc-finger nucleases (ZFNs), TAL-effector nucleases (TALENs) and RNA-guided or DNA-guided nucleases such as Cas9, Cpf1, CasX, CasY, C2c1, C2c3, certain argonout systems (see e.g. Osakabe and Osakabe, Plant Cell Physiol. 2015 March; 56(3):389-400; Ma et al., Mol Plant. 2016 Jul. 6; 9(7):961-74; Bortesie et al., Plant Biotech J, 2016, 14; Murovec et al., Plant Biotechnol J. 2017 Apr. 1; Nakade et al., Bioengineered 8-3, 2017; Burstein et al., Nature 542, 37-241; Komor et al., Nature 533, 420-424, 2016; all incorporated herein by reference). Donor nucleic acids can be used as a template for repair of the DNA break induced by a sequence specific nuclease, but can also be used as such for gene targeting (without DNA break induction) to introduce a desired change into the genomic DNA. 
     Accordingly, using these technologies, plants lacking a functional restorer gene for wheat G-type cytoplasmic male sterility (non-restoring plants) can be converted to restoring plants by making the desired changes to existing PPR genes or alternatively to introduce one or more complete sequences encoding functional PPR Rf proteins, e.g. as described herein, at a specific genomic location. 
     Mutagenesis as used herein, refers to e.g. EMS mutagenesis or radiation induced mutagenesis and the like. 
     Thus, transgenic cereal cells, e.g. transgenic wheat cells, comprising in their genome a recombinant chromosome fragment as described or an (isolated) nucleic acid molecule as described or a chimeric gene as described comprising a functional restorer gene allele as described are also an embodiment of the invention. In one aspect the DNA molecule comprising Rf allele is stably integrated into the cereal (e.g. wheat) genome. 
     Thus, cereal plants, plant parts, plant cells, or seeds thereof, especially wheat, comprising a chromosome fragment or a nucleic acid molecule according to the invention or a polypeptide according to the invention or a chimeric gene according to the invention encoding a functional restorer gene according to the invention, are provided, said plant having the capacity to restore fertility against wheat G-type cytoplasmic male sterility are provided herein. In one embodiment, the chromosome fragment, nucleic acid molecule, polypeptide or chimeric gene is heterologous to the plant, such as transgenic cereal plants or transgenic wheat plants. This also includes plant cells or cell cultures comprising such a chromosome fragment or nucleic acid molecule, polypeptide or chimeric gene, independent whether introduced by transgenic methods or by breeding methods. The cells are e.g. in vitro and are regenerable into plants comprising the chromosome fragment or chimeric gene of the invention. Said plants, plant parts, plant cells and seeds may also be hybrid plants, plant parts, plant cells or seeds. 
     Such plants may also be used as male parent plant in a method for producing F1 hybrid seeds or F1 hybrid plants, as described above. 
     A plant-expressible promoter as used herein can be any promoter that drives sufficient expression at least during (early) pollen development and meiosis, such as in anther or, more specifically, tapetum, or developing microspore. This can for example be a constitutive promoter, an inducible promoter, but also a pollen-, anther- or, more specifically tapetum- or microspore-specific/preferential promoter. 
     A constitutive promoter is a promoter capable of directing high levels of expression in most cell types (in a spatio-temporal independent manner). Examples of plant expressible constitutive promoters include promoters of bacterial origin, such as the octopine synthase (OCS) and nopaline synthase (NOS) promoters from  Agrobacterium , but also promoters of viral origin, such as that of the cauliflower mosaic virus (CaMV) 35S transcript (Hapster et al., 1988, Mol. Gen. Genet. 212: 182-190) or 19S RNAs genes (Odell et al., 1985, Nature. 6; 313(6005):810-2; U.S. Pat. No. 5,352,605; WO 84/02913; Benfey et al., 1989, EMBO J. 8:2195-2202), the enhanced 2×35S promoter (Kay at al., 1987, Science 236:1299-1302; Datla et al. (1993), Plant Sci 94:139-149) promoters of the cassava vein mosaic virus (CsVMV; WO 97/48819, U.S. Pat. No. 7,053,205), 2×CsVMV (WO2004/053135) the circovirus (AU 689 311) promoter, the sugarcane bacilliform badnavirus (ScBV) promoter (Samac et al., 2004, Transgenic Res. 13(4):349-61), the figwort mosaic virus (FMV) promoter (Sanger et al., 1990, Plant Mol Biol. 14(3):433-43), the subterranean clover virus promoter No 4 or No 7 (WO 96/06932) and the enhanced 35S promoter as described in U.S. Pat. Nos. 5,164,316, 5,196,525, 5,322,938, 5,359,142 and 5,424,200. Among the promoters of plant origin, mention will be made of the promoters of the plant ribulose-biscarboxylase/oxygenase (Rubisco) small subunit promoter (U.S. Pat. No. 4,962,028; WO99/25842) from  zea mays  and sunflower, the promoter of the  Arabidopsis thaliana  histone H4 gene (Chaboute et al., 1987), the ubiquitin promoters (Holtorf et al., 1995, Plant Mol. Biol. 29:637-649, U.S. Pat. No. 5,510,474) of Maize, Rice and sugarcane, the Rice actin 1 promoter (Act-1, U.S. Pat. No. 5,641,876), the histone promoters as described in EP 0 507 698 A1, the Maize alcohol dehydrogenase 1 promoter (Adh-1) (from http://www.patentlens.net/daisy/promoters/242.html)). Also the small subunit promoter from  Chrysanthemum  may be used if that use is combined with the use of the respective terminator (Outchkourov et al., Planta, 216: 1003-1012, 2003). 
     Pollen/microspore-active promoters include e.g. a maize pollen specific promoter (see, e.g., Guerrero (1990) Mol. Gen. Genet. 224:161 168), PTA29, PTA26 and PTAI 3 (e.g., see U.S. Pat. No. 5,792,929) and as described in e.g. Baerson et al. (1994 Plant Mol. Biol. 26: 1947-1959), the NMT19 microspore-specific promoter as e.g. described in WO97/30166. Further anther/pollen-specific or anther/pollen-active promoters are described in e.g. Khurana et al., 2012 (Critical Reviews in Plant Sciences, 31: 359-390), WO2005100575, WO 2008037436. Other suitable promoters are e.g the barley vrnl promoter, such as described in Alonso-Peral et al. (2001, PLoS One. 2011; 6(12):e29456). 
     It will be clear that the herein identified nucleic acids and polypeptides encoding functional restorer genes can be used to identify further functional restorer genes for wheat G-type cytoplasmic male sterility. Thus, the invention also provides the use of the (isolated) nucleic acids or polypeptides as disclosed herein, such as SEQ ID NO. 16 or 17, to identify one or more further functional restorer genes for wheat G-type cytoplasmic male sterility. 
     Further, homologous or substantially identical functional restorer genes can be identified using methods known in the art. Homologous nucleotide sequence may be identified and isolated by hybridization under stringent or high stringent conditions using as probes a nucleic acid comprising e.g. the nucleotide sequence of SEQ ID NO: 16 or part thereof, as described above. Other sequences encoding functional restorer genes may also be obtained by DNA amplification using oligonucleotides specific for genes encoding functional restorer genes as primers, such as but not limited to oligonucleotides comprising or consisting of about 20 to about 50 consecutive nucleotides from SEQ ID NO: 16 or its complement. Homologous or substantially identical functional restorer genes can be identified in silico using Basic Local Alignment Search Tool (BLAST) homology search with the nucleotide or amino acid sequences as provided herein. 
     Functionality of restorer genes or alleles thereof, such as identified as above, can be validated for example by providing, e.g. by transformation or crossing, such a restorer gene under control of a plant-expressible promoter in a cereal (wheat) plant that does not have the capacity to restore fertility of offspring of a G-type cytoplasmic male sterile wheat plant, crossing the thus generated cereal plant with a G-type cytoplasmic male sterile wheat plant and evaluating seed set in the progeny. Alternatively, a restorer line can be transformed with an RNAi construct or gene-edited with e.g. CRISPR-Cas technology or any other sequence specific nuclease so to generate a loss of function that renders the plant non-restoring. Similarly, other means for mutating the restorer gene (e.g. EMS, g-radiation) can be used to evaluate the effect of a loss of function mutation on restoring ability. 
     In any of the herein described embodiments and aspects the plant may comprise or may be selected to comprise or may be provided with a further functional restorer gene for wheat G-type cytoplasmic male sterility (located on or obtainable from the same or another chromosome), such as Rf1 (1A), Rf2 (7D), Rf4 (6B), Rf5 (6D), Rf6 (5D), Rf7 (7B), Rf8, 6AS or 6BS (Tahir &amp; Tsunewaki, 1969; Yen et al., 1969; Bahl &amp; Maan, 1973; Du et al., 1991; Sihna et al., 2013; Ma et al., 1991; Zhou et al., 2005). 
     Any of the herein described methods, markers and marker alleles, nucleic acids, polypeptides, chimeric genes, plants etc may also be used to restore fertility against S v -type cytoplasm, as e.g. described in Ahmed et al 2001 (supra). 
     As used herein a “chimeric gene” refers to a nucleic acid construct which is not normally found in a plant species. A chimeric nucleic acid construct can be DNA or RNA. “Chimeric DNA construct” and “chimeric gene” are used interchangeably to denote a gene in which the promoter or one or more other regulatory regions, such as the a transcription termination and polyadenylation region of the gene are not associated in nature with part or all of the transcribed DNA region, or a gene which is present in a locus in the plant genome in which it does not occur naturally or present in a plant in which it does not naturally occur. In other words, the gene and the operably-linked regulatory region or the gene and the genomic locus or the gene and the plant are heterologous with respect to each other, i.e. they do not naturally occur together. 
     A first nucleotide sequence is “operably linked” with a second nucleic acid sequence when the first nucleic acid sequence is in a functional relationship with the second nucleic acid sequence. For example, a promoter is operably linked to a coding sequence if the promoter affects the transcription or expression of the coding sequence. When recombinantly produced, operably linked nucleic acid sequences are generally contiguous, and, where necessary to join two protein-coding regions, in the same reading frame (e.g., in a polycistronic ORF). However, nucleic acids need not be contiguous to be operably linked. 
     “Backcrossing” refers to a breeding method by which a (single) trait, such as fertility restoration (Rf), can be transferred from one genetic background (a “donor”) into another genetic background (also referred to as “recurrent parent”), e.g. a plant not comprising such an Rf gene or locus. An offspring of a cross (e.g. an F1 plant obtained by crossing an Rf containing with an Rf lacking plant; or an F2 plant or F3 plant, etc., obtained from selfing the F1) is “backcrossed” to the parent. After repeated backcrossing (BC1, BC2, etc.) and optionally selfings (BC1S1, BC2S1, etc.), the trait of the one genetic background is incorporated into the other genetic background. 
     “Marker assisted selection” or “MAS” is a process of using the presence of molecular markers, which are genetically linked to a particular locus or to a particular chromosome region (e.g. introgression fragment), to select plants for the presence of the specific locus or region (introgression fragment). For example, a molecular marker genetically and physically linked to an Rf locus, can be used to detect and/or select plants comprising the Rf locus. The closer the genetic linkage of the molecular marker to the locus, the less likely it is that the marker is dissociated from the locus through meiotic recombination. 
     “LOD-score” (logarithm (base 10) of odds) refers to a statistical test often used for linkage analysis in animal and plant populations. The LOD score compares the likelihood of obtaining the test data if the two loci (molecular markers loci and/or a phenotypic trait locus) are indeed linked, to the likelihood of observing the same data purely by chance. Positive LOD scores favor the presence of linkage and a LOD score greater than 3.0 is considered evidence for linkage. A LOD score of +3 indicates 1000 to 1 odds that the linkage being observed did not occur by chance. 
     A “biological sample” can be a plant or part of a plant such as a plant tissue or a plant cell. 
     “Providing genomic DNA” as used herein refers to providing a sample comprising genomic DNA from the plant. The sample can refer to a tissue sample which has been obtained from said plant, such as, for example, a leaf sample, comprising genomic DNA from said plant. The sample can further refer to genomic DNA which is obtained from a tissue sample, such as genomic DNA which has been obtained from a tissue, such as a leaf sample. Providing genomic DNA can include, but does not need to include, purification of genomic DNA from the tissue sample. Providing genomic DNA thus also includes obtaining tissue material from a plant or larger piece of tissue and preparing a crude extract or lysate therefrom. 
     “Isolated DNA” as used herein refers to DNA not occurring in its natural genomic context, irrespective of its length and sequence. Isolated DNA can, for example, refer to DNA which is physically separated from the genomic context, such as a fragment of genomic DNA. Isolated DNA can also be an artificially produced DNA, such as a chemically synthesized DNA, or such as DNA produced via amplification reactions, such as polymerase chain reaction (PCR) well-known in the art. Isolated DNA can further refer to DNA present in a context of DNA in which it does not occur naturally. For example, isolated DNA can refer to a piece of DNA present in a plasmid. Further, the isolated DNA can refer to a piece of DNA present in another chromosomal context than the context in which it occurs naturally, such as for example at another position in the genome than the natural position, in the genome of another species than the species in which it occurs naturally, or in an artificial chromosome. 
     Whenever reference to a “plant” or “plants” according to the invention is made, it is understood that also plant parts (cells, tissues or organs, seed pods, seeds, severed parts such as roots, leaves, flowers, pollen, etc.), progeny of the plants which retain the distinguishing characteristics of the parents (especially the restoring capacity), such as seed obtained by selfing or crossing, e.g. hybrid seed (obtained by crossing two inbred parental lines), hybrid plants and plant parts derived there from are encompassed herein, unless otherwise indicated. 
     In some embodiments, the plant cells of the invention may be non-propagating cells. 
     The obtained plants according to the invention can be used in a conventional breeding scheme to produce more plants with the same characteristics or to introduce the characteristic of the presence of the restorer gene according to the invention in other varieties of the same or related plant species, or in hybrid plants. The obtained plants can further be used for creating propagating material. Plants according to the invention can further be used to produce gametes, seeds, flour, embryos, either zygotic or somatic, progeny or hybrids of plants obtained by methods of the invention. Seeds obtained from the plants according to the invention are also encompassed by the invention. 
     In any of the above embodiment where reference is made to the SNP in SEQ ID NO. 16/18, i.e. where C at the nucleotide position corresponding to nucleotide position 429 of SEQ ID NO 16/18 is present in the restorer line, use can also be made of the further identified sequence polymorphisms (SNPs) in SEQ ID NO. 22 as described in Example 6. 
     “Creating propagating material”, as used herein, relates to any means know in the art to produce further plants, plant parts or seeds and includes inter alia vegetative reproduction methods (e.g. air or ground layering, division, (bud) grafting, micropropagation, stolons or runners, storage organs such as bulbs, corms, tubers and rhizomes, striking or cutting, twin-scaling), sexual reproduction (crossing with another plant) and asexual reproduction (e.g. apomixis, somatic hybridization). 
     Transformation, as used herein, means introducing a nucleotide sequence into a plant in a manner to cause stable or transient expression of the sequence. Transformation and regeneration of both monocotyledonous and dicotyledonous plant cells is now routine, and the selection of the most appropriate transformation technique will be determined by the practitioner. The choice of method will vary with the type of plant to be transformed; those skilled in the art will recognize the suitability of particular methods for given plant types. Suitable methods can include, but are not limited to: electroporation of plant protoplasts; liposome-mediated transformation; polyethylene glycol (PEG) mediated transformation; transformation using viruses; micro-injection of plant cells; micro-projectile bombardment of plant cells; vacuum infiltration; and  Agrobacterium -mediated transformation. 
     As used herein, the term “homologous” or “substantially identical” may refer to nucleotide sequences that are more than 85% identical. For example, a substantially identical nucleotide sequence may be 85.5%; 86%; 87%; 88%; 89%; 90%; 91%; 92%; 93%; 94%; 95%; 96%; 97%; 98%; 99% or 99.5% identical to the reference sequence. A probe may also be a nucleic acid molecule that is “specifically hybridizable” or “specifically complementary” to an exact copy of the marker to be detected (“DNA target”). “Specifically hybridizable” or “specifically complementary” are terms that indicate a sufficient degree of complementarity such that stable and specific binding occurs between the nucleic acid molecule and the DNA target. A nucleic acid molecule need not be 100% complementary to its target sequence to be specifically hybridizable. A nucleic acid molecule is specifically hybridizable when there is a sufficient degree of complementarity to avoid non-specific binding of the nucleic acid to non-target sequences under conditions where specific binding is desired, for example, under stringent hybridization conditions, preferably highly stringent conditions. 
     “Stringent hybridization conditions” can be used to identify nucleotide sequences, which are homologous or substantially identical to a given nucleotide sequence. Stringent conditions are sequence dependent and will be different in different circumstances. Generally, stringent conditions are selected to be about 5° C. lower than the thermal melting point (T m ) for the specific sequences at a defined ionic strength and pH. The T m  is the temperature (under defined ionic strength and pH) at which 50% of the target sequence hybridizes to a perfectly matched probe. Typically stringent conditions will be chosen in which the salt concentration is about 0.02 molar at pH 7 and the temperature is at least 60° C. Lowering the salt concentration and/or increasing the temperature increases stringency. Stringent conditions for RNA-DNA hybridizations (Northern blots using a probe of e.g. 100 nt) are for example those which include at least one wash in 0.2×SSC at 63° C. for 20 min, or equivalent conditions. 
     “High stringency conditions” can be provided, for example, by hybridization at 65° C. in an aqueous solution containing 6×SSC (20×SSC contains 3.0 M NaCl, 0.3 M Na-citrate, pH 7.0), 5×Denhardt&#39;s (100×Denhardt&#39;s contains 2% Ficoll, 2% Polyvinyl pyrollidone, 2% Bovine Serum Albumin), 0.5% sodium dodecyl sulphate (SDS), and 20 μg/ml denaturated carrier DNA (single-stranded fish sperm DNA, with an average length of 120-3000 nucleotides) as non-specific competitor. Following hybridization, high stringency washing may be done in several steps, with a final wash (about 30 min) at the hybridization temperature in 0.2-0.1×SSC, 0.1% SDS. 
     “Moderate stringency conditions” refers to conditions equivalent to hybridization in the above described solution but at about 60-62° C. Moderate stringency washing may be done at the hybridization temperature in 1×SSC, 0.1% SDS. 
     “Low stringency” refers to conditions equivalent to hybridization in the above described solution at about 50-52° C. Low stringency washing may be done at the hybridization temperature in 2×SSC, 0.1% SDS. See also Sambrook et al. (1989) and Sambrook and Russell (2001). 
     For the purpose of this invention, the “sequence identity” of two related nucleotide or amino acid sequences, expressed as a percentage, refers to the number of positions in the two optimally aligned sequences which have identical residues (×100) divided by the number of positions compared. A gap, i.e., a position in an alignment where a residue is present in one sequence but not in the other, is regarded as a position with non-identical residues. The “optimal alignment” of two sequences is found by aligning the two sequences over the entire length according to the Needleman and Wunsch global alignment algorithm (Needleman and Wunsch, 1970, J Mol Biol 48(3):443-53) in The European Molecular Biology Open Software Suite (EMBOSS, Rice et al., 2000, Trends in Genetics 16(6): 276-277; see e.g. http://www.ebi.ac.uklemboss/alignlindex.html) using default settings (gap opening penalty=10 (for nucleotides)/10 (for proteins) and gap extension penalty=0.5 (for nucleotides)/0.5 (for proteins)). For nucleotides the default scoring matrix used is EDNAFULL and for proteins the default scoring matrix is EBLOSUM62. It will be clear that whenever nucleotide sequences of RNA molecules are defined by reference to nucleotide sequence of corresponding DNA molecules, the thymine (T) in the nucleotide sequence should be replaced by uracil (U). Whether reference is made to RNA or DNA molecules will be clear from the context of the application. 
     As used herein “comprising” is to be interpreted as specifying the presence of the stated features, integers, steps or components as referred to, but does not preclude the presence or addition of one or more features, integers, steps or components, or groups thereof. Thus, e.g., a nucleic acid or protein comprising a sequence of nucleotides or amino acids, may comprise more nucleotides or amino acids than the actually cited ones, i.e., be embedded in a larger nucleic acid or protein. A chimeric gene comprising a nucleic acid which is functionally or structurally defined, may comprise additional DNA regions etc. 
     Unless stated otherwise in the Examples, all recombinant DNA techniques are carried out according to standard protocols as described in Sambrook et al. (1989) Molecular Cloning: A Laboratory Manual, Second Edition, Cold Spring Harbor Laboratory Press, NY and in Volumes 1 and 2 of Ausubel et al. (1994) Current Protocols in Molecular Biology, Current Protocols, USA. Standard materials and methods for plant molecular work are described in Plant Molecular Biology Labfax (1993) by R. D. D. Croy, jointly published by BIOS Scientific Publications Ltd (UK) and Blackwell Scientific Publications, UK. Other references for standard molecular biology techniques include Sambrook and Russell (2001) Molecular Cloning: A Laboratory Manual, Third Edition, Cold Spring Harbor Laboratory Press, NY, Volumes I and II of Brown (1998) Molecular Biology LabFax, Second Edition, Academic Press (UK). Standard materials and methods for polymerase chain reactions can be found in Dieffenbach and Dveksler (1995) PCR Primer: A Laboratory Manual, Cold Spring Harbor Laboratory Press, and in McPherson at al. (2000) PCR—Basics: From Background to Bench, First Edition, Springer Verlag, Germany. 
     All patents, patent applications, and publications or public disclosures (including publications on internet) referred to or cited herein are incorporated by reference in their entirety. 
     The sequence listing contained in the file named “BCS16-2009-WO1_ST25”, which is 67 kilobytes (size as measured in Microsoft Windows®), contains 27 sequences SEQ ID NO: 1 through SEQ ID NO: 27, is filed herewith by electronic submission and is incorporated by reference herein. 
     The invention will be further described with reference to the examples described herein; however, it is to be understood that the invention is not limited to such examples. 
     SEQ ID NO. 1-SEQ ID NO. 14: marker sequences (see table 1 and 2) 
     SEQ ID NO. 15: contig containing Rf3-PPR 
     SEQ ID NO. 16: coding sequence Rf3-PPR Chinese spring 
     SEQ ID NO. 17 amino acid sequence Rf3-PPR Chinese spring 
     SEQ ID NO. 18: coding sequence Rf3-PPR 
     SEQ ID NO. 19: amino acid sequence Rf3-PPR 
     SEQ ID NO. 20: mRNA1 Rf3-PPR
         Nt 1-432: 5′UTR   Nt 433-2259: CDS   Nt 2260-3145: 3′UTR       

     SEQ ID NO. 21: mRNA2 Rf3-PPR 
     Nt 1-432: 5′UTR 
     Nt 433-2259: CDS 
     Nt 2260-2759: 3′UTR 
     SEQ ID NO. 22: Genome 
     Nt 4469-4747: 3′UTR Rf3-PPR-SV2 (complement) 
     Nt 5223-6097: 3′UTR Rf3-PPR-SV1 (complement) 
     Nt 5597-6097: 3′UTR Rf3-PPR-SV2 (complement) 
     Nt: 6098-7924: cds (complement) 
     Nt: 7925-8357: 5′UTR (complement) 
     SEQ ID NO. 23: predicted RNA target 
     SEQ ID NO. 24: ORF256 
     Nt 87-857: cds 
     SEQ ID NO. 25: Fw primer 
     SEQ ID NO. 26: Rev primer 
     SEQ ID NO. 27: Probe 
     EXAMPLES 
     Example 1: Plant Materials and Genetic Mapping 
     A male sterile line carrying  Triticum timopheevii  CMS, CMS005, and a male sterile restorer line responding to  Triticum timopheevii  CMS ( T. timopheevii/ 2* lowin/12* Quivira, Accession number PI 583676, USDA National Small Grains Collection; http://www.ars.usda.gov/Main/docs.htm?docid=21891, also known as Dekalb 582M and registered as US PVP 7400045, available via the National Plant Germplasm System https://npgsweb.ars-grin.gov/gringlobal/accessiondetail.aspx?id=1478647), were used as parents to generate F1 progeny. The F1 progeny was selfed to generate an F2 population. The F2 population, consisting of 281 individuals, was used for identification of the markers linked to the restorer locus. A genetic map with total of 2080 SNP markers was established and covered all chromosomes of the wheat genome. The chromosome 1B is described by 150 SNP markers. 
     Example 2: Fertility Classification and Coarse Mapping 
     The 276 plants in this F2 population were phenotypically classified according to seed set on the main, bagged head. Plants without seeds under the bag were classified as sterile. Plants with seed set were classified as fertile.  FIG. 1  details the number of F2s per amount of seeds set on a single head for 2 different locations. 41 and 45 F2 plants in the 2 locations, were classified as sterile. Fully sterile F2 plants were noticed in the 2 locations. 
     Using a genetic map of 2080 SNP, QTL analysis was carried out using Haley-Knott regression to test the effect of variation in seed set across all markers. Significant marker-trait associations are distinguished by −log-transformed p-values higher than 3. Such, an interval of significantly associated markers was delineated, including left and right flanking markers (SEQ ID NO. 2 and SEQ ID NO. 8). The marker with the highest significance and biggest effect on restoration is the peak marker of SEQ ID NO. 6 (as indicated by X in Table 1 below). An interval of significantly associated markers was delineated using the following criteria: significance threshold at 2.5, significance drop at 1.5 and significance drop between peaks at 2. This delimited the interval to 15.8 cM for 1B by the left and right flanking markers ( FIG. 2 ). 
     
       
         
           
               
             
               
                 TABLE 1 
               
             
            
               
                   
               
               
                 Markers in the interval with significance of marker-trait association and effect size on restoration (in number 
               
               
                 of seeds above average seed set in the entire population) on 1B. 
               
            
           
           
               
               
               
               
               
               
               
               
               
               
            
               
                   
                   
                 SNP 
                 Chrnomosome 
                   
                   
                 mean 
                 additive 
                 dominance 
                 phenotypic 
               
               
                 SEQ 
                 Rf donor 
                 position in 
                 Position 
                 Significance 
                 Significance 
                 seed 
                 effect on 
                 effect on 
                 variance 
               
               
                 ID NO 
                 allele 
                 SEQ ID NO 
                 (cM) 
                 (−log10(p)) 
                 interval 
                 set 
                 seed set 
                 seed set 
                 explained 
               
               
                   
               
            
           
           
               
               
               
               
               
               
               
               
               
               
            
               
                 1 
                 A 
                 51 
                 35.206 
                 7.51 
                   
                 31.68 
                 10.05 
                 1.02 
                 0.13 
               
               
                 2 
                 T 
                 51 
                 35.753 
                 8.2 
                 x 
                 31.4 
                 10.51 
                 1.32 
                 0.14 
               
               
                 3 
                 C 
                 51 
                 38.165 
                 10.49 
                 x 
                 31.26 
                 11.8 
                 1.85 
                 0.18 
               
               
                 4 
                 T 
                 51 
                 38.37 
                 10.51 
                 x 
                 31.26 
                 11.8 
                 1.83 
                 0.18 
               
               
                 5 
                 T 
                 51 
                 42.221 
                 10.41 
                 x 
                 30.65 
                 11.78 
                 2.56 
                 0.18 
               
               
                 6 
                 A 
                 32 
                 46.302 
                 10.67 
                 X 
                 31.51 
                 12.06 
                 1.53 
                 0.18 
               
               
                 7 
                 A 
                 51 
                 46.911 
                 10.5 
                 x 
                 31.52 
                 11.97 
                 1.51 
                 0.18 
               
               
                 8 
                 G 
                 51 
                 51.588 
                 9.05 
                 x 
                 30.85 
                 10.85 
                 2.44 
                 0.15 
               
               
                 9 
                 T 
                 51 
                 51.772 
                 9.05 
                   
                 30.85 
                 10.85 
                 2.44 
                 0.15 
               
               
                   
               
            
           
         
       
     
     The mapping positions were confirmed when using seed set on a secondary head in both locations and when using phenotypic data of F3 progeny of this populations the next year in two locations. 
     Example 3: Fine-Mapping of Rf Region in 1B 
     For further fine-mapping, 40 F2 individuals that were heterozygous in the QTL region were selected based on phenotype and genotype. A total of 2560 individual F3 plants were grown in the field at 2 locations. For each plant, seed set on the main head under a bag was measured. Additional SNP assays were developed to increase the marker density in the QTL interval. A total of 374 additional SNP markers were using in mapping the 1B region. Table 2 provides exemplary SNP markers that were mapped in the region. 
     Marker-trait association using genetic maps of the chromosome 1B, established on F2 and F3 genotyping data, were determined using R-QTL. A total of 1094 individuals with genotype and phenotype data were processed per location. The Rf locus could be further delimited to a region of about 1.25 cM 1B (from 6.8 to 8.05 cM along chromosome 1B). 
     
       
         
           
               
             
               
                 TABLE 2 
               
             
            
               
                   
               
               
                 Exemplary markers in the fine-mapped region on 1B. Significant 
               
               
                 markers (highlighted with x) are examples of markers that are in 
               
               
                 the QTL support interval (LOD threshold &gt; 3; drop of 2 LODs 
               
               
                 from highest marker). The marker closest to the peak is marked 
               
               
                 with (v). Other markers residing outside the significant interval 
               
               
                 are indicated by ‘left flanking region’ (above) and ‘right 
               
               
                 flanking region (below). 
               
            
           
           
               
               
               
               
               
               
            
               
                   
                   
                   
                 finemap 
                 significant 
                   
               
               
                 SEQ 
                 Rf donor 
                 SNP 
                 map 
                 marker 
                 peak 
               
               
                 ID NO 
                 allele 
                 position 
                 position (cM) 
                 interval I 
                 marker 
               
               
                   
               
            
           
           
               
               
               
               
               
               
            
               
                 10 
                 T 
                 51 
                 6.1 
                   
                   
               
               
                 11 
                 C 
                 51 
                 7.1 
                 x 
               
               
                 12 
                 A 
                 51 
                 7.3 
                 x 
               
               
                 13 
                 T 
                 51 
                 7.35 
                 x 
                 v 
               
               
                 14 
                 T 
                 108 
                 8.05 
                 x 
               
               
                 5 
                 T 
                 51 
                 8.1 
               
               
                   
               
            
           
         
       
     
     Example 4: Integration of the Fine Map with Partial Genome Sequence and Candidate Gene Identification 
     Sequence of fine-mapped markers was used for Blasts to contigs and scaffolds of genome sequence of Chinese Spring. Stringent BLAST and parsing criteria were applied to position the SNPs in the partial genome sequence, such as &gt;98% sequence identity, alignment length of &gt;158 bp, hit in 1B sequence, and additional criteria for non-aligning overhang. Scaffolds were ordered to the fine map (and additional genetic maps). Next, the Rf clade of pentatricopeptide repeat protein sequences from maize, Sorghum, rice and Brachypodium were collected, using a gene family analysis of Fujii et al. (PNAS, 2011, supra, see Table S1). A total of 43 protein sequences were used for BLASTs and identified one locus in the fine-mapped interval. 
     The scaffold containing the PPR gene is given as SEQ ID NO. 15. 
     The thus identified PPR gene is represented by SEQ ID NO. 16 (nt—coding sequence) and 17 (aa). 
     Example 5—Further Fine-Mapping of Rf Region in 1B (F4) and in Silico Analysis 
     A set of SNP markers that were used for fine-mapping of the Rf3 locus were aligned to appropriate reference genome(s) to define a physical region representing the Rf3 QTL region on the reference genome. This QTL region was used to identify potential candidate genes and to develop additional markers for BAC-library screening (see below). Structural annotation of the Rf3 QTL region using ab initio gene annotation programs an in-house annotation pipeline, as well as by alignment of wheat EST sequences, wheat FL-cDNA sequences, wheat gene models and known restorer genes from orthologous species available from public databases. Functional annotation of genes in the QTL region was carried out using Blast2GO and PLAZA software programs as well as consultation of published literature. These candidate genes were then prioritized on the basis of their predicted functionality and their homology to known Rf genes (Chen and Liu, 2014; Dahan and Mireau, 2013). 
     Mapping fine-mapping genetic markers to the ‘Chinese Spring’ reference genome defined a region of ˜1.3 Mb on chromosome 1B that represented the Rf3 QTL region. In the ‘Chinese Spring’ reference, this region contained the identified pentacotripeptide (PPR) gene. PPR proteins are a large family of proteins that are characterized by possession of the canonical, degenerate 35-amino acid repeat motifs and that have been identified in other crops as being involved in restoration of fertility. This is mainly through mechanisms involving modification of the processing and/or transcription of cytotoxic mitochondrial transcripts (Dahan and Mireau, 2013; Gaborieau et al., 2016) (Chen and Liu, 2014; Schmitzlinneweber and Small, 2008). Restoration of fertility-type PPRs (Rf-PPRs) are members of the P-class of PPR proteins that typically bind single-stranded RNA in a sequence-specific fashion (Barkan et al., 2012; Binder et al., 2013; Chen and Liu, 2014; Gaborieau et al., 2016; Schmitzlinneweber and Small, 2008). Comparison of the sequences of the PPR gene sequences present in the Rf3 QTL region showed that they clustered with known P-class Rf-PPR orthologues from other crop species (data not shown). 
     Example 6—BAC Libraries of Restorer Line 
     In parallel with the in silico analysis (see above), a BAC library was constructed for the above described wheat restorer line (hereafter referred to as ‘Resource-5’), by digesting high-molecular weight ‘Resource-5’ gDNA with a restriction enzyme, and transforming the resultant fragments (mean insert size ˜80-130 Kb), into  E. coli . The fine-mapping SNP marker sequences, or markers developed from the Rf3 QTL region on the reference genome, were then used to design PCR primers to screen the pooled BAC clones. Once PCR-positive BAC pools had been identified, BACs from the pool were individualized and screened again with the same marker. Individual, PCR-positive BACs were then subjected to BAC-end sequencing to confirm integrity and the presence of the screening marker sequences. Finally verified positive BACs were deep sequenced using PacBio technology and reads assembled to generate a consensus sequence for the BAC insert. Sequenced, positive BACs were then aligned either by de novo assembly, or by assembly to the reference genome or tiled using the screening markers to generate a new ‘Resource-5’ reference sequence for the Rf3 QTL region. The ‘Resource-5’ Rf3 QTL reference sequence was then structurally and functionally annotated to identify any structural changes and/or differences in gene content and/or polymorphisms in the candidate gene captured within the region relative to the (non-restorer) reference genome. 
     The ‘Resource-5’ BAC library was screened multiple times using PCR markers developed from fine-mapping markers, reference genomes or isolated BAC sequences. Fourteen individualized and sequenced BACs were then tiled to create a contiguous sequence of ˜650 Kb and one additional sequence of 121 Kb separated by a gap of ˜75 Kb relative to the ‘Chinese Spring’ reference genome. These contigs represent the unique ‘Resource-5’ genome sequence for the Rf3 QTL region and were found to capture the Rf-PPR candidate gene initially identified. 
     As shown in  FIG. 3  A, the gene structure for Rf3-PPR is relatively simple consisting of a single exon and with no intron. While there is a potential splice variant for Rf3-PPR this does not impact the coding sequence. This relatively simple gene structure appears to be typical for Rf-PPRs). 
     Comparison of the ‘Resource-5’ Rf3-PPR candidate gene to the ‘Chinese Spring’ orthologue indicated that the sequence is highly conserved and that there is only one SNP present in the CDS but none +/−3 Kb up and downstream of the CDS; a single non-synonymous G to C SNP between CS and the Rf genomic sequence was identified at position 429 out of 1827 bp (SEQ ID NO. 18). This leads to a mehionone (M) to Isoleucine (I) amino acid change in the protein sequence on position 143 out of 608 (SEQ ID NO. 19). 
     SEQ ID NO. 20 and 21 represent the splice variants of the mRNA sequence Rf3-PPR, differing in their 3′ end but both leading to the same coding sequence (SEQ ID NO. 18) and amino acid sequence (SEQ ID NO. 19). 
     SEQ ID NO. 22 represents the genomic DNA sequence of the Rf3-PPR gene. 
     Three additional SNPs were identified in the genomic region surrounding Rf_PPR3: 
     In SEQ ID NO 22, which is in the reverse orientation, the A of the ATG start codon corresponds to the T at position 7924. 
     A SNP located 4489 downstream (T→C) from the ATG thus locates at position 3435 of SEQ ID NO. 22, where a C is present in the Rf3 restorer sequence. In the sense orientation, this thus corresponds to a A→G SNP 
     A SNP located 149 bp upstream from the ATG (C→T) thus locates at position 9073 of SEQ ID NO. 22, where a T is present in the Rf3 restorer sequence. In the sense orientation, this thus corresponds to a G→A SNP 
     A SNP located 3732 bp upstream from the ATG (A→G) thus locates at position 11656 of SEQ ID NO. 22, where an G is present in the Rf3 restorer sequence. In the sense orientation, this thus corresponds to a T→C SNP 
     Example 7—Annotation of the PPR Amino Acid Sequence 
     Known Rf-PPRs are members of the P-class of PPR proteins, and contain up to ˜30 PPR motifs per protein, with each motif comprising 35 amino acids (Gaborieau et al., 2016). Structurally PPR proteins consist of 2 α-helices that form a hairpin and a super-groove, and it is this super groove that interacts with an RNA molecule. The amino acid composition of the individual PPR motifs determines RNA which nucleotide is recognized, and the number of PPR motifs determines the length of the RNA sequence on the target transcript. Here the Rf3-PPR candidate was annotated to identify PPR motifs and other sequence features and the results summarized in  FIGS. 3  B and C. 
     Rf3-PPR is 608 amino acids long and contains 16 consecutive complete 35 amino-acid PPR motifs (SEQ ID NO. 19). This is similar to the Rf-1A gene cloned from rice, which is 791 amino acids long and contains 16 PPR repeats (Akagi et al., 2004; Komori et al., 2004). 
     Each PPR motif consists of 2 antiparallel helices that form a hairpin structure that interacts with a single stranded RNA molecule. Studies have demonstrated the existence of a recognition code linking the identity of specific amino acids within the repeats and the target RNA sequence of the PPR protein studied (Barkan et al., 2012; Yagi et al., 2013). In particular the identity of the 5th and the 35th amino acids of each motif have been shown to be particularly important and in the context of CMS, specificity is essential to specifically target the CMS-conferring transcript. On the basis of the identity of the amino acids at positions 5 and 35 in the Rf-PPR motif the predicted target transcript sequence for Rf3-PPR can be determined. Following the PPR code (Melonek et al., 2016, supra), the predicted RNA target sequence is thus 5′-AUUUKCASNCNYACGU-3′ (SEQ ID NO. 23, see also Table 3 below). 
     As shown in  FIG. 4 , alignment of the predicted target sequence of Rf3-PPR to the chimeric mitochondrial ORF-256 transcript (SEQ ID NO. 24, which has been proposed to be responsible for the CMS phenotype (Hedgcoth et al., 2002) indicates that there is a potential interaction site at positions 139-154 (sequence ATTTGCACTTTTGTAT). 
     The results here indicate that Rf3-PPR potentially binds the chimeric ORF256 transcript responsible for the CMS phenotype rand where it is thought to act by reducing the steady-state level of the deleterious ORF256 either by decreasing the stability of the corresponding RNA or by reducing translation (Binder et al., 2013). 
     The SNP 429 substitution impacts Met-143, which is a hydrophobic amino acid and relatively non-reactive replacing it with an isoleucine which is also hydrophobic, non-reactive amino acid, but is more bulky. The M→I substitution occurs in PPR motif no. 6 (see Table 3 as well as  FIG. 3 ), but does not impact one of the conserved positions required for determining nucleotide specificity. 
     The Met-lie substitution could potentially affect hairpin-formation of the α-helices, and so alter RNA-binding capacity or could impact potential dimerization of Rf3-PPR molecule. E.g. it was found that ‘Thylakoid assembly 8’ (THA8) protein is a pentatricopeptide repeat (PPR) RNA-binding protein required for the splicing of the transcript of ycf3, a gene involved in chloroplast thylakoid-membrane biogenesis. THA8 forms an asymmetric dimer once bound to single stranded RNA, with the bound RNA at the dimer interface. This dimer complex formation is mediated by the N-terminal PPR motifs 1 and 2 and the C-terminal motifs 4 and 5 (Ke et al., 2013, Nature Structural &amp; Molecular Biology, 20, 1377-1382). 
     
       
         
           
               
             
               
                 TABLE 3 
               
             
            
               
                   
               
               
                 PPR motifs and base recognition * Met→Ile SNP at 
               
               
                 position 145 in restorer line. See also FIG. 3. 
               
            
           
           
               
               
               
               
            
               
                   
                 Aa positions 
                   
                   
               
               
                 PPR motif 
                 (SEQ ID NO. 17/19) 
                 Position 5 and 35 
                 Base recognition 
               
               
                   
               
            
           
           
               
               
               
               
            
               
                 1 
                 10-44 
                 TN 
                 A 
               
               
                 2 
                 45-79 
                 ND 
                 U 
               
               
                 3 
                  80-114 
                 ND 
                 U 
               
               
                 4 
                  115-149* 
                 ND 
                 U 
               
               
                 5 
                 150-184 
                 AD 
                 G/U 
               
               
                 6 
                 185-219 
                 NN 
                 C 
               
               
                 7 
                 220-254 
                 SG 
                 A 
               
               
                 8 
                 255-290 
                 GD 
                 G/C 
               
               
                 9 
                 291-325 
                 HD 
                 ? 
               
               
                 10 
                 326-360 
                 NS 
                 C 
               
               
                 11 
                 361-395 
                 GT 
                 ? 
               
               
                 12 
                 396-430 
                 NC 
                 C/U 
               
               
                 13 
                 431-465 
                 SN 
                 A 
               
               
                 14 
                 466-500 
                 NN 
                 C 
               
               
                 15 
                 501-535 
                 SD 
                 G 
               
               
                 16 
                 536-570 
                 NE 
                 U 
               
               
                   
               
            
           
         
       
     
     Example 8—Expression Analysis 
     mRNA 
     Total RNA was isolated from −70-100 mgfw tissue using the Sigma Spectrum Plant Total RNA Kit (Sigma-Aldrich), and any gDNA contamination removed using the Qiagen RNase-Fee DNase Set (Cat. No. 79254). DNA concentration and integrity were determined with an Agilent Expert BioAnalyser. Tissue was sampled at four developmental stages (young leaf, spike 2.5-3.5, spike 3.5-4.5, spike 4.5-5.5 cm and anthers), using individuals from an F4-population of progeny derived from ‘Resource-5’. These progeny were genotyped using fine-mapping markers, phenotyped for fertility traits, and classified as either non-restoring (−/−), or heterozygous for Rf3 (Rf3/−). Three individual biological replicates were prepared per tissue type per genotype. 
     qRT-PCR Analyses 
     mRNA from each of the tissue/Rf3 genotypes was converted into cDNA using the EcoMix dry kit from Clonetech. Gene-specific probes were designed to quantify gene expression levels using the TaqMan assay as summarized in table 4. Probe specificity and efficiency were tested and optimised and expression analyses carried out on cDNA samples generated as above. 
     
       
         
           
               
             
               
                 TABLE 4 
               
             
            
               
                   
               
               
                 TaqMan primer and probe sequences used for  
               
               
                 gene expression analyses. 
               
            
           
           
               
               
               
               
               
               
            
               
                   
                   
                   
                   
                   
                 SEQ 
               
               
                 Gene 
                   
                   
                 Target 
                   
                 ID 
               
               
                 i.d. 
                 Name 
                 Type 
                 Region 
                 Sequence 5′-&gt;3′ 
                 NO. 
               
               
                   
               
               
                 Rf3- 
                 Fw3 
                 Primer 
                 549 . . . 567 
                 CCCCAACGTGGTGGC 
                 25 
               
               
                 PPR 
                   
                   
                   
                 ATAT 
                   
               
               
                   
               
               
                   
                 Rev3 
                 Primer 
                 complement 
                 CAGATTGCATGCCTT 
                 26 
               
               
                   
                   
                   
                 (603 . . . 624) 
                 GCCTACT 
                   
               
               
                   
               
               
                   
                 P3 
                 Probe 
                 569 . . . 583 
                 CCACGGTCATCCACG 
                 27 
               
               
                   
               
            
           
         
       
     
     Gene expression was examined in individual plants selected from f4 fine-mapping progeny segregating for the Rf3 locus, in four different tissues. Young leaf, developing spike 2.5-3.5 cm, developing spike 3.5-4.5 cm, developing spike 4.5-5.5 cm and anthers. Since it is expected that the cytoplasmic male sterile phenotype is due to the production of non-viable pollen, Rf genes must at least be expressed during the period of pollen development and meiosis. It is also expected that Rf gene expression will be highest in the early stages of pollen development. 
     As shown in  FIG. 5 , it is clear that mean expression of the PPR gene, is exclusively associated with the presence of the Rf3 locus, and is also highest at the 3.5-4.5 cm stage of spike development. 
     The SNP identified in Rf-PPR3 could thus also affect mRNA or protein stability, thereby contributing to an increased expression in the restorer line. 
     Example 9 Candidate Gene Validation 
     By Mutagenesis 
     A mutagenized population of the restore line is constructed. Based on sequencing, mutant plants with an inactivating mutation in the Rf candidate PPR gene are identified. The homozygous mutant plants and their wildtype segregants are screened for fertility restoration capacity. The plants that have a mutated PPR gene no longer has restoring ability, confirming that the identified candidate PPR gene is a functional Rf gene. 
     By Overexpression 
     The coding sequence of the candidate PPR-Rf gene is cloned under the control of a constitutive UBIQUITIN promoter (e.g. pUbiZm from maize), or under the control of a constitutive cauliflower mosaic virus promoter (p35S), or under the control of a vernalisation-related barley promoter (pvrn1) (or under control of its native promoter), in a T-DNA expression vector comprising a selectable marker, such as the bar gene. The resulting vector is transformed into a wheat line having no restoration capacity such as the transformable variety Fielder (or Chinese spring) according to methods well known in the art for wheat transformation (see e.g. Ishida et al Methods Mol Biol. 2015; 1223:189-98). The copy number of the transgene in the transgenic plant is determined by real time PCR on the selectable marker gene. The transformed plants comprising the candidate PPR-Rf gene cassette, preferably in single copy, are transferred to the greenhouse. Expression of the transgene in leaf tissue and in young developing spikes is tested by qRT-PCR. Transgenic TO plants expressing the candidate PPR-Rf gene are crossed as male parents to a G-type cytoplasmic male sterile (“CMS”) wheat line. F1 progeny of the crosses contain the G-type cytoplasm and show partial or complete restoration of male fertility due to the presence of the candidate PPR Rf gene. 
     The level of restoration in F1 progeny is tested using four different assays. In the first assay the mitochondrial ORF256 protein is quantified on Western blot using polyclonal antibodies raised against synthetic ORF256 protein. Expression of a functional candidate PPR Rf gene leads to reduced accumulation of the ORF256 protein. In the second assay pollen accumulation and pollen viability is quantified using the AmphaZ30 device. Expression of a functional candidate PPR Rf gene leads to higher numbers of viable pollen. In the third assay the integrity of anther tissues is inspected microscopically. Expression of a functional candidate PPR-Rf gene leads to better preservation of functional tapetum layer. In the fourth assay seed set per ear from self-pollination is quantified. Expression of a functional candidate PPR-Rf gene leads to higher number of grains per ear. In all tests the F1 progeny from crosses of non-transgenic Fielder plants to the same G-type cytoplasmic male sterile (“CMS”) wheat line serves as a control. 
     By Targeted Knock-Out 
     Guide RNAs for CRISPR-mediated gene editing targeting the mRNA coding sequence, preferably the protein coding sequence of the candidate PPR Rf gene, or the immediately upstream promoter sequence of the candidate PPR Rf gene are designed by using e.g. the CAS-finder tool. Preferably four unique or near-unique guide RNAs are designed per target gene. The guide RNAs are tested for targeting efficiency by PEG-mediated transient co-delivery of the gRNA expression vector with an expression vector for the respective nuclease, e.g. Cas9 or Cpf1, under control of appropriate promoters, to protoplasts of a wheat restorer line containing the candidate PPR-Rf gene of interest, preferably the line designated as  T. timopheevii/ 2* lowin/12* Quivira, USDA Accession number PI 583676. Genomic DNA is extracted from the protoplasts after delivery of the guide RNA and nuclease vectors. After PCR amplification, integrity of the targeted candidate PPR Rf gene sequence is assessed by sequencing. 
     The one or two most efficient guide RNAs are used for stable gene editing in same wheat restorer line also containing the G-type CMS cytoplasm. For this purpose, the selected guide RNA expression vector, together with a nuclease expression module and a selectable marker gene, are introduced into embryos isolated from the before mentioned wheat restorer line using e.g. particle gun bombardment. Transgenic plants showing resistance to the selection agent are regenerated using methods known to those skilled in the art. Transgenic TO plants containing gene targeting events, preferably small deletions likely resulting in a non-functional target candidate Rf PPR gene are identified by PCR amplification and sequencing. 
     Transgenic TO plants containing the G-type CMS cytoplasm and likely to contain a functional knock-out of the candidate PPR-Rf gene, preferably in homozygous state, but alternatively in heterozygous state, are crossed as female parents to a spring wheat line with normal cytoplasm and without PPR-Rf genes. The F1 progeny of the crosses contains the G-type “CMS” cytoplasm and 50% (in case of heterozygous TO) or 100% (in case of homozygous TO) of the F1 progeny will lack a functional version of the target Rf PPR gene. The F1 plants lacking a functional target Rf PPR gene are identified using genomic PCR assays. The F1 plants show partial or complete loss of male fertility due to the knock-out of the candidate PPR Rf gene. 
     The level of male fertility in the F1 progeny lacking a functional version of the candidate Rf PPR gene is tested using four different assays. In the first assay the mitochondrial ORF256 protein is quantified on Western blot using polyclonal antibodies raised against synthetic ORF256 protein. The knock-out of a functional candidate PPR Rf gene leads to increased accumulation of the ORF256 protein. In the second assay pollen accumulation and pollen viability is quantified using the AmphaZ30 device. The knock-out of a functional candidate PPR Rf gene leads to lower numbers of viable pollen. In the third assay the integrity of anther tissues is inspected microscopically. The knock-out of a functional candidate PPR Rf gene leads to early deterioration of the tapetum layer. In the fourth assay seed set per ear from self-pollination is quantified. The knock-out of a functional candidate PPR Rf gene leads to reduced number of grains per ear. In all tests the F1 progeny from crosses of non-edited Rf plants to the same spring wheat line serve as a control. 
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