Abstract:
A plant peptide transport gene and its nucleotide sequence are disclosed. The gene may be used to confer herbicide resistance to plants, and to render plants resistant to insect pests. The invention also relates to plants that possess non-naturally occurring alleles of peptide transport gene.

Description:
FIELD OF THE INVENTION 
     The invention relates to plant molecular genetics, and more specifically, to the cloning of a plant peptide transport gene. The plant peptide transport gene may be used to confer herbicide resistance, and pest resistance to recipient plants. The gene may also be used to facilitate the delivery of desired molecules into plants. The invention pertains to the peptide transport gene, to plants that contain the gene, and to methods for using the gene. 
     BACKGROUND OF THE INVENTION 
     Peptide uptake is the process by which individual cells are able to transport intact peptides across their plasma membranes. The process is a general physiological phenomenon of bacteria, fungi, plant cells and mammalian cells (Becker, J. M. et al, In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 257-279 (1980); Matthews, D. M. et al., Curr. Top. Membr. Transp. 14:331-425 (1980)). In every case studied so far, peptide transport is a specific biochemical process in which small peptides (≦6 amino acids) are transported across a membrane by energy-dependent, saturable carriers. 
     Three genetically distinct systems of peptide uptake have been identified in gram-negative bacteria. An oligopeptide permease (Opp) system has been identified in bacteria such as E. coli, and S. typhirnurium (Andrews, J. C. et al., J. Bacteriol. 161:484-492 (1985); Hogarth, B. G. et al., J. Bacteriol. 153:1548-1551 (1983)). The Opp system is capable of transporting peptides having up to 5 amino acid residues, regardless of their side chains (Payne, J. W. et al, J. Biol. Chem. 243:3395-3403 (1968); Payne, J. W. et al., J. Biol. Chem. 243:6291-6299 (1968)). In contrast, tripeptide permease (Tpp) systems, such as that of S. typhimurium, exhibit an apparent affinity for peptides having hydrophobic amino acid residues (Gibson, M. M. et al., J. Bacteriol. 160:122-130 (1984)). The third system, a dipetide permease (Dpp) system, has a preference for transporting dipeptides (Abouhamad, W. N., et al., Mol. Microbiol. 5:1035-1047 (1991)). Functionally similar systems have been described in fungi and yeast (Naider, F. et al., In: Current Topics in Medial Mycology, volume II, McGinnis, M. M. (ed.) (1987)), but have not been well characterized. 
     The genes that encode the protein components of the oligopeptide transporters of E. coil (Kashiwagi, K. et al, J. Biol. Chem. 265:8387-8391 (1990)), Salmonella typhimurium (Hiles, I. D. et al., Eur. J. Biochem. 158:561-567 (1986); Hiles, I. D. et al, J. Molec. Biol 195:125-142 (1987)), Bacillus subtills (Rudner, D. Z. et al., J. Bacteriol. 173:1388-1398 (1991); Perego, M. et al., Mol. Microbiol. 5:173-185 (1991)), Streptococcus pneumoniae (Alloing, G. et al., Mol. Microbiol. 4:633-644 1990)), and Lactococcus lactis as well as two dipeptide permeases, one in E. coil (Abouhamad, W. N., et al., Mol. Microbiol. 5:1035-1047 (1991)), and the other in Bacillus subtilis (Mathiopoulos, C. et al., Mol. Microbial. 5:1903-1913 (1991)) have been cloned and sequenced. 
     The ability of bacteria and plant cells to accumulate peptides has been found to be dependent upon peptide transport systems (Becker, J. M. et al., In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 257-279 (1980); Matthews, D. M. et al., Curr. Top. Membr. Transp. 14:331-425 (1980); Higgins, C. F. et al., In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 211-256 (1980); Naider, F. et al., In: Current Topics in Medial Mycology, volume II, McGinnis, M. M. (ed.) (1987)). These systems are distinct from the mechanisms that mediate the uptake of amino acids. 
     The existence of peptide transport systems in plants was demonstrated by showing that plants could accumulate non-hydrolyzable, non-physiological peptide substrates, intact and against a concentration gradient (Higgins, C. F. et al., Planta 134:205-206 (1977); Higgins, C. F. et al., Planta 136:71-76 (1977); Higgins, C. F. et al, Planta 138:211-216 (1978); Higgins, C. F. et al., Planta 142:299-305 (1978); Sopanen, T. et al., FEBS Lett. 79:4-7 (1977)). The transport system was found to exhibit saturation kinetics and to be inhibited by a range of metabolic inhibitors (Higgins, C. F. et al., Planta 136:71-76 (1977)). The plant peptide transport system can transport both di- and tripeptides (Sopanen, T. et al., FEBS Lett. 79:4-7 (1977); Higgins, C. F. et al., Planta 142:299-305 (1978)). Plant peptide transport systems are capable of transporting a wide variety of peptides. These systems exhibit broad transport specificity with respect to amino acid side-chains. The presence of D-amino acids, however, reduces the transport rate, thus indicating that the transporters have strong stereospecificity. Two proteins, approximately 66 D and 41 D, have been suggested as components of the plant peptide transport system in barley grains (Payne, J. W. et al., Planta 170:263-271 (1987). 
     The primary function of peptide transport is to supply amino acids for nitrogen nutrition (Payne, J. W. et al., In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 257-279 (1980); Matthews, D. M. et al., Curr. Top. Membr. Transp. 14:331-425 (1980); Becker, J. M. et al., In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 257-279 (1980); Adibi, S. A. et al., Metabolism 36:1001-1011 (1987); Higgins, C. F. et al., Planta 138:211-216 (1978); Sopanen, T. et al., FEBS Lett. 79:4-7 (1977); Higgins, C. F. et al., Planta 138:217-221 (1978)). In bacteria, peptide transport has, however, also been associated with sporulation (Perego, M. et al., Mol. Microbiol. 5:173-185 (1991); Mathiopoulos, C. et al., Mol. Microbiol. 5:1903-1913 (1991)); chemotaxis (Manson, M. D. et al., Nature 321:253-256 (1986), and the recycling of cell wall peptides (Goodell, E. W. et al., J. Bacteriol 169:3861-3865 (1987)). 
     A variety of plant pathogens attack plants by secreting toxic peptides. A capacity to control peptide transport may permit the development of pathogen-resistant plants. The present invention provides polynucleotide molecules, and methods that may be useful for producing such valuable plants. 
     SUMMARY OF THE INVENTION 
     The invention concerns a plant peptide transport gene. The gene mediates the uptake of di- and tri-peptides, and confers upon recipient plants the ability to grow on such peptides. Such a capability may be used to facilitate the delivery of desired molecules, such as proteins, etc. into plant cells. By mutating the gene, it is possible to render a plant resistant to toxic peptides, and thus provide the plant with resistance to herbicides and insect toxins. The present invention is directed to polynucleotides that encode the peptide transport gene, to the encoded protein, to antisense molecules that attenuate the expression of the transport gene, and to methods for using all such compositions to improve plant vitality and resistance. The invention also includes plants having non-naturally occurring alleles of the transport gene. 
     In detail, the invention provides, a substantially purified nucleic acid molecule containing a polynucleotide portion of a plant gene that encodes a peptide transport protein. The polynucleotide portion may encode a functional transport protein, a non-functional transport protein, or a non-functional fragment of either. 
     The invention additionally concerns a plant cell containing any of such substantially purified nucleic acid molecules, especially, wherein the polynucleotide portion of the plant gene encodes a non-functional transport protein or a non-functional fragment of a peptide transport protein, and wherein the presence of the polynucleotide impairs a capacity of the cell to transport peptides. 
     The invention also concerns plants and plant products (fruit, leaves, seeds) containing the above-described plant cells. 
     The invention also provides a method for increasing the resistance of a plant to an herbicidal peptide which comprises: 
     A. providing a polynucleotide to cells of the plant, the polynucleotide encoding a mutated peptide transport protein or a fragment of a peptide transport protein, wherein the presence of the polynucleotide impairs a capacity of the cells to transport peptides; 
     B. permitting the polynucleotide to impair the capacity of the plant cells to transport the herbicidal peptide. 
     The invention also provides a method for selectively inhibiting the growth of an undesired peptide transport proficient plant relative to the growth of a desired peptide transport deficient plant, the method comprising: 
     A. providing a peptide to the undesired plant, and optionally also to the desired plant, wherein the peptide comprises a toxic moiety capable of inhibiting the growth of a plant when transported into a cell of the plant; and 
     B. permitting the undesired plant to transport the toxic moiety-containing peptide into its cells and further permitting the transported toxic moiety to mediate the inhibition of the growth of the undesired plant. 
     The invention further concerns a method for delivering an affector of a plant characteristic to a plant, which comprises: 
     A. providing a polynucleotide to cells of the plant, the polynucleotide encoding a peptide transport protein, wherein the presence of the polynucleotide provides or augments a capacity of the cells to transport peptides; 
     B. providing a peptide conjugate to the plant, the conjugate containing a moiety that comprises the affector; and 
     C. permitting the peptide transport protein to mediate the delivery of the affector to the plant. 
     The invention additionally provides a method for identifying an affector of a plant characteristic which comprises: 
     A. incubating a candidate affector, the affector being conjugated to a peptide, in the presence of a peptide transport deficient Saccharomyces cerevisiae strain; 
     B. incubating the conjugated candidate affector in the presence of a peptide transport proficient Saccharomyces cerevisiae strain; and 
     C. determining whether the candidate affector is capable of affecting a characteristic of the peptide transport proficient Saccharomyces cerevisiae strain but is incapable of affecting the characteristic in the peptide transport deficient Saccharomyces cerevisiae strain. 
     The invention also provides a method for identifying polynucleotides that encode a plant peptide transport protein which comprises: 
     A. introducing a candidate polynucleotide into a peptide transport deficient Saccharomyces cerevisiae strain; 
     B. incubating the peptide transport deficient Saccharomyces cerevisiae strain in the presence of a peptide; and 
     C. determining whether the introduction of the candidate polynucleotide is sufficient to permit the Saccharomyces cerevisiae strain to mediate the transport of the peptide. 
    
    
     DESCRIPTION OF THE FIGURES 
     FIG. 1 shows the complete nucleotide sequence of the 2.8 kb insert of Arabidopsis cDNA in plasmid pPTF4. The sequence starts with the complete 5&#39; Notl restriction site and stops four nucleotides past the 3&#39; Notl restriction site. The start and stop codons are highlighted in bold. The deduced amino acid sequence of the ATPTR2Ap protein is represented by the single letter amino acid code appearing below the nucleotide sequence. Amino acids predicted to be hydrophobic segments are underlined. 
     FIG. 2 shows the complete nucleotide sequence of the 2.0 kb insert of Arabidopsis cDNA in plasmid pDTF1. The sequence starts with the complete 5&#39; Notl restriction site and stops four nucleotides past the 3&#39; Notl restriction site. The deduced amino acid sequence of the ATPTR2Bp protein is represented by the single letter amino acid code appearing below the nucleotide sequence. 
     FIG. 3 shows the uptake of L-  3  H!dileucine by ATPTR2Ap. The Figure shows uptake by wild-type S288C, S. cerevisiae peptide transport mutant PB1X-9B, and PB1X-9B transformed with pPTF4. The competitor is 100× unlabelled dileucine. (∘) S288C+dileucine; () PB1X-9B; (open ∇) PB1X-9B pPTF4!; (solid ∇) PB1X-9B pPTF4!+dileucine. 
    
    
     DESCRIPTION OF THE PREFERRED EMBODIMENTS 
     I. The Peptide Transport Gene of the Present Invention 
     The present invention arises, in part, from the exploitation of the S. cerevisiae peptide transport (PTR) system. In the yeast system, peptides are transported with little amino acid side-chain specificity but with strong stereospecificity for L-amino acids. Transport is under nitrogen repression control and can be induced by micromolar amounts of amino acids (Becker, J. M. et al., In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 257-279 (1980); Island, M. D. et al., J. Bacteriol. 169:2132-2136 (1987)). At least three genes (designated ptr1, ptr2 and ptr3) are known to be involved in this process (Island, M. D. et al., Curr. Genet. 20:457-463 (1991)). Although S. cerevisiae strains that carry mutations in PTR1 and PTR2 are completely deficient for peptide transport (as defined by their resistance to toxic dipeptides and lack of uptake of radiolabeled peptide substrates), such mutations exhibit a substantial reversion frequency. This reversion frequency complicates their use. 
     Thus, one aspect of the present invention is the construction of a stable S. cerevisiae ptr2 mutant. Methods for isolating such mutants are described below, and by Perry, J. R. et al. (In: &#34;Isolation and Characterization of a Saccharomyces cerevisiae Peptide Transport Gene,&#34; Molecular and Cellular Biology, volume 14 (1994), herein incorporated by reference in its entirety). Polynucleotides that encode the peptide transport genes of higher plants have been identified and isolated by their capacity to complement the peptide transport deficiency of the stable S. cerevisiae ptr2 strain. The nucleotide sequences of two such polynucleotides isolated from Arabidopsis thaliana are described herein in SEQ ID NO:1 and SEQ. ID NO:3. 
     The present invention relates in part to the isolation of a novel polynucleotide that is capable of hybridizing to, or recombining with, a plant gene that encodes a peptide transport protein. The polynucleotides of the present invention are &#34;substantially&#34; purified,&#34; in that they have been purified from undesired plant genes with which they are associated in nature. The molecules may be in either a double-stranded or single-stranded form. Such polynucleotides are capable of augmenting the transport capacity of a recipient plant, and thus may be used to facilitate the delivery of desired compounds to the plant. In an alternative embodiment, the polynucleotides of the present invention can be used to disrupt or otherwise inactivate endogenous transport systems. Such disruption renders the plant incapable of transporting toxic peptides, and thus resistant to pathogens that produce such peptides. 
     The capacity of the polynucleotides of the present invention to hybridize to a plant gene arises out of the extent of homology between the respective sequences of the polynucleotides. As used herein, a polynucleotide of the present invention is said to be able to &#34;hybridize&#34; to a plant gene if the two molecules are capable of forming an anti-parallel, double-stranded nucleic acid structure. The molecules are said to be &#34;minimally complementary&#34; if they can hybridize to one another with sufficient stability to permit them to remain annealed to one another under at least conventional &#34;low-stringency&#34; conditions. Similarly, the molecules are said to be &#34;complementary&#34; if they can hybridize to one another with sufficient stability to permit them to remain annealed to one another under conventional &#34;high-stringency&#34; conditions. Such conventional stringency conditions are described by Sambrook, J., et al., (In: Molecular Cloning, a Laboratory Manual, 2nd Edition, Cold Spring Harbor Press, Cold Spring Harbor, N.Y. (1989)), and by Haymes, B. D., et al. (In: Nucleic Acid Hybridization, A Practical Approach, IRL Press, Washington, D.C. (1985)), both herein incorporated by reference). 
     Complementary molecules thus need not exhibit &#34;complete complementarity,&#34; but need only be sufficiently complementary in sequence to be able to form a stable double-stranded structure. Departures from complete complementarity are therefore permissible, so long as such departures do not completely preclude the capacity of the molecules to form a double-stranded structure. In contrast, where two nucleic acid molecules exhibit &#34;complete complementarity,&#34; every nucleotide of one of the molecules is complementary to a nucleotide of the other; such molecules need not have the same lengths. 
     The capacity of the polynucleotides of the present invention to recombine with a plant gene is determined by the extent of sequence &#34;homology&#34; between the polynucleotide and the plant gene. Homologous recombination is a well-studied natural cellular process which involves the exchanges of a region of one polynucleotide with a region of another (see, Sedivy, J. M., Bio-Technol. 6:1192-1196 (1988)). Sufficient homology for recombination requires only minimal homology in regions of the polynucleotide that flank the portion of the polynucleotide that undergoes recombination. The region may be of any length from a single base to a substantial fragment of a chromosome. Generally, a region having a length of about ten nucleotide residues is sufficient. Recombination is catalyzed by enzymes which are naturally present in both prokaryotic and eukaryotic cells. 
     The polynucleotides of the present invention comprise isolated nucleic acid molecules that can complement a peptide transport deficiency of S. cerevisiae. The term &#34;polynucleotide&#34; encompasses nucleic acid molecules that encode a complete protein, as well as nucleic acid molecules that encode fragments of a complete protein. The polynucleotides may comprise the wild-type allele (or a portion of such allele) of a functional peptide transport gene, or they may comprise mutated or disrupted (as by the insertion of additional DNA or RNA) alleles of such genes. As used, herein a &#34;fragment&#34; of a polynucleotide is an oligonucleotide whose nucleotide sequence is identical to that of a region of the polynucleotide, and whose length is greater than about 15 nucleotide residues, and preferably greater than about 20 nucleotide residues. The above-identified polynucleotides of Arabidopsis thaliana, SEQ. ID NO:1 and SEQ. ID NO:3, and fragments thereof comprise the preferred polynucleotides thereof. 
     The isolation and cloning of polynucleotides that encode Arabidopsis thaliana peptide transport proteins permits the isolation of analogous, complementary polynucleotides from other plants. The functional role of such isolated polynucleotides can be readily determined by transforming them into the above-described stable peptide transport-deficient yeast strain, and evaluating whether transformants acquire the capacity to transport intact peptides. Thus, the methods of the present invention permit the isolation of polynucleotides from other plant species. Such polynucleotides are the equivalents of the preferred polynucleotides of the present invention. 
     In one embodiment of the invention, the polynucleotides will be operably linked to regulatory sequences sufficient to permit the polynucleotide&#39;s transcription. Such polynucleotides may be incorporated into nucleic acid vectors that are sufficient to permit either the propagation or maintenance of the polynucleotide within a host cell. The nature of the regulatory elements will depend upon the host cell, and the desired manner of expressing the polynucleotide. Examples of suitable regulatory elements include constitutive or inducible prokaryotic promoters, such as the λpL or pR promoters, or other well-characterized promoters (e.g., lac, gal, trp, ara, hut, etc.). Other promoters which may be employed are the nos, ocs and CaMv promoters. Efficient plant promoters that may be used are over-producing plant promoters such as the small subunit (ss) of the ribulose 1, 5 biphosphate carboxylase from soybean (Berry-Lowe, et al., J. Molec. App. Gen. 1:483-498 (1982)) and the promoter of the chlorophyll a/b binding protein. These two promoters are known to be light induced in eukaryotic plant cells (see Genetic Engineering of Plants, An Agricultural Perspective,&#34; Cashmore, A. (ed), Plenum, N.Y., pp. 29-38 (1983); Coruzzi, G. et al., J. Biol. Chem. 258:1399 (1983); and Dunsmeier, P. et al., J. Molec. App. Gen. 2:285 (1983)). The 35S promoter is particularly preferred. 
     Preferred prokaryotic vectors include plasmids such as those capable of replication in E. coil such as, for example, pBR322, ColE1, pSC101, pACYC 184, πVX. Such plasmids are, for example, disclosed by Maniatis, T., et al. (In: Molecular Cloning, A Laboratory Manual, Cold Spring Harbor Press, Cold Spring Harbor, N.Y. (1982)). Bacillus plasmids include pC194, pC221, pT127, etc. Such plasmids are disclosed by Gryczan, T. (In: The Molecular Biology of the Bacilli, Academic Press, N.Y. (1982), pp. 307-329). Suitable Streptomyces plasmids include plJ101 (Kendall, K. J., et al., J. Bacteriol. 169:4177-4183 (1987)), and Streptomyces bacteriophages such as .o slashed.C31 (Chater, K. F., et al., In: Sixth International Symposium on Actinomycetales Biology, Akademiai Kaido, Budapest, Hungary (1986), pp. 45-54). Pseudomonas plasmids are reviewed by John, J. F., et al. (Rev. Infect. Dis. 8:693-704 (1986)), and Izaki, K. (Jpn. J. Bacteriol. 33:729-742 (1978)). 
     Examples of suitable yeast vectors include the yeast 2-micron circle, the expression plasmids YEP13, YCP and YRP, etc., or their derivatives. Such plasmids are well known in the art (Botstein, D., et al., Miami Wntr. Syrup. 19:265-274 (1982); Broach, J. R., In: The Molecular Biology of the Yeast Saccharomyces: Life Cycle and Inheritance, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y., p. 445-470 (1981); Broach, J. R., Cell 28:203-204 (1982); Sherman, F. et al., In: Methods in Yeast Genetics, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1986)). 
     As indicated, the invention particularly contemplates providing the polynucleotides of the present invention to plants, especially tobacco, coffee, wheat and other cereals, apple and other non-citrus fruit producers, and citrus fruit crops. Suitable plants include, for example, species from the genera Fragaria, Lotus, Medicago, Onobrychis, Trifolium, Trigonefla, Vigna, Citrus, Linum, Geranium, Manicot, Daucus, Arabidopsis, Brassica, Raphanus, Sinapis, A tropa, Capsicum, Datura, Hyoscyamus, Lycopersion, Nicotiana, Solanum, Petunia, Digitalis, Majorana, Cichorium, Helianthus, Lactuca, Bromus, Asparagus, Antirrhinum, Hemerocallis, Nemesia, Pelargonium, Panicurn, Pennisetum, Ranunculus, Senecio, Salpiglossis, Cucumis, Browallia, Glycine, Lolium, Zea, Triticum, Sorghum, Ipomoea, Passiflora, Cyclamen, Malus, Prunus, Rosa, Rubus, Populus, Santalure, Allium, Lilium, Narcissus, Ananas, Arachis, Phaseolus, Pisum and Datura. 
     In one embodiment, such polynucleotides will be provided without promoters or other regulatory elements, but under conditions sufficient to permit the polynucleotide to recombine with and replace a region of the endogenous plant peptide transport gene. In an alternative embodiment, the polynucleotides will be administered to the plant operably linked to regulatory elements and/or vector elements. 
     Any of a variety of methods may be used to introduce the polynucleotides of the present invention into a plant cell. The genetic material can be microinjected directly into the plant embryo cells or introduced by electroporation as described in Fromm et al., &#34;Expression of Genes Transformed into Monocot and Dicot Plant Cells by Electroporation,&#34; Proc. Nat&#39;l. Acad. Sci. U.S.A. 82:5824-28 (1985) or it can be introduced by direct precipitation using polyethylene glycol as described in Paszkowski et al., EMBO J. 3:2717-22 (1984). In the case of monocotyledonous plants, pollen may be transformed with total DNA or an appropriate functional clone providing resistance, and the pollen then used to produce progeny by sexual reproduction. 
     The Ti plasmid of Agrobacterium tumefaciens provides a means for introducing DNA into plant cells (Caplan, A., et al., Science 815-821 (1983); Schell, J. et al., Bio/Technology, April 1983, pp. 175-1980; Fraley, R. T., et al., Proc. Nat&#39;l. Acad. Sci. U.S.A. 80:4803 (1983); (Hooykass, P. J. J. et al., In: Molecular Form and Function of the Plant Genome, Vlotan-Doltan, L. et al. (eds.), Plenum Press, N.Y., pp. 655-667 (1984); Horsch, R. B. et al., In: Current Communications in Molecular Biology, Cold Spring Harbor Press, Cold Spring Harbor, N.Y., pp. 13-19 (1988); Horsch et al., Science 233:496-498 (1984); all herein incorporated by reference). As such, it provides a highly preferred method for introducing the polynucleotides of the present invention into plant cells 
     Ti plasmids contain two regions essential for the production of transformed cells. One of these, termed &#34;transfer DNA&#34; (T DNA), induces tumor formation. The other, termed &#34;virulent region,&#34; is essential for the formation but not maintenance of tumors. It is possible to insert the polynucleotides of the present invention into the T DNA region without affecting its transfer function. By removing the tumor-causing genes so that they no longer interfere, the modified Ti plasmid can then be used as a vector for the transfer of the gene constructs of the invention into an appropriate plant cell. The polynucleotides of the present invention are preferably inserted between the terminal sequences that flank the T-DNA. 
     A particularly useful Ti plasmid vector is pGV3850, a non-oncogenic derivative of the nopaline Ti plasmid C58 (Caplan, A., et al., Science 815-821 (1983)). This vector utilizes the natural transfer properties of the Ti plasmid. The internal T DNA genes that determine the undifferentiated crown gall phenotype have been deleted and are replaced by any commonly used cloning vehicle (such as pBR322). The cloning vehicle sequence contained between T DNA border regions serves as a region of homology for recombination to reintroduce foreign DNA cloned in a derivative of the same cloning vehicle. Any polynucleotide of the present invention cloned in such plasmid can thus be inserted into pGV3850 by a single recombination of the homologous sequences. Antibiotic resistance markers can be added to the plasmid to select for the recombination event. The presence of the nopaline synthase (nos) gene in pGV3850 facilitates the monitoring of the transformation. 
     The introduction of the Ti plasmid is typically accomplished by infecting a wounded leaf of the plant with Agrobacterium tumefaciens bacteria that contains the plasmid. Under appropriate growth conditions, a ring of calli forms around the wound (Hooykass, P. J. J. et al., In: Molecular Form and Function of the Plant Genome, Vlotan-Doltan, L. et al. (eds.), Plenum Press, N.Y., pp. 655-667 (1984)). The calli are then transferred to growth medium, allowed to form shoots, roots and develop further into plants. 
     The procedure can alternatively be performed in tissue culture. All plants from which protoplasts can be isolated and cultured to give whole regenerated plants can be transformed by the present invention so that whole plants are recovered which contain the introduced polynucleotide. There is an increasing body of evidence that practically all plants can be regenerated from cultured cells or tissues, including but not limited to all major cereal crop species, sugarcane, sugar beet, cotton, fruit and other trees, legumes and vegetables (Hooykass, P. J. J. et al., In: Molecular Form and Function of the Plant Genome, Vlotan-Doltan, L. et al. (eds.), Plenum Press, N.Y., pp. 655-667 (1984); Horsch, R. B. et al., In: Current Communications in Molecular Biology, Cold Spring Harbor Press, Cold Spring Harbor, N.Y., pp. 13-19 (1988)). Methods for regenerating plants from cultural protoplasts are described by Evans et al. (Handbook of Plant Cell Culture 1:124-176; by Davey, M. R., In: Protoplasts 1983--Lecture Proceedings, pp. 19-29, Birkhauser, Basel (1983)); Dale, P. J. (In: Protoplasts 1983--Lecture Proceedings, pp. 31-41, Birkhauser, Basel (1983)); Binding, H. (In: Plant Protoplasts, CRC Press, Boca Raton, pp. 21-37 (1985)) and Cooking, E. C. In: Molecular Form and Function of the Plant Genome, Vlotan-Doltan, L. et al. (eds.), Plenum Press, N.Y., pp. 27-32 (1984)). 
     Regeneration efficiency varies from species to species of plants, but generally a suspension of transformed protoplasts containing the introduced gene sequence is formed. Embryo formation can then be induced from the protoplast suspensions, to the stage of ripening and germination as natural embryos. The culture media will generally contain various amino acids and hormones, such as auxin and cytokinins. It is also advantageous to add glutamic acid and proline to the medium, especially for such species as corn and alfalfa. Shoots and roots normally develop simultaneously. Efficient regeneration will depend on the medium, on the genotype, and on the history of the culture. If these three variables are controlled, then regeneration is fully reproducible and repeatable. 
     Other systems, such as cauliflower mosaic virus, CaMV (Hohn, B., et al., In &#34;Molecular Biology of Plant Tumors,&#34; Academic Press, New York, pp. 549-560; and Howell, U.S. Pat. No. 4,407,956) can also be used to introduce the polynucleotides of the present invention into plant cells. In accordance with such methods, the entire CaMV viral DNA genome is inserted into a parent bacterial plasmid thus creating a recombinant DNA molecule which can be propagated in bacteria. After cloning, the recombinant plasmid is cleaved with restriction enzymes either at random or at unique sites in the viral portion of the recombinant plasmid for insertion of the polynucleotides of the present invention. The modified viral portion of the recombinant plasmid is then excised from the parent bacterial plasmid, and used to inoculate the plant cells or plants. 
     After transformation of the plant cell or plant, the same may be selected by aid of an appropriate marker, such as antibiotic resistance, and then assessed to determine whether it contains the desired polynucleotide of the invention. The mature plants, grown from the transformed plant cells, can be selfed to produce an inbred plant whose seeds will contain the introduced polynucleotides of the present invention. These seeds can be grown to produce plants that exhibit any of a set of desired properties. 
     In one embodiment of the present invention, the exhibited property will be an increased facility to transport peptides. In this embodiment, the polynucleotides of the invention are provided to the plant or plant cells along with transcriptional regulatory sequences, such that an overexpression of the plant&#39;s peptide transport gene occurs. Such plants are desirable in that their enhanced peptide transport system can be used to facilitate the up take of peptide-associated molecules. 
     In an alternative embodiment, the exhibited property will be an impairment or obliteration of the plant&#39;s peptide transport system. Such plants are produced by providing cells with mutated polynucleotides and permitting such polynucleotides to recombine with, and mutate, the cells&#39; endogenous peptide transport gene. As a consequence of such recombination, the plant will have lost the capacity to mediate peptide transport. Such plants, and their fruit, are valuable in that they are resistant to the toxic peptides produced by plant pathogens. 
     Parts obtained from the regenerated plant, such as flowers, seeds, leaves, branches, bark, fruit, and the like are covered by the invention. Progeny and variants, and mutants of the regenerated plants are also included within the scope of this invention. 
     II. Uses of the Peptide Transport Gene of the Present Invention 
     A. Resistance to Plant Pathogens and Herbicides 
     Several plant pathogens have been found to attack plants through the production of toxic peptides. For example, phaseotoxin, produced by Pseudomonas syringae pv. phaseolicola, the causal agent of halo blight of bean, is a tripeptide that is further processed by peptidases in vivo to a smaller active form (Willis, D. K. et al., Experimentia 47:765-771 (1991); Gross, D. C., Ann. Rev. Phytopathol. 29:247-278 (1991)). Likewise, tabtoxin, produced by Pseudomonas syringae pv. tabaci, is the causal agent of wildfire of tobacco. Many phytopathogenic fungi produce toxic peptides (Higgins, C. F. et al., In: Encyclopedia of Plant Phsyiology, N. S., volume 14A, Boulter, D. et al. (eds.) Springer, N.Y., pp. 438-458 (1982)). Such resistance can be manifested by hardier plants, or by foodstuffs (fruit, leaves, etc.) that are more resistant to spoilage or decay. 
     Substantial evidence suggests that the uptake of toxic peptides is mediated by peptide transport systems (McCarthy, P. J. et al., Antimicrob. Agents Chemother. 28:494-499 (1985); McCarthy, P. J. et al., J. Gen. Micro. 131:775-780 (1985); Moneton, P. et al., J. Gen. Micro. 132:2147-2153 (1986); Yadan, J. C. et al., J. Bacteriol. 160:884-888 (1984)); Payne, J. W. et al., FEMS Microbiol. Letts. 28:55-60 (1985); Mehta, R. J. et al., Antimicrob. Agents Chemother. 25:373-374 (1984)). Since the polynucleotides of the present invention define the genetic loci responsible for peptide transport such polynucleotides can be used to produce plants that lack functional peptide transport systems. Such plants would be unable to transport such conjugated peptides and hence would be resistant to such pathogens. 
     In this regard, the present invention provides a method for conjugating an antimicrobial or antifungal agent or a pesticide to a peptide in order to provide a more effective treatment against such pathogens. In a similar manner, toxic peptide derivatives may be used as herbicides to eliminate undesired peptide transport proficient plants (such as weeds, etc.) that would otherwise compete with peptide transport deficient plants for soil nutrients. 
     Examples of toxic peptide or peptidyl molecules that may be used as antimicrobial, herbiciadal, or pesticidal agents include: 
     (A) metabolic toxins (such as the antifungal agent FMDP  N 3  -(4-methoxyfumaroyl)-L-2,3 diaminopropanoic acid), toxic nucleotides (such as halogenated nucleotides (e.g., 5-fluoroorotic acid), dideoxynucleotides, mutagenic nucleotide or nucleoside analogs, etc. (Kingsbury, W. D. et al., J. Med. Chem. 27:1447-1451 (1984); Andruszkiewicz, R. et al., J. Med. Chem. 30:1715-1719 (1987); Andruszkiewicz, R. et al., J. Med. Chem. 33:132-135 (1990); Andruszkiewicz, R. et al., J. Med. Chem. 33:2755-2759 (1990); Milewski, S. et al., J. Drugs Expt. Clin. Res. 14:461-465 (1988)); 
     (B) peptides that contain toxic amino acids (such as oxalysine, fluorophenylalanine, ethionine, unusual D amino acids, etc.) (McCarthy, P. J. et al., Antimicrob. Agents Chemother. 28:494-499 (1985); Marder, R. et al., J. Bacteriol. 36:1174-1177 (1978); Moneton, P. et al., J. Gen. Micro. 132:2147-2153 (1986); Mehta, R. J. et al., Antimicrob. Agents Chemother. 25:373-374 (1984); Bosrai, M. et al., J. Gen. Microbiol. 138:2353-2362 (1992)); 
     (C) toxic peptides and peptidyl molecules such as bacilysin (Milewski, S. et al., Arch. Microbiol. 135:130-136 (1983); Moneton, P. et al., J. Gen. Microbiol. 132:2147-2153 (1986); Kenig, M. et al. J. Gen. Microbiol. 94:37-45 (1976)), polyoxins (especially polyoxin D) (Becker, J. M. et al., Antimicrob. Agents Chemother. 23:926-929 (1983)), nikkomycins (especially nikkomycin Z) (Dahn, U. et al., Arch. Microbiol. 107:143-160 (1976)), and their analogs (Smith, H. A. et al., Antimicrob. Agents Chemother. 29:33-39 (1986); Naider, F. et al., Antimicrob. Agents Chemother. 24:787-796 (1983); Krainer, E. et al., J. Med. Chem. 34:174-180 (1991); Shenbagamurthi. P. et al., J. Med. Chem. 26:1518-1522 (1983); Shenbagamurthi. P. et al., J. Med. Chem. 29:802-809 (1986); Khare, R. K. et al., J. Med. Chem. 83:650-656 (1988); Emmer, G. et al., J. Med. Chem. 28:278-281 (1985); Decker, H. et al., J. Gen Microbiol. 137:1805-1813 (1991); Delzer, J. et al., J. Antibiot. 37:80-82 (1984); all herein incorporated by reference). 
     In a preferred embodiment, the peptides of such conjugates will be N-α-acetylated, since such modification facilitates the uptake of peptide molecules. 
     The impairment of the native capacity of the host plant to mediate peptide transport may be impaired in any of a variety of ways. In one embodiment, such impairment may be accomplished by mutating the normal, functional (i.e. &#34;wild-type) endogenous allele of a plant cell&#39;s peptide transport gene. Such mutagenesis may be accomplished by subjecting seedlings to mutagenic agents, such radiant energy (e.g., ultra-violet light, X-rays, etc.) or chemical mutagens. Suitable chemical mutagens include base analogs (such as, 5-bromouracil, or 2-aminopurine); deaminating agents (such as, for example, nitrous acid, hydroxylamine); alkylating agents (such as, for example, methyl methane sulfonate, ethyl methane sulfonate nitrosoguanidine); intercalating agents (such as, for example, acridine orange, ethidium bromide, psoralen.), and other mutagens. Techniques for mutagenizing nucleic acid molecules may be found in Miller, J. H. (In: Experiments in Molecular Biology, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1972)), and Silhavy, T. J., et al. (In: Experiments with Gene Fusions, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1984)). 
     It is possible that methods of site-directed mutagenesis (Itakura, K., et al., Ann. Rev. Biochem. 53:323-356 (1984), Adelman et al., DNA 2:183 (1983) and Crea et al., Proc. Natl. Acad.. Sci. (U.S.A.) 75:5765 (1978)) may be expanded to permit the use of vectors to create predefined mutations in the peptide transport polynucleotides. Such mutated molecules could then be introduced into a plant cell and permitted to recombine with the cell&#39;s endogenous peptide transport gene, to thereby produce a peptide transport deficient plant cell. 
     The successful mutation of the endogenous gene can be readily determined by evaluating the capacity of the cell or plant to take up peptides. Methods for performing such determinations are presented below. Alternatively, the cloned polynucleotide sequences can be used as probes to determine the extent of cellular transcription of the endogenous peptide transport gene. 
     In yet another embodiment, the sequences of the polynucleotides of the present invention can be used to define &#34;antisense oligonucleotides&#34; that can repress the transcription or translation of a functional endogenous peptide transport gene. Such antisense molecules can be provided to the plant via a vector, such as a CaMV vector, that expresses the antisense molecule, using a promoter such as the 35S promoter. In general, an &#34;antisense oligonucleotide&#34; is a nucleic acid (either DNA or RNA) whose sequence is sufficiently complementary to the sequence of a target mRNA molecule (or its corresponding gene) that it is capable of binding to, or hybridizing with, the mRNA molecule (or the gene), and thereby impairing (i.e. attenuating or preventing) the translation of the mRNA molecule into a gene product. To act as an antisense oligonucleotide, the nucleic acid molecule must be capable of binding to or hybridizing with that portion of target mRNA molecule (or gene) which mediates the translation of the target mRNA. Thus, antisense molecules of the present invention are capable of binding to an endogenous peptide transport gene or mRNA and inhibiting its activity. Antisense oligonucleotides are disclosed in European Patent Application Publication Nos. 263,740; 335,451; and 329,882, and in PCT Publication No. WO90/00624, all of which references are incorporated herein by reference. 
     One manner in which an antisense oligonucleotide may achieve these goals is by having a sequence complementary to that of the translation initiation region of the target mRNA molecule. The size of such an oligomer can be any length that is effective for this purpose. Preferably, the antisense oligonucleotide will be about 10-30 nucleotides in length, most preferably, about 15-24 nucleotides in length. 
     Alternatively, one may use antisense oligonucleotides that are of a length that is too short to be capable of stably hybridizing to an mRNA molecule under physiological, in vivo conditions. Such an oligonucleotide may be from about 6-10, or more nucleotides in length. To be used in accordance with the present invention, such an oligonucleotide is preferably modified to permit it to bind to a locus of the translation region of the target mRNA. Examples of such modified molecules include oligonucleotides bound to an antibody (or antibody fragment), or other ligand (such as a divalent crosslinking agent (such as, for example, trimethylpsoralin, 8-methoxypsoralin, etc.) capable of binding to a single-stranded mRNA molecules. 
     In yet another embodiment, ribozymes can be employed as inhibitors of the endogenous peptide transport gene. Ribozymes (RNA enzymes) are catalytic RNA molecules that can cleave RNA target molecules with which they hybridize (Cech, T. et al., Cell 27:487 (1981); Cech, T., Science 256:1532-1539 (1987); Cech, T. et al., Ann. Rev. Biochem. 55:599-630 (1986); James, W., Antivir. Chem. Chemother. 2: 191-214 (1991)). 
     An artificial ribozyme can be designed to specifically cleave a target RNA by flanking sequences complementary to the target (Haseloff, J. et al., Nature 334:585-591 (1988); Cameron, F. et al., Proc. Natl. Acad. Sci. U.S.A. 86: 9139-9143 (1989); James, W., Antiviral Chemistry &amp; Chemotherapy 2: 191-214 (1991). The minimum requirement for cleavage within the target RNA is the location of a suitable three base sequence GUC, GUA, or GUU preceding the cleavage site. Artificial ribozymes having a characteristic &#34;hammerhead&#34; secondary structure have been designed by Haseloff, J. et al. (Nature 334:585-591 (1988); Jeffries, A. et al., Nucleic Acids Res. 17:1371-1377 (1989); Gerlach et al. WO Patent No. 8905852 (1989); Goodchild, J. et al., Arch. Biochem. Biophys. 254:386-391 (1991); James, W., Antivir. Chem. Chemother. 2: 191-214 (1991)). 
     B. Targeted Delivery of Desired Affector Compounds 
     The capacity to control the extent of expression of plant peptide transport genes provides a means for facilitating the delivery of desired compounds into plant cells. Such desired compounds are &#34;affectors of a plant characteristic&#34; if they confer or cause a detectable change in a plant trait. Such characteristics include size, growth rate, resistance to pathogens or herbicides, color scent, nutritional value, sensitivity to cold or heat, sensitivity to drought or overwatering. The affectors of such characteristics may be nucleotides, polynucleotides, auxins, organic molecules (including proteins, peptides, pigments, perfumes), etc. A capacity to augment the cellular ability to incorporate desired peptides can be used to produce superior or more nutritious foods (Adibi, S., Metab. 36:1001-1011 (1987)). Similarly, such a capacity can facilitate the uptake of non-peptide affectors that have been conjugated or associated with a peptide, such that the affector is delivered into the plant in conjunction with the peptide (Higgins, C., Nature 327:655-656 (1987)). For example, chromogenic affectors may be conjugated to peptides in order to produce flowers having more desired coloration. Alternatively, the peptides may be conjugated to auxin affectors (such as gibberelin, indoleacetic acid, etc.) in order to facilitate plant growth and/or development. 
     The extent of expression can be controlled by providing the plant&#39;s cells with vectors that contain multiple copies of the peptide transport polynucleotides. Alternatively, such vectors may contain efficient (and/or inducible) promoters that are operably linked to the polynucleotide, and which can therefore mediate its transcription at an elevated rate. 
     In an alternative embodiment, the polynucleotides of the present invention may be joined to high efficiency promoters, and then introduced into the plant cell under conditions sufficient to recombine with the endogenous gene. Such action will result in the replacement of the endogenous promoter with a high efficiency promoter. 
     In lieu of altering the transcriptional regulation of the peptide transport gene, the methods of the present invention permit one to mutate the cloned polynucleotides in order to produce a polynucleotide that encodes a more active (or otherwise more desirable) peptide transport gene. Such desired variant genes can be readily evaluated by determining the transport capacity of yeast cells containing such variant polynucleotides, or by using the polynucleotides of the present invention as probes of mRNA transcription. 
     Having now generally described the invention, the same will be more readily understood through reference to the following examples which are provided by way of illustration, and are not intended to be limiting of the present invention. 
     EXAMPLE 1 
     Isolation of S. cerevisiae Mutants Carrying Mutations in their Peptide Transport System 
     As a means for cloning a plant peptide transport gene, the gene that controls peptide transport in S. cerevisiae was cloned. The isolation of this gene permitted the construction of a stable, transport-deficient yeast strain. 
     The ptr2 gene of S. cerevisiae was isolated by functional complementation of the dipeptide transport-deficient (ptr2 - ) phenotype. Yeast strain PB1X-9B (MATα ura3-52 leu2-3 lys1-1 his4-38 ptr2-2) was transformed with a YCp50-based S. cerevisiae genomic DNA library obtained from the American Type Culture Collection (Rose, M. D. et al., Gene 29:113-124 (1984)) (ATCC 37415). To prepare the library, bacterial cells were resuspended in 5 ml of LB broth and plated on LB plates containing 50 μg of ampicillin per ml. Approximately 10,000 clones were harvested, and the plasmid DNA was isolated by the alkaline lysis method (Sambrook, J. et al., In: Molecular Cloning A Laboratory Manual, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1989)). pZ523 columns were used to remove contaminating chromosomal DNA (Zervos, P. H. et al., Biotechniques 6:238-242 (1988)). 
     Yeast strains were transformed by the LiCl method (Ito, H. et al., J. Bacteriol. 153:163-168 (1983)). The cells were then plated on solid minimal medium (MM) supplemented with 1.3 mM L-histidine and 10 mM L-lysyl-L-leucine. The histidine served to induce the peptide transport system and to meet the auxotropic requirement conferred by the his4-38 mutation present in the host strain. L-Lysyl-L-leucine served as a source of lysine and leucine in those yeast transformants capable of transporting the dipeptide. Two yeast transformants, designated PB1X-9B(pJP1) and PB1X-9B(pJP2), were recovered after incubation at 30° C. for 5 days. 
     Whole-cell DNA, isolated from both primary yeast transformants and the transforming plasmids, was subsequently amplified and recovered in E. coil HB101. Plasmid DNA was isolated from the resulting bacterial transformants and partially characterized with restriction enzymes. Both plasmids, pJP1 and pJP2, yielded identical restriction patterns when digested with Pstl and BamHI. The ptr2 gene encodes a 602 amino acid hydrophobic polypeptide with 12 putative hydrophobic segments. The protein demonstrates all the previously identified characteristics of peptide transport in yeast. A data base search indicated the yeast peptide transporter may be the second protein discovered in a new class of membrane bound proteins (Tsay, Y-F. et al., Cell 72:705-713 (1993). The nucleotide sequence of the yeast ptr gene, and the deduced amino acid sequence of the protein is provided by Perry, J. R. et al. (In: &#34;Isolation and Characterization of a Saccharomyces cerevisiae Peptide Transport Gene,&#34; Molecular and Cellular Biology, volume 14 (1994), herein incorporated by reference). 
     Plasmid pJP2 was then reintroduced into PB1X-9B. The resulting secondary yeast transformants were tested for the ability to use a variety of dipeptides as sources of amino acids and for sensitivity to the toxic dipeptide L-alanyl-L-ethionine. Thus, strains were grown in YEPG broth at 30° C. to a titer of 10 8  cells per ml. The cells were harvested by centrifugation, washed twice with sterile water and resuspended at 1.0×10 7  cells per ml. A 5-μl aliquot was applied to solid MM containing dipeptides and amino acids as required. Four types of solid media were routinely used in assessing dipeptide utilization: MM+L-leucyl-L-leucine-L-lysine+L-histidine, MM-L-lysl-L-lysine-L-leucine-L-histidine, MM-L-lysl-L-leucine-L-histidine, and MM-L-histydyl-L-leucine-L-lysine. All dipeptides were present at a concentration of 80 μM, while amino acids and nucleotide bases were added as required at standard concentrations (Sherman, F. et al., In: Methods in Yeast Genetics, Cold Spring Harbor Laboratory, Clod Spring Harbor, N.Y. (1986)). The plates were incubated at 30° C. for 48 hours and then scored for growth. The secondary yeast transformants were able to utilize all dipeptides tested as sources of amino acids and were sensitive to the growth-inhibiting effects of L-alanyl-L-ethionine. In addition, PB1X-9B(pJP2) was able to transport radiolabeled dileucine at levels approximating those of the wild type, while the control strain PB1X-9B(YCp50), failed to accumulate the radiolabeled substrate. These results showed that the transformant had the expected wild-type phenotype and that the ptr2-2-complementing activity was plasmid-associated and not due to a reversion event at the ptr2 locus. 
     In order to form a more stable yeast ptr mutant, a one step method (Orr-Weaver, T. L. et al., Methods Enzymol. 101:228-245 (1983)) was used to cause the chromosomal disruption of the ptr gene of a non-mutant yeast strain. A 2.0-kb DNA fragment carrying the LEU2 gene of S. cerevisiae BamHI-HindIII DNA fragment from plasmid p J J283 (Jones, J. S. et al., Yeast 6:363-366 (1990)). The fragment was isolated from an agarose gel treated with T4 DNA polymerase, and then blunt-end ligated into a 653-bp deleted region of the PTR2 protein coding region of plasmid pJP15 was constructed by cloning a 1.64-kbp BamHI-EcoRI DNA fragment from plasmid pJP9 into plasmid pRS3062. This 1.65-kbp fragment contained a DNA sequence that includes 495 bp of the promoter region and 1,147 bp of the protein coding region of the ptr2 gene. Plasmid pRS3062 is a derivative of plasmid PRS306 (Sikorski, R. S. et al., Genetics 122:19-27 (1989)) in which a unique Aatll restriction endonuclease site had been removed by the digestion with Aatll, treatment with T4 DNA polymerase, and religation. The deleted region of plasmid PJ15 was generated by restriction endonuclease digestion with Aatll and Mscl, resulting in the excision of a 653-bp region that is contaminated within the PTR2 protein coding region. The ends of the deleted pJP15 molecule were made blunt with T4 DNA polymerase and ligated with the blunt-ended LEU2 DNA fragment. The resulting plasmid, pJP23(Cowan, S. W. et al., Nature 358:727-733 (1992)) was recovered in E. coil, and the structure was confirmed by restriction endonuclease analysis. Plasmid PJP23 contains the LEU2 gene oriented so that the direction of transcription opposes that of ptr2. A 2.6-kbp NdeI-Dral DNA fragment containing the inserted LEU2 gene flanked by ptr2 DNA sequences was excised and used as a substrate in transforming the ptr2 +  strain PB 1 X-2A. 
     Leu +  yeast transformants were selected on MM medium supplemented with uracil, L-lysine, and L-histidine. The resulting leu +  yeast transformants were patched onto fresh medium and then tested for the ability to use L-lysyl-L-leucine as a source of lysine in growth experiments and for sensitivity to L-alanyl-L-ethionine in disk assays. A single yeast transformant displaying the leu +  ptr -  phenotype, designated PB1X2AΔ was considered for further characterization. The integration event at the ptr2 locus was confirmed by Southern transfer hybridization analysis. 
     EXAMPLE 2 
     Isolation of Arabidopsis thaliana cDNAs Capable of Complementing S. cerevisiae PTR Mutants 
     The isolation of plant genes responsible for peptide transport was accomplished by preparing cDNA from the grass, Arabidopsis thailiana, and then determining whether that cDNA was capable of complementing the PTR deficiency of the above-described yeast mutants. 
     An Arabidopsis thaliana cDNA library was obtained from Minet, F. et al. (Centre National de la Recherche Scientifique, Gif sur Yvette, France). The cDNA of the library was prepared from the mRNA of complete young seedlings (stage II leaves) including roots of Arabidopsis thaliana (L). Heynh (Landsberg erecta ecotype). The cDNAs were ligated to CACA adapters and then inserted into BstXI sites flanked by Notl sites in the yeast/E. coil expression vector pFL61 (Minet, M. et al., Plant J. 2:417-422 (1992)). Expression in yeast is controlled by the phosphoglycerate kinase (PGK) promoter. 
     For amplification and storage, the library was maintained in E. coil strain DH5α (supE44 hsdR17 recA1 gyrA96 thi-1 relA1). Yeast hosts used were S288C (MATα SUC2 mal mel gal2 CUP1), PBIX-9B (MATα ura3-52 leu2-3,112 lys1-1 his4-38 ptr2-2), PB1X-2A (MATα ura3-52 leu 2-3, 112 lys1-1 his4-38 ptr2-2), and PBIX-2AΔ (MATα ura3-52 leu2-3, 112 lys1-1 his4-38 ptr2::leu2). All yeast strains, except PB1X-2AΔ, were constructed using the methods described by Sherman, F. et al., In: Methods in Yeast Genetics, Cold Spring Harbor Laboratory, Clod Spring Harbor, N.Y. (1986), and by Perry, J. R. et al. (In: &#34;Isolation and Characterization of a Saccharomyces cerevisiae Peptide Transport Gene,&#34; Molecular and Cellular Biology, volume 14 (1994), both herein incorporated by reference). As indicated above, PB1X-2AΔ was generated from strain PB1X-2A using a one-step gene disruption/replacement strategy (Rothstein, R. J. et al., Methods Enzymol. 101:202-211 (1983)) where a 653-bp region internal to the coding region was deleted and replaced by 2.0 kb fragment containing the LEU2 gene of S. cerevisiae. 
     S. cerevisiae S288C, PB1X-9B, PB1X-2A, and PB1X-2AΔ were maintained on YEPD agar containing (w/v) 1% yeast extract-2% Bacto-Peptone (Difco Laboratories, Detroit Mich.) and 2% glucose. All experiments conducted with these strains were done in synthetic complete medium (SC) containing yeast nitrogen base (Difco) without amino acids and ammonium sulfate, 1 mg of allantoin per ml, 2% glucose and amino acid supplements as indicated. Amino acids were supplied as 0.15 mM unless indicated otherwise. Solid media contained 2% agar or 2% nobel agar in the case of disk assays. All yeast strains were incubated at 30° C. E. coil strain DH5α was routinely maintained on SOB medium (Sambrook, J. et al., In: Molecular Cloning A Laboratory Manual, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1989)) while transformed DH5α strains were grown on LB medium plus 100 ml ampicillin at 37° C. 
     The Saccharomyces cerevisiae strains PB1X-9B and PB1X-2AΔ, which carry mutations in leucine, histidine, and lysine biosynthesis as well as in peptide transport, are unable to grow on minimal medium supplemented with dipeptides containing amino acids which satisfy the auxotrophic requirements of the mutants. To isolate a plant gene which codes a peptide transporter, strains PB1X-9B and PB1X-2AΔ were transformed with the cDNA library (Gietz, D., et al., Nuc. Acid. Res 20:1425 (1992)) and transformants were selected on SC media supplemented with L-leucine, L-lysine, L-histidine (100 μM), washed from plates with sterile dH20 and selected on dipeptide media (SC plus 80 μM his-leu, and 80 μM lys-leu). A total of 21 clones were recovered (15 from PB1X-9B and 6 from PB1X-2AΔ). Colonies were reselected on solid dipeptide medium and those colonies able to grow were analyzed on drop out plates and plasmid cured to show concomitant loss of the selectable marker and peptide transport phenotypes. Plasmid DNA was isolated and reintroduced into both PB1X-9B and PB1X-2A. Plasmids able to restore the growth of the mutants on dipeptide media were recovered, purified and analyzed further. 
     Two clones from each group were able to restore peptide transport. Notl restriction analysis of the two PB1X-2AΔ transformants showed an identical insert of 2.0 kb (designated pDTF1 and pDTF2) and the two PB1X-9B transformants showed an identical insert of 2.8 kb (pPTF3 and pFTF4). The remaining clones showed either no insert at all or multiple bands upon restriction with Notl. The 2.0 kb transformants pDTF1 and pDTF2 did not show sensitivity to toxic peptides (discussed below) while the 2.8 kb transformants, pPTF3 and pPTF4 displayed sensitivity to all peptides tested. Plasmids pPTF3 and pPTF4 transformed into the deletion strain PB1X-2A showed identical phenotypes to that of pPTF3 and pPTF4 transformed into the PB1X-9B genetic background as judged by growth on peptides and disk assay. By southern hybridization, an α- 32  P labeled probe consisting of the entire Notl 2.8 kb insert hybridized to uncut, and Notl digest pPTF3 and pPTF4 plasmid DNA but not to uncut and Notl digested pDTF1 or pDTF2 plasmid DNA. Based on these results, the 2.8 kb plasmid pPTF4 was chosen for further analysis. Plasmid pPTF4 was found to comprise cDNA for an Arabidopsis peptide transport protein. 
     The Arabidopsis gene carried within the 2.8 kb insert of plasmid pPTF4 was designated &#34;atptr2a,&#34; and the protein encoded by this gene was termed &#34;ATPTR2Ap protein.&#34; The sequence of the atptr2a cDNA is presented herein as SEQ ID NO:1; the deduced sequence of the ATPTR2Ap protein is presented herein as SEQ ID NO:2. 
     The Arabidopsis gene carried within the 2.0 kb insert of plasmid pDTF1 was designated &#34;atptr2b,&#34; and the protein encoded by this gene was termed &#34;ATPTR;2Bp protein.&#34; The sequence of the atptr2b cDNA is presented herein as SEQ ID NO:3; the deduced sequence of the ATPTR2Bp protein is presented herein as SEQ ID NO:4: 
     In sum, functional complementation of yeast mutants has been used successfully to clone plant polynucleotides that are capable of complementing a yeast PTR deficiency. The method permits the rapid identification of those plant genes that are functionally homologous to yeast genes. Although functional complementation has been used to clone a number of plant transport genes including potassium ion transporters, a sucrose transporter and two amino acid permeases, its applicability requires not only well characterized yeast mutants, but also the capacity of the plant gene to function in the yeast. Thus, the applicability of the method to the cloning of a particular plant gene cannot be assessed in advance. Expression of plant genes in yeast also affords greater flexibility in analyzing the functional characteristics of the protein product. 
     EXAMPLE 3 
     Sequence Analysis of Cloned Arabidopsis thaliana cDNA 
     The nucleotide sequence of the Arabidopsis cDNA that complemented the PTR yeast deficiency was determined using the dideoxy chain-termination sequencing method of Sanger, F. et al. (Proc. Natl. Acad. Sci. (U.S.A.) 74:5463-5467 (1977)) using Sequenase Version ;2.0 (United States Biochemical, Cleveland, Ohio). A Notl, 2.8 kb cDNA fragment was cloned into Bluescript SKII (Stratagene, La Jolla, Calif.). An Exolll/Mung Bean deletion kit (Stratagene, La Jolia, Calif.) was used to generate a deletion series of the fragment. Double-stranded template DNA was sequenced using T 3  and M13 primers of pBluescript. Standard molecular techniques, unless otherwise stated, were performed according to Sambrook, J. et al. (In: Molecular Cloning A Laboratory Manual, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1989)). Nucleotide and amino acid sequence analysis and comparisons were performed with the NCBI BLAST algorithm search program (Altschul, S. F. et al., J. Molec. Biol. 215:403-410 (1990)). 
     Such DNA sequence analysis of insert isolated from pPTF4 showed a 1833 bp open reading frame within the 2799 bp insert (FIG. 1 ). The open reading frame encoded a polypeptide of 610 amino acids (67,510 d). Hydropathy analysis (Kyte, J. et al., J. Molec. Biol 157:105-132 (1982)) showed the predicted protein, ATPTR2Ap, to be highly hydrophobic with 10-12 putative transmembrane domains. Four potential glycosylation sites were identified which favor a 12 transmembrane domain configuration. A search of the protein sequence data base using the NCBI BLAST algorithm (Altschul et al. 1990) revealed homologies to the yeast peptide transporter YSCPTR2p (probability High Score 654, 52% identity, 68% similarity) and to the A. thaliana nitrate transporter ATHCHL1p (Tsay, Y. F. et al., Cell 72:705-713 (1993)) (probability High Score 82, 36% identity, 47% similarity). FIG. 1 shows the nucleotide sequence of the atptr2a cDNA (SEQ ID NO:1) of plasmid pPTF4 and the deduced amino acid sequence of the encoded ATPTR2Ap protein (SEQ ID NO:2). FIG. 2 shows the nucleotide sequence of the atptr2b cDNA (SEQ ID NO:3) of plasmid pDTF1 and the deduced amino acid sequence of the encoded ATPTR2Bp protein (SEQ ID NO:4). 
     Protein sequences from ATPTR2A, SACPTR2, and ATHCHL1A were aligned with the program Pileup in the sequence analysis software package GCG (Devereux, J. et al., Nuc. Acids Res. 12:387-395 (1984); Genetics Computer Group 1991: The Program Manual for the GCG Sequence Analysis Software Package, Version 7, University Research Park, Madison, Wis. (1991)), and a consensus sequence was generated with the GCG program, Pretty, from the alignment generated with Pileup. Pileup aligns a group of related sequences using progressive pairwise alignments. The gap weight was 3.0 and the gap length weight was 0.10. A consensus sequence was generated by the GCG program, Pretty, using the output from Pileup. The consensus was generated at a minimum plurality of 2.00. 
     Protein sequences reported to be involved in peptide transport plus sequences from the ABC transporter superfamily were aligned again using the GCG Pileup program to produce a dendrogram displaying the sequence similarity relationships amongst all the proteins. The clustering strategy represented by the dendrogram is called UPGN1A (unweighted pair-group method using arithmetic averages which scores the similarity between every possible pair of sequences. The similarity scores are then used to create a clustering order that can be translated into a dendrogram where the horizontal branch lengths are proportional to the similarity between the sequences. The following data bases were used in the searches: GenBank, release 78.0; EMBL (Modified), release 35.0; Swiss-Prot, release 26.0 
     The sequence similarities divided into two groups. The first group (Group I) included proteins generally associated with ATP binding or those identified as having an ATP binding consensus sequence. The second group (Group II) included proteins containing hydrophobic segments and generally thought to be membrane bound. Within Group II, the ATPTR2A, SACPTR2, ATHCHL1A, and CaPTR (a Candida albicans peptide transporter) proteins comprised a smaller group distinct from any of the other groups in the analysis. 
     EXAMPLE 4 
     Peptide Transport Characteristics of the ATPTR2A and ATPTR2B Genes 
     The yeast peptide transport system has been shown to transport a wide variety of peptides with little discrimination between amino acid side-chains. To test whether this was the case for the plant transporter, a number of peptides varying in both composition and length were examined for their ability to support growth of pPTF4-transformed yeast. 
     Thus, the peptide transport mutant PB1X-9B and deletion strain PB1X-2AΔ transformed with plasmids pPTF4 (ATPTR2A) or pDTF1 (ATPTR2B) were grown on various peptides to assess the specificity of the plant peptide transporter. In addition, untransformed PB1X-9B, PB1X-9B transformed with plasmid pJP9 encoding the above-described yeast peptide transport gene, PB1X-2AΔ and PB1X-2A, the ptr2 +  parental strain to PB1X-2AΔ strain, were also assayed. Each strain was grown overnight in SC media plus uracil (non-transformed) or minus uracil (transformed) plus amino acids to stationary phase and harvested by centrifugation. Cells were then washed twice with sterile dH 2  O and resuspended at 5×10 6  cells/ml. 5 μl of each suspension was applied as a small spot to a 2 ml volume of solid media in a 24 well plate. All peptides were suspended in sterile, deionized water and added to an equal volume of SC medium plus the appropriate amino acids and uracil when required. The medium for each assay thus consisted of SC medium plus or minus uracil supplemented with 80 μM of a specific peptide and auxotrophic requirements minus the amino acid components of the added peptide. The plates were incubated at 30° C. for 72 hrs. and then scored for growth. Growth was scored as uniform colony formation compared to negative controls which showed no growth. 
     The mutant PBIX-9B was incapable of growing on any of the peptides. PBIX-9B transformed with pJP9 containing the yeast peptide transport gene showed growth on all peptides except tri-Lys, tetra-Lys (SEQ ID NO:5), poly-Lys, Met-M et-Leu and peptides longer than 3 amino acids (i.e. Gly-Leu-Gly-Leu (SEQ ID NO:6), Thr-Pro-Arg-Lys (SEQ ID NO:7), Tyr-Gly-Gly-Phe-Leu (SEQ ID NO:8), Trp-His-Trp-Leu-Gln-Leu (SEQ ID NO:9)). The plant peptide transport gene showed a similar pattern to that of yeast except that it was able to utilize Met-M et-Leu. The parent strain to the yeast peptide transport mutant PBIX-9B, PBIX-2A (his, leu, lys, ptr) also did not utilize Met-M et-Leu (data not shown). The results indicate that ATPTR2Ap transports both di- and tripeptides with a slightly different specificity than that of SACPTR2p (Table 1; N/A indicates not applicable due to the restoration of leucine prototrophy caused by the insertion of the leu2 gene in the host strain). 
     
                                           TABLE 1__________________________________________________________________________                PBIX-9B                     PBIX-9B                          PBIX-2AΔPeptide        PBIX-9B                (pJP9)                     (pPTF4)                          (pDTF1)__________________________________________________________________________Ala--Eth       R     S    S    RLys--Leu       -     +    +    N/AHis--Leu       -     +    +    N/AHis--Lys       -     +    +    +Lys--Lys       -     +    +    +tri-Lys        -     -    -    -tetra-Lys      -     -    -    -poly-Lys       -     -    -    -Leu--Leu       -     +    +    N/Atri-Leu        -     +    +    N/AAla--Leu       -     +    +    N/AAla--Ala--Leu  -     +    +    N/AAla--Lys       -     +    +    +Lys--Ala--Ala  -     +    +    +Met--Met--Leu  -     -    -    N/AGly--Leu--Gly--Leu          -     -    -    N/AThr--Pro--Arg--Lys          -     -    -    -Tyr--Gly--Gly--Phe--Leu          -     -    -    N/ATrp--His--Trp--Leu--Gln--Leu          -     -    -    -SC--Ura        +     +    +    +__________________________________________________________________________ 
    
     EXAMPLE 5 
     Capacity of the ATPTR2A Gene to Alter Cellular Resistance or Sensitivity to Toxic Peptides 
     As indicated above, peptides are frequently associated with plant diseases, exerting toxic or hormone-like effects on plant growth. Plants that are incapable of transporting such toxic peptides are resistant to such peptides. Such resistance can be obtained by mutating the ptr genes of the plant genome. Indeed, peptides containing a toxic amino acid analog have been used to characterize peptide transport (Island, M. D. et al., J. Bacteriol. 169:2132-2136 (1987)) and to isolate peptide transport genes (Island, M. D. et al., Curr. Genet. 20:457-463 (1991)). 
     Since ptr mutants are deficient in peptide transport, they are unable to take up toxic peptides. This inability renders such mutants resistant to the toxic effect of the peptides. In order to determine whether the polynucleotides of the present invention could restore toxic peptide sensitivity to ptr2 mutants, the sensitivity of plasmid-transformed cells was determined. Sensitivity to toxic amino acids and peptides was measured as described by Island, M. D. et al. (J. Bacteriol. 169:2132-2136 (1987)) Briefly, a filter disk containing 0.38 μmoles of the toxic compound was placed on a lawn containing 5×10 6  cells and the plate incubated at 30° C for 1 to 2 days. Resulting halos were measured across their diameter. The toxic dipeptides Leu-Eth, Ala-Eth, Leu-F-Phe and Oxalysine were synthesized by standard solution phase techniques (Naider, F. et al., J. Biol. Chem. 249:9-20 (1974). The results of this experiment are shown in Table 2 (values are the mean of the diameters of the observed zone of inhibition in millimeters±standard error of the mean of at least two independent experiments). 
     
                       TABLE 2______________________________________        Strain                  PB1X-   PB1X-9B                                 PB1X-9BToxic Peptide  S288C   9B      (pJP9) (pPTF4)______________________________________Eth            39.0 ±                  44.5 ±                          46.5 ± 1.5                                 46.5 ± 0.5          3.0     3.5F--Phe         25.0 ±                  14.0 ±                          20.0 ± 0.0                                 19.5 ± 0.5          4.0     1.0Leu--Eth       36.0 ±       47.0 ± 1.0                                 45.0 ± 1.0          2.0Ala--Eth       33.5 ±       42.5 ± 2.5                                 35.0 ± 1.0          2.5Leu--F--Phe    28.0 ±       20.5 ± 3.0                                 37.0 ± 1.0          4.0Lys--Ala--Eth  26.0 ±       36.0 ± 1.5                                 37.5 ± 1.5          3.0Lys--Leu--Ala--Eth          0       0       0      0Lys--Leu--Leu--Ala--Eth          0       0       0      0Lys--Leu--Eth  30.0 ±       36.0 ± 0.5                                 35.0 ± 1.0          0.0Lys--Leu--Leu--Eth          0       0       0      0Lys--Leu--Leu--Leu--Eth          0       0       0      0______________________________________ 
    
     The peptide transport mutant PBIX-9B was found to be resistant to peptides containing the toxic amino acid analog ethionine. Transformation of PB1X-9B with the plasmid-borne yeast peptide transport gene restored sensitivity to these toxic compounds. PBIX-9B transformed with pPTF4 also restores sensitivity to the toxic dipeptides Ala-Eth, Leu-Eth and Leu-f-Phe (Table 2). The halos obtained on S288C and PB1X-9B (pJP9) with leu-F-Phe exhibited a hazy background within the halo; the halo obtained on PB1X-9B (pJP9) with Lys-Ala-Eth exhibited a broad border around within the halo. 
     The experiment thus demonstrates that whereas PBIX-9B showed complete resistance to the toxic peptides, both the mutant and transformant are sensitive to ethionine and fluorophenylalanine (F-Phe). In addition, the deletion strain PBIX-2AΔ also showed complete resistance to the toxic peptides. None of the strains tested were sensitive to Lys-Leu-Ala-Eth, Lys-Leu-Leu-Ala-Eth or to Lys-Leu-Leu-Eth, Lys-Leu-Leu-Leu-Eth. Both the yeast and plant peptide transporter showed similar patterns of sensitivity to toxic peptides with the plant peptide transporter expressed in yeast. 
     The yeast peptide transport mutant transformed with the Arabidopsis peptide transport gene thus showed similar sensitivity, as measured by halo size, and specificity to a range of toxic peptides as that of Saccharomyces wild type or peptide transport mutant transformed with the yeast peptide transport gene. Both transformants and wild type (S288C) are most sensitive to ethionine and ethionine containing peptides which produce the largest halos and appear less sensitive to fluorophenylalanine and Leu-f-Phe which is consistent with the data of Island, M. D. et al. (J. Bacteriol. 169:2132-2136 (1987)). S288C and the transformants are not sensitive to any of the toxic peptides with chain lengths four residues and longer. The data indicate this is most likely due to chain length as the tri-peptides Lys-Ala-Eth and Lys-Leu-Eth were toxic to both wild type and transformants while the longer peptides of similar composition were not toxic to the cells (Table 2). This is consistent with reports that wild type Saccharomyces cerevisiae does not readily transport peptides four residues and longer (Becker, J. M. et al., In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 257-279 (1980)). However, this inability to take up longer peptides has not been tested with a wide range of peptides varying in amino acid side chain composition. 
     EXAMPLE 6 
     ATPTR2A-Mediated Uptake of Peptides in S. cerevisiae 
     The kinetics of ATPTR2A-mediated transport of peptides in yeast was evaluated by transforming pPTF4 into the S. cerevisiae peptide transport mutant, PBIX-9B and measuring the uptake of tritiated Leu-Leu dipeptide. 
     L-leucyl-L   3  H!leucine trifluoroacetic acid (TFA) was synthesized by standard solution phase techniques (Naider, F. et al., J. Biol. Chem. 249:9-20 (1974)). Uptake of L-leucyl-L- H!leucine was performed as by Island, M. D. et al. (J. Bacteriol. 169:2132-2136 (1987)), with the following modifications. Cells were grown to late log phase (2-6×10 7  cells/ml) overnight in SC with 2% glucose, 1 mg/ml allantoin plus amino acids to supplement auxotrophic markers. To induce peptide transport. 5-15 ml from this culture was added to 100 ml fresh medium such that the density was 3.0×10 6  cells/ml. This culture was allowed to grow (approx. 2 hrs.) to a density of 6.0×10 6  cells/ml and then harvested by centrifugation. The pelleted cells were washed twice with 10 ml cold dH 2  O and suspended in cold 2% glucose to a final concentration of 2×10 8  cells/ml and incubated at 30° C. for 15 min. 500 μl of cells were then added to an equal volume of reaction mixture (30° C.) and incubated at 30° C. At 20, 40, 60, 90, and 120 sec. intervals, 190 μl portions were removed, filtered over filters (pore size, 0.45 μm; GN-6; Gelman Sciences, Inc., Ann Arbor, Mich.) and washed 2 times with 5 ml cold, sterile dH 2  O and once with 5 ml dH 2  O at room temperatures. Filters were placed in scintillation vials with 5 ml of Budget-Solve scintillation cocktail (Research Products International Corp., Mount Prospect, Ill.) and counted (liquid scintillation counter; LS-7000; Beckman Instruments, Inc., Fullerton, Calif.). The final concentration of the components in the uptake assay was 1% glucose, 40 mM sodium citrate-potassium phosphate buffer (pH 5.5), and 1.5×10 5  M L-leucyl-L-  3  H!leucine (specific activity, 10 mCi/mmole). Uptake is expressed as nanomoles per mg dry weight. 
     Transformation with pPTF4 restored  H 3  !-dileucine uptake to wild-type levels (FIG. 3). Uptake of the radiolabeled substrate could be inhibited with 100-fold cold dileucine and 100-fold cold leucine had no effect on the uptake rate. Uptake rates conferred by the plant peptide transporter are also consistent with uptake rates of PBIX-9B transformed with the yeast peptide transporter. A number of peptides could compete for uptake of  H 3  !-dileucine and uptake competition similar to that seen for Leu-Leu was also seen for Ala-Ala, Ala-Ala-Ala, Ala-M et, Met-Met-Leu, Met-Met and Leu-Phe in PBIX-9B transformed with pJP9 or pPTF4. γ-aminolevulinic acid, which is structurally similar to glycyl-glycine, and recently shown to be transported by the dpp operon in both E. coil and Salmonella typhimurium (Elliot, T. et al., J. Bacteriol. 175:325-331 (1993); Verkamp, E. et al, J. Bacteriol. 175:1452-1456 (1993)), did not compete with dileucine for uptake in PBIX-9B pPTF4! while ALA was able to compete with radiolabeled dileucine uptake in PBIX-9B pJP9!, the yeast peptide transport system. 
     Yeast cells transformed with the plant peptide transport gene were thus able to take up radiolabeled dileucine to a level comparable to that of wild type. The fact that excess leucine did not reduce uptake indicated that the peptide is not transported via an amino acid transporter. Transport of dileucine was found to be inhibited by a number of peptides containing hydrophobic residues. This finding is consistent with the data from the peptide growth experiment and supports a strong bias toward transport of peptides composed in part or entirely of hydrophobic residues such as Ala-Ala, tri-Ala, Gly-Ile, Val-Val, Phe-Ala-Glu, Leu-Leu, Leu-Gly (Sopanen, T. et al., FEBS Lett. 79:4-7 (1977); Higgins, C. F. et al., Planta 138:211-216 (1978); Higgins, C. F. et al., Planta 142:299-305 (1978)). These studies also showed that Gly-Gly was a poor competitor for substrates such as Gly-Ile, tri-Ala and Ala-Ala which is supported by lack of inhibition of dileucine transport by ALA, a Gly-Gly analog, in yeast cells transformed with the plant peptide transport gene. 
     EXAMPLE 7 
     Sensitivity of A. thaliana to Toxic Peptides 
     To determine if the experimental results obtained with ATPTR2Ap expressed in yeast were comparable to ATPTR2Ap expressed in an Arabidopsis genetic background, toxic peptides were applied to Arabidopsis seedlings in an experiment analogous to the disk assay. Thus, A. thaliana seeds and seedlings were exposed to Ethionine, Ala-Eth, Leu-Eth, Leu-fluorophenylalanine or oxalysine containing peptides, and the minimum inhibitory concentrations (MIC) were determined for each of the toxic compounds. 
     Approximately 15 A. thaliana seeds were placed in a row at one end of 10 cm plate containing 20 ml of Arabidopsis growth media (Kranz and Kirchheim 1987). The seeds were incubated 3-5 days in the light with the plate set in an upright position. When the roots were approximately 1-2 cm long, sterile paper filter disks were placed immediately in front of the root tips on the right and left side of the plate 2 cm from the edge of the plate. A line was drawn across the plate using the top of the disks as a guide marking zero growth. 5 μl of toxic amino acid analog, toxic peptide, or toxic peptide plus competitor was added to one disk while H 2  O was place on the other disk. The plates were incubated for an additional 3-5 days. The average length of the roots was measured from the line and the results expressed as a percentage of control root growth. 
     To measure the minimum inhibitory concentration of the toxic peptides, 10 to 15 A. thaliana seeds were place on solid Arabidopsis growth media with decreasing concentrations of toxic peptide. The seeds were incubated for 4 days in the dark and then scored for germination. 
     Ala-Eth, Leu-Eth and Oxa-Lys were found to inhibit germination of A. thaliana seeds and root elongation of seedlings at 0.038 μmoles while ethionine inhibited germination and root elongation at 0.0038 μmoles. Both seed germination and root elongation was not inhibited by Leu-f-Phe. This inhibition did not appear to effect other parts of the plant as the leaves looked comparable to the unaffected control. Seeds exposed to ethionine, ethionine containing peptides as well as oxalysine (a toxic lysine analog) germinated and grew a root 1-2 mm in length after which growth was arrested suggesting that this peptide transport gene is not expressed immediately upon imbibation and germination but later, after the emergence of the root primordia. 
     Competitor peptides added with the toxic peptides showed differences in their ability to reverse toxicity of the ethionine containing peptides in the root assay. Ala-M et and Met-Met were able to reverse the toxicity of Ala-Eth which might be expected considering the similarity in structure. This was also the case for Leu-M et and Met-Met reversing the toxicity of Leu-Eth. Met, Ala-Ala, Ala-Ala-Ala, and ALA were unable to reverse the inhibition of root growth mediated by Ala-Eth or Leu-Eth (Table 3). 
     
                       TABLE 3______________________________________         Toxix PeptideCompetitor      Ala--Eth Leu--Eth______________________________________Met             0        0Ala--Ala        0        0tri-Ala         0        --Met--Met        40       --Ala--Met        70       --Leu--Met        --       100ALA             0        0______________________________________ 
    
     A common feature between the yeast and plant peptide transporter is the lack of side-chain specificity of each of the peptide transport systems. In the results of the peptide growth assay, both systems are able to take up and utilize peptides which, in general, have a hydrophobic character to them. These peptides contain one or more of the hydrophobic amino acids alanine, leucine, or methionine. This was also generally the case with earlier work on S. cerevisiae and the barley system. Peptides containing two or more lysines did not support the growth of either the plant or yeast transformants. This finding is consistent with previous work which showed that peptides containing basic amino acids such as histidine or lysine or peptides with glycine as a component, did not support growth in yeast (Lichliter, W. D. et al., Agents Chemother 10:483-490 (1976); or plants (Sopanen, T. et al., Plant Physiol. 61:630:633 (1978); Higgins, C. F. et al., Planta 138:217-221 (1978); Higgins, C. F. et al., Planta 142:299-305 (1978)). The results from the toxic peptide disk assays also demonstrate little difference in specificity between the plant and yeast peptide transport systems (Table 2). One notable difference is the plant gene confers greater and more complete sensitivity, as judged by size and appearance of the halo, to leucine-fluorophenylalanine that does the yeast transport gene. Since very few phenylalanine containing peptides were tested, it is difficult to conclude whether this difference has any significance for the interaction of the peptide with its binding site between the two transporters. 
     EXAMPLE 8 
     ATPTR2A Expression in A. thaliana 
     The isolation of the ATPTR2A cDNA provided a probe capable of measuring the extent of ATPTR2A transcription in plant tissue. 
     The expression of atptr2a was determined by reverse transcription-polymerase chain reaction (RT-PCR). Reverse transcription and PCR were performed as described by Sambrook, J. et al. (In: Molecular Cloning A Laboratory Manual, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1989)).). Total RNA (10 μg), from roots and leaves of 7 day old Arabidopsis seedlings grown on defined media under sterile conditions, was pretreated with RNase-free DNase and reverse transcribed with AMV reverse transcriptase using an oligo dT primer. The first-strand synthesized cDNA (treated with RNase A) was amplified by PCR (94° C., 1 min.; 55° C., 1.5 min.; 72° C., 1.5 min.; 30 cycles) by Taq polymerase (Promega Corp. Madison, Wis.). The primers used were an upstream primer starting at base 1975 (SEQ ID NO:10): 
     
         SEQ ID NO:10 GCTTCCATGATTTACGCTGC 
    
     and a downstream primer starting at base 2528 (SEQ ID NO:11): 
     
         SEQ ID NO:11 GCATAAACGCCTACCGG 
    
     The primers generate a 569 bp fragment of the open reading frame of atptr2a. The amplified DNAs were electrophoresed and transferred to nitrocellulose filters. The filters were probed with an α- 32  P-dCTP labeled 720 bp BamHI-Notl DNA fragment from plasmid pFL61 containing the atptr2a gene. The blots were exposed to autoradiographic film at -80° C. for 24 hrs. The blots revealed that atptr2a expression occurs in the roots of in vitro grown Arabidopsis seedlings. The probe also hybridized to total RNA from seedling leaves, and PCR generated products from plasmid pFL61 harboring the atptr2a gene and Arabidopsis genomic DNA. 
     The results indicate that Arabidopsis seedlings germinated under defined growth conditions expressed the ATPTR2A peptide transporter in the roots and the leaves. This data supports the results of the root assay indicating that Arabidopsis seedlings express a root specific peptide transporter which can transport toxic and non-toxic peptides. 
     Transport has been reported in root tips and aleurone layers of germinated barley grains but at uptake levels less than 1% of that seen with scutella (Sopanen, T. et al., Plant Physiol. 61:630:633 (1978)). Results from the seed and seedling experiments, in which Arabidopsis seeds exposed to toxic peptides were able to germinate and inhibition of root growth by toxic peptides occurred with roots 1-2 cm in length, indicated that the expression of the peptide transporter reported here is root and not seed specific which would imply a transport system different from that described for barley grains. However, this difference may be more related to expression of the target of the toxic amino acid analog rather than the ability to transport the peptide. Indeed, Payne, J. W. et al. (Planta 170:263-271 (1987)) identified two proteins which were shown to be involved with peptide transport in barley grains, one of which was approximately 65-67 kd in size which is in good agreement with the 67.5 kd size predicted for ATPTR2Ap. These proteins become detectable in a scutellar epithelia extract after 15 hrs. imbition, coincident with an increase in peptide transport activity, and remain present three days after the onset of germination. This lag in protein expression is similar to the lag in toxicity seen in germinating Arabidopsis seeds which may indicate that the peptide transport system identified here is similar or identical to the one described for barley grains. 
     Clearly, from a physiological standpoint, the Arabidopsis peptide transporter exhibits transport characteristics similar to that of the yeast peptide transporter including transport of peptides with similar chain length and composition as well as inhibition of transport by various competing peptide substrates. Sequence comparison between these two proteins also shows considerable similarity at the sequence level. Adding the ATHCHL1A sequence to the comparison produces a consensus sequence which shows homology generally confined to the hydrophobic segments of each of the polypeptides. This result, however, may have more to do with these proteins presumably being membrane bound rather than their function as transporters. When these same proteins, including the CaPTR protein, are compared to other transport proteins, they clearly comprise a distinct, separate group, designated Group III. Since other proteins in this comparison also contain hydrophobic segments, such as the Tap and Mdl proteins and the b and c components of the bacterial transporters, and they are not grouped along with Group Ill proteins, the resulting clustering order indicates conserved consensus sequences among particular groups of proteins which are conserved for other reasons than their association with a particular subcellualr structure. Interestingly, the most closely related group to Group III is composed of two clusters of proteins (Group IV and Group V) reported to be the membrane bound components of bacterial peptide transporters (Perego, M. et al., Mol. Microbiol. 5:173-185 (1991); Rudner, D. Z. et al., J. Bacteriol. 173:1388-1398 (1991); Mathiopoulos, C. et al., Mol. Microbiol. 5:1903-1913 (1991); Hiles, I. D. et al., J. Molec. Biol 195:125-142 (1987); Alloing, G. et al., Mol. Microbiol. 4:633-644 1990)). These proteins are postulated to mediate the passage of peptides across the plasma membrane (Pearce, S. R. et. al, Mol. Microbiol. 6:47-57 (1992)). So, while these three groups of proteins have similar topology and function, their sequence conservation suggests they evolved into separate families of proteins. 
     Other functions of plant peptide transport other than a nutritional one postulated for barley grains are not known, though a wide range of peptides and peptide compounds are known to occur in plants (Higgins, C. F. et al., In: Encyclopedia of Plant Phsyiology, N.S., volume 14A, Boulter, D. et al. (eds.) Springer, N.Y., pp. 438-458 (1982)). Clearly, more research in this area is necessary. Isolation of a plant peptide transport gene does bring about the possibility of exploiting this system for delivery of toxic or growth promoting substances to plants in a manner analogous to that postulated for human pathogens (Fickel, T. E. et al., Nature New Biol 241:161-163 (1973); Higgins, C. F. et al., Nature 327:655-656 (1987)). 
     Thus, the above-described yeast mutants were used to clone an Arabidopsis thaliana peptide transport gene that was capable of functionally complementing the yeast peptide transport mutant. The plant peptide transporter (ATPTR2Ap) conferred growth on di- and tripeptides but not peptides four residues and higher. The plant peptide transporter also conferred sensitivity to a variety of ethionine-containing, toxic peptides of chain length three or less, and the ability to take up radiolabeled dileucine at levels similar to wild type. Dileucine uptake was reduced by the addition of a variety of growth-promoting peptides. Root growth of A. thaliana seedlings exposed to ethionine-containing, toxic peptides was inhibited and growth could be restored by addition of various peptides shown to compete with dileucine uptake in yeast expressing the A. thaliana transport gene. The peptide transporter is expressed in the roots and leaves of A. thaliana seedlings. The sequence of a cDNA insert of 2.8 kb indicated an open reading frame encoding a 610 amino acid polypeptide (67.5 kd). Hydropathy analysis predicted a highly hydrophobic protein with 12 potential hydrophobic segments. The plant peptide transporter shows homology to ATHCHL1A, the nitrate inducible nitrate transporter and considerable homology to the S. cerevisiae peptide transporter SACPTR2, but little homology to other proteins known to be involved in peptide transport. This represents the first reported sequence of a plant peptide transporter and the third protein identified in a potentially new family of membrane transport proteins. 
     The recognition that the yeast and plant peptide transport systems share a number of characteristics supports the idea that structural components of these systems may be homologous. In separate studies with Saccharomyces cerevisiae and barley grains, competition experiments demonstrated complete inhibition of dipeptide uptake by tripeptides, and vice versa, indicating that the same peptide transport system transports both di- and tri-peptides (Sopanen, T. et al., FEBS Lett. 79:4-7 (1977); Higgins, C. F. et al., Planta 138:217-221 (1978); Marder, R. et al., J. Bactiol. 131:906-916 (1977); Becker, J. M. et al., Arch. Biochem. Biophys. 178:245-255 (1977)). 
     Transport of peptides containing D-residues is reduced in both plants and yeast although this is somewhat position dependent. D-residues at the C-terminal end of the peptide are not transported in plants while peptides with D-residues at the N-terminus are taken up but at a reduced rate (Higgins, C. F. et al., Planta 142:299-305 (1978); Higgins, C. F. et al., Planta 138:211-216 (1978)). Similar results have been obtained in yeast in that although peptides with a D-residue at the C-terminus are transported, such transport is at a lower rate than those with D-residues at the N-terminus (Becker, J. M. et al., In: Microorganisms and Nitrogen Sources, Payne, J. W. (ed.), John Wiley and Sons, Inc., pp. 257-279 (1980)). 
     A number of similarities are present concerning the energetics of both peptide transport systems. Both have an acidic pH optima for transport (pH 5.5 for yeast, pH 3.8 for barley seeds) and both exhibit saturation kinetics (Higgins, C. F. et al., Planta 138:217-221 (1978); Becker, J. M. et al., Arch. Biochem. Biophys. 178:245-255 (1977)). Energy uncouplers such as sodium azide, dinitrophenol, and potassium cyanide all cause complete inhibition of transport of peptides in both yeast and plants (Higgins, C. F. et al., Planta 138:217-221 (1978); Becker, J. M. et al., Arch. Biochem. Biophys. 178:245-255 (1977)). 
     In sum, the above-described experiments demonstrate the ability of an A. thaliana gene to restore peptide transport to a S. cerevisiae mutant unable to transport di- and tripeptides. The yeast mutant transformed with the A. thaliana gene conferred sensitivity to toxic peptides, allowed growth of the mutant on a wide variety of peptides, and restored uptake of radiolabled dileucine. Growth of A. thaliana roots was inhibited by toxic peptides and this inhibition was reversed by a number of peptide competitors which is consistent with the peptide transporters&#39; expression in the roots. This plant peptide transport gene encodes a protein which shows a high degree of homology to the Arabidopsis nitrate transporter ATHCHL1Ap and to the yeast peptide transporter SACPTR2p and is the third in a growing group of proteins whose derived consensus sequence shows little homology to other proteins involved in peptide transport. 
     While the invention has been described in connection with specific embodiments thereof, it will be understood that it is capable of further modifications and this application is intended to cover any variations, uses, or adaptations of the invention following, in general, the principles of the invention and including such departures from the present disclosure as come within known or customary practice within the art to which the invention pertains and as may be applied to the essential features hereinbefore set forth and as follows in the scope of the appended claims. 
     
         __________________________________________________________________________SEQUENCE LISTING(1) GENERAL INFORMATION:(iii) NUMBER OF SEQUENCES: 11(2) INFORMATION FOR SEQ ID NO:1:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 2799 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: double(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(iv) ANTI-SENSE: NO(vi) ORIGINAL SOURCE:(A) ORGANISM: Arabidopsis thalliana(vii) IMMEDIATE SOURCE:(B) CLONE: atptr2a(xi) SEQUENCE DESCRIPTION: SEQ ID NO:1:GCGGCCGCCAGTGTGAGTAATTTAGGAGAAATTCAAAAACCTTGAGTGGAAACTCCTCAT60CGTTCGTATAATAATCGTTTGACCTCTTTTGTTTGGAGTTGGGACTTTCTCCACACTTTC120ACATACATACACTTTTAATTTCCAAGTATTTATTTAATACATTAAGGAAAAATTTTTTCA180TTCTAAAAATTTTTCTTTTTTTATTATTATTGTCATAAATACTTATTTGTTGTTGTGTAT240ATTTAATCTTGTTTTAAATACCCTTTCTCACTCTCACTCACTTTCATATTTCTTACTCTT300AGTTGAGTTAGTCGGCCTTCGATACACATATAAAAGTGTTTATTTTAACTTTTTTGTGAA360TTCACTTGTCAATTTTGTGTAATTAGTTTGACTAATTATTATTATTATTATTTTTGATCT420ATTCTTTTTTTTATCTTTTGTACTACATTGTTTTTTAATCTTTCGCTTGTTTACGTTATT480TTTCTCTTCCTCTTTTTTCCCTTTTAATATTCGCCTCTTTTGTTTTCTCGTTTCATTGTA540ATTATTTTATACCCAAAAATTGTTCTTGAAACTTCTGTTCATTCTCTTTTTTATTATTAT600TTTTGATTTTCATACGATCGATTTCCTACATTCAATTTACCTGTGTTTACAATGAGTAGC660ATTGAAGAACAAATTACGAAATCGGACTCCGATTTCATCATTTCAGAAGATCAATCCTAC720TTAAGCAAGGAGAAAAAGGCTGATGGTTCTGCCACCATCAACCAAGCTGACGAACAATCC780TCCACCGATGAACTCCAAAAATCCATGTCCACCGGCGTCCTCGTCAATGGTGACTTATAC840CCTTCTCCTACCGAAGAAGAATTAGCCACCCTTCCTAGTGTTTGCGGTACTATTCCTTGG900AAAGCCTTTATTATCATTATTGTCGAGCTTTGCGAACGTTTCGCTTACTATGGACTCACT960GTTCCCTTTCAAAATTATATGCAATTCGGTCCTAAGGATGCTACTCCAGGTGCCCTTAAT1020TTAGGCGAAACCGGTGCTGACGGTCTTTCTAATTTCTTCACATTTTGGTGTTATGTCACC1080CCGGTTGGCGCTGCACTTATTGCTGATCAATTCCTTGGTAGGTACAATACCATTGTTTGC1140TCTGCTGTCATTTACTTTATTGGTATCTTGATTCTTACATGTACTGCTATTCCTTCTGTC1200ATTGATGCCGGAAAAAGTATGGGTGGGTTTGTCGTCTCTTTGATCATCATTGGGCTTGGA1260ACCGGTGGTATCAAATCCAATGTTTCCCCCTTGATGGCTGAACAGCTTCCAAAAATTCCT1320CCTTATGTAAAGACAAAGAAAAATGGTAGCAAGGTCATTGTTGACCCAGTCGTCACCACC1380TCTCGTGCCTATATGATTTTCTACTGGACAATTAACGTCGGTTCTCTCTCCGTATTAGCC1440ACAACTAGTTTGGAAAGTACTAAAGGTTTTGTTTACGCATACTTGCTTCCCTTGTGCGTC1500TTTGTTATCCCCTTAATTATTTTGGCTGTTAGTAAGACAGCTTTTACAAGCACACTCCTC1560CCTCCGGTTCCATCTTTGTTCGTGTTGGTCAAGTGTTCTTCCTTGCTGCTCAAAACAAAT1620TTAATCTCGAAAAAACTAAACCATCTTGCACTACTACTGTTGGAGCGTTACGTCAAGGAT1680CAGTGGGATGACTTGTTTATCGACGAATTGAAACGTGCCTTACGCGCCTGCAAAACTTTT1740CTCTTTTACCCTATCTATTGGGTATGCTATGGTCAAATGACCAACAACTTAATTTCTCAA1800GCTGGACAAATGCAAACGGGTAATGTCTCTAACGATCTTTTCCAAGCCTTCGATTCAATC1860GCCTTGATTATTTTCATTCCCATTTGTGACAATATCATCTATCCATTATTGCGTAAGTAT1920AACATCCCTTTCAAACCCATCCTTCGTATTACTTTAGGGTTTATGTTTGCTACTGCTTCC1980ATGATTTACGCTGCTGTTTTACAAGCAAAGATTTATCAAAGAGGCCCTTGCTATGCAAAT2040TTTACTGATACATGTGTTTCCAATGACATCAGTGTTTGGATCCAAATCCCTGCTTACGTT2100TTGATTGCTTTCTCTGAAATTTTTGCCAGTATTACTGGTTTAGAATTTGCATTTACCAAG2160GCCCCTCCTTCAATGAAATCCATTATTACTGCTTTGTTCTTGTTCACCAATGCATTCGGT2220GCCATTCTATCTATTTGCATTTCTTCTACTGCTGTCAATCCTAAGCTTACTTGGATGTAC2280ACTGGTATTGCCGTCACTGCCTTTATTGCTGGTATTATGTTTTGGGTTTGCTTCCACCAC2340TATGATGCAATGGAAGATGAACAAAATCAACTTGAGTTCAAGCGTAATGATGCGTTAACG2400AAGAAGGACGTTGAAAAGGAAGTTCATGATAGTTATAGCATGGCAGATGAGTCCCAATAC2460AATTTGGAAAAAGCTAACTGCTGAAGAGGAAATCATGAAAAGCACATAATACTTAATTTA2520ACTTAATTCGTATTTGCGGATGGCCAATTTTTCTTTTCAAAATTTCAAAAAATTGGGGTT2580TGCATGTTTTGTTTCCATCTTTTTTTTTGTTATGATGCTGTTGTTCTACTGATGCTCCTT2640ATTTAAATGCAGTAGTACTTATCCACTCTCAGAAAATAGAGTTTTACAGTGGGTCTATAT2700ACCAGAATTTACTACAGTGTGATTTAATGAAAATATATATTGCTGTGCATAATTTAAAAA2760AAAAAAAAAACTAAATTACTCACACTGGCGGCCGCCCGC2799(2) INFORMATION FOR SEQ ID NO:2:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 610 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: protein(iii) HYPOTHETICAL: NO(vi) ORIGINAL SOURCE:(A) ORGANISM: Arabidopsis thalliana(vii) IMMEDIATE SOURCE:(B) CLONE: ATPTR2Ap(xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:MetSerSerIleGluGluGlnIleThrLysSerAspSerAspPheIle151015IleSerGluAspGlnSerTyrLeuSerLysGluLysLysAlaAspGly202530SerAlaThrIleAsnGlnAlaAspGluGlnSerSerThrAspGluLeu354045GlnLysSerMetSerThrGlyValLeuValAsnGlyAspLeuTyrPro505560SerProThrGluGluGluLeuAlaThrLeuProSerValCysGlyThr65707580IleProTrpLysAlaPheIleIleIleIleValGluLeuCysGluArg859095PheAlaTyrTyrGlyLeuThrValProPheGlnAsnTyrMetGlnPhe100105110GlyProLysAspAlaThrProGlyAlaLeuAsnLeuGlyGluThrGly115120125AlaAspGlyLeuSerAsnPhePheThrPheTrpCysTyrValThrPro130135140ValGlyAlaAlaLeuIleAlaAspGlnPheLeuGlyArgTyrAsnThr145150155160IleValCysSerAlaValIleTyrPheIleGlyIleLeuIleLeuThr165170175CysThrAlaIleProSerValIleAspAlaGlyLysSerMetGlyGly180185190PheValValSerLeuIleIleIleGlyLeuGlyThrGlyGlyIleLys195200205SerAsnValSerProLeuMetAlaGluGlnLeuProLysIleProPro210215220TyrValLysThrLysLysAsnGlySerLysValIleValAspProVal225230235240ValThrThrSerArgAlaTyrMetIlePheTyrTrpThrIleAsnVal245250255GlySerLeuSerValLeuAlaThrThrSerLeuGluSerThrLysGly260265270PheValTyrAlaTyrLeuLeuProLeuCysValPheValIleProLeu275280285IleIleLeuAlaValSerLysThrAlaPheThrSerThrLeuLeuPro290295300ProValProSerLeuPheValLeuValLysCysSerSerLeuLeuLeu305310315320LysThrAsnLeuIleSerLysLysLeuAsnHisLeuAlaLeuLeuLeu325330335LeuGluArgTyrValLysAspGlnTrpAspAspLeuPheIleAspGlu340345350LeuLysArgAlaLeuArgAlaCysLysThrPheLeuPheTyrProIle355360365TyrTrpValCysTyrGlyGlnMetThrAsnAsnLysIleSerGlnAla370375380GlyGlnMetGlnThrGlyAsnValSerAsnAspLeuPheGlnAlaPhe385390395400AspSerIleAlaLeuIleIlePheIleProIleCysAspAsnIleIle405410415TyrProLeuLeuArgLysTyrAsnIleProPheLysProIleLeuArg420425430IleThrLeuGlyPheMetPheAlaThrAlaSerMetIleTyrAlaAla435440445ValLeuGlnAlaLysIleTyrGlnArgGlyProCysTyrAlaAsnPhe450455460ThrAspThrCysValSerAsnAspIleSerValTrpIleGlnIlePro465470475480AlaTyrValLeuIleAlaPheSerGluIlePheAlaSerIleThrGly485490495LeuGluPheAlaPheThrLysAlaProProSerMetLysSerIleIle500505510ThrAlaLeuPheLeuPheThrAsnAlaPheGlyAlaIleLeuSerIle515520525CysIleSerSerThrAlaValAsnProLysLeuThrTrpMetTyrThr530535540GlyIleAlaValThrAlaPheIleAlaGlyIleMetPheTrpValCys545550555560PheHisHisTyrAspAlaMetGluAspGluGlnAsnGlnLeuGluPhe565570575LysArgAsnAspAlaLeuThrLysLysAspValGluLysGluValHis580585590AspSerTyrSerMetAlaAspGluSerGlnTyrAsnLeuGluLysAla595600605AsnCys610(2) INFORMATION FOR SEQ ID NO:3:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 1939 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: double(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iv) ANTI-SENSE: NO(vi) ORIGINAL SOURCE:(A) ORGANISM: Arabidopsis Thalliana(B) STRAIN: atptr2b(xi) SEQUENCE DESCRIPTION: SEQ ID NO:3:GCGGCCGCCAGTGTGAGTAATTTAGCGAAAACGATGGGTTCCATCGAAGAAGAAGCAAGA60CCTCTCATCGAAGAAGGTTTAATTTTACAGGAAGTGAAATTGTATGCTGAAGATGGTTCA120GTGGACTTTAATGGAAACCCACCATTGAAGGAGAAAACAGGAAACTGGAAAGCTTGTCCT180TTTATTCTTGGTAATGAATGTTGTGAGAGGCTAGCTTACTATGGTATTGCTGGGAATTTA240ATCACTTACCTCACCACTAAGCTTCACCAAGGAAATGTTTCTGCTGCTACAAACGTTACC300ACATGGCAAGGGACTTGTTATCTCACTCCTCTCATTGGAGCTGTTCTGGCTGATGCTTAC360TGGGGACGTTACTGGACCATCGCTTGTTTCTCCGGGATTTATTTCATCGGGATGTCTGCG420TTAACTCTTTCAGCTTCAGTTCCGGCATTGAAGCCAGCGGAATGTATTGGTGACTTTTGT480CCATCTGCAACGCCAGCTCAGTATGCGATGTTCTTTGGTGGGCTTTACCTGATCGCTCTT540GGAACTGGAGGTATCAAACCGTGTGTCTCATCCTTCGGTGCCGATCAGTTTGATGACACG600GACTCTCGGGAACGAGTTAGAAAAGCTTCGTTCTTTAACTGGTTTTACTTCTCCATCAAT660ATTGGAGCACTTGTGTCATCTAGTCTTCTAGTTTGGATTCAAGAGAATCGGGGGTGGGGT720TTAGGGTTTGGGATACCAACAGTGTTCATGGGACTAGCCATTGCAAGTTTCTTCTTTGGC780ACACCTCTTTATAGGTTTCAGAAACCTGGAGGAAGCCCTATAACTCGGATTTCCCAAGTC840GTGGTTGCTTCGTTCCGGAAATCGTCTGTCAAAGTCCCTGAAGACGCCACACTTCTGTAT900GAAACTCAAGACAAGAACTCTGCTATTGCTGGAAGTAGAAAAATCGAGCATACCGATGAT960TGCCAGTATCTTGACAAAGCCGCTGTTATCTCAGAAGAAGAATCGAAATCCGGAGATTAT1020TCCAACTCGTGGAGACTATGCACGGTTACGCAAGTCGAAGAACTCAAGATTCTGATCCGA1080ATGTTCCCAATCTGGGCTTCTGGTATCATTTTCTCAGCTGTATACGCACAAATGTCCACA1140ATGTTTGTTCAACAAGGCCGAGCCATGAACTGCAAAATTGGATCATTCCAGCTTCCTCCT1200GCAGCACTCGGGACATTCGACACAGCAAGCGTCATCATCTGGGTGCCGCTCTACGACCGG1260TTCATCGTTCCCTTAGCAAGAAAGTTCACAGGAGTAGACAAAGGATTCACTGAGATACAA1320AGAATGGGAATTGGTCTGTTTGTCTCTGTTCTCTGTATGGCAGCTGCAGCTATCGTCGAA1380ATCATCCGTCTCCATATGGCCAACGATCTTGGATTAGTCGAGTCAGGAGCCCCAGTTCCC1440ATATCCGTCTTGTGGCAGATTCCACAGTACTTCATTCTCGGTGCAGCCGAAGTATTCTAC1500TTCATCGGTCAGCTCGAGTTCTTCTACGACCAATCTCCAGATGCAATGAGAAGCTTGTGC1560AGTGCCTTAGCTCTTTTGACCAATGCACTTGGTAACTACTTGAGCTCGTTGATCCTCACG1620CTCGTGACTTATTTTACAACAAGAAATGGGCAAGAAGGTTGGATTTCGGATAATCTCAAT1680TCAGGTCATCTCGATTACTTCTTCTGGCTCTTGGCTGGTCTTAGCCTTGTGAACATGGCG1740GTTTACTTCTTCTCTGCTGCTAGGTATAAGCAAAAGAAAGCTTCGTCGTAGTAATGCTGT1800TATCTATCTACTTTCATTACATACAAAAGTTTGTTTCTTTCAACTGTAACTGTCTCTGTA1860TCAATAACAACATTGCTGTGTACTTTTCCTTTCAATTTCAAAAGTTTAAGTCGCCTAAAT1920TACTCACACTGGCGGCCGC1939(2) INFORMATION FOR SEQ ID NO:4:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 585 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: protein(iii) HYPOTHETICAL: NO(vi) ORIGINAL SOURCE:(A) ORGANISM: Arabidopsis thalliana(vii) IMMEDIATE SOURCE:(B) CLONE: ATPTR2Bp(xi) SEQUENCE DESCRIPTION: SEQ ID NO:4:MetGlySerIleGluGluGluAlaArgProLeuIleGluGluGlyLeu151015IleLeuGlnGluValLysLeuTyrAlaGluAspGlySerValAspPhe202530AsnGlyAsnProProLeuLysGluLysThrGlyAsnTrpLysAlaCys354045ProPheIleLeuGlyAsnGluCysCysGluArgLeuAlaTyrTyrGly505560IleAlaGlyAsnLeuIleThrTyrLeuThrThrLysLeuHisGlnGly65707580AsnValSerAlaAlaThrAsnValThrThrTrpGlnGlyThrCysTyr859095LeuThrProLeuIleGlyAlaValLeuAlaAspAlaTyrTrpGlyArg100105110TyrTrpThrIleAlaCysPheSerGlyIleTyrPheIleGlyMetSer115120125AlaLeuThrLeuSerAlaSerValProAlaLeuLysProAlaGluCys130135140IleGlyAspPheCysProSerAlaThrProAlaGlnTyrAlaMetPhe145150155160PheGlyGlyLeuTyrLeuIleAlaLeuGlyThrGlyGlyIleLysPro165170175CysValSerSerPheGlyAlaAspGlnPheAspAspThrAspSerArg180185190GluArgValArgLysAlaSerPhePheAsnTrpPheTyrPheSerIle195200205AsnIleGlyAlaLeuValSerSerSerLeuLeuValTrpIleGlnGlu210215220AsnArgGlyTrpGlyLeuGlyPheGlyIleProThrValPheMetGly225230235240LeuAlaIleAlaSerPhePhePheGlyThrProLeuTyrArgPheGln245250255LysProGlyGlySerProIleThrArgIleSerGlnValValValAla260265270SerPheArgLysSerSerValLysValProGluAspAlaThrLeuLeu275280285TyrGluThrGlnAspLysAsnSerAlaIleAlaGlySerArgLysIle290295300GluHisThrAspAspCysGlnTyrLeuAspLysAlaAlaValIleSer305310315320GluGluGluSerLysSerGlyAspTyrSerAsnSerTrpArgLeuCys325330335ThrValThrGlnValGluGluLeuLysIleLeuIleArgMetPhePro340345350IleTrpAlaSerGlyIleIlePheSerAlaValTyrAlaGlnMetSer355360365ThrMetPheValGlnGlnGlyArgAlaMetAsnCysLysIleGlySer370375380PheGlnLeuProProAlaAlaLeuGlyThrPheAspThrAlaSerVal385390395400IleIleTrpValProLeuTyrAspArgPheIleValProLeuAlaArg405410415LysPheThrGlyValAspLysGlyPheThrGluIleGlnArgMetGly420425430IleGlyLeuPheValSerValLeuCysMetAlaAlaAlaAlaIleVal435440445GluIleIleArgLeuHisMetAlaAsnAspLeuGlyLeuValGluSer450455460GlyAlaProValProIleSerValLeuTrpGlnIleProGlnTyrPhe465470475480IleLeuGlyAlaAlaGluValPheTyrPheIleGlyGlnLeuGluPhe485490495PheTyrAspGlnSerProAspAlaMetArgSerLeuCysSerAlaLeu500505510AlaLeuLeuThrAsnAlaLeuGlyAsnTyrLeuSerSerLeuIleLeu515520525ThrLeuValThrTyrPheThrThrArgAsnGlyGlnGluGlyTrpIle530535540SerAspAsnLeuAsnSerGlyHisLeuAspTyrPhePheTrpLeuLeu545550555560AlaGlyLeuSerLeuValAsnMetAlaValTyrPhePheSerAlaAla565570575ArgTyrLysGlnLysLysAlaSerSer580585(2) INFORMATION FOR SEQ ID NO:5:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 4 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:5:LysLysLysLys(2) INFORMATION FOR SEQ ID NO:6:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 4 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:6:GlyLeuGlyLeu1(2) INFORMATION FOR SEQ ID NO:7:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 4 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:7:ThrProArgLys1(2) INFORMATION FOR SEQ ID NO:8:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 5 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:8:TyrGlyGlyPheLeu15(2) INFORMATION FOR SEQ ID NO:9:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 6 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:9:TrpHisTrpLeuGlnLeu15(2) INFORMATION FOR SEQ ID NO:10:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 20 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(vi) ORIGINAL SOURCE:(A) ORGANISM: Arabidopsis thalliana(xi) SEQUENCE DESCRIPTION: SEQ ID NO:10:GCTTCCATGATTTACGCTGC20(2) INFORMATION FOR SEQ ID NO:11:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 17 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(iv) ANTI-SENSE: NO(vi) ORIGINAL SOURCE:(A) ORGANISM: Arabidopsis thalliana(xi) SEQUENCE DESCRIPTION: SEQ ID NO:11:GCATAAACGCCTACCGG17__________________________________________________________________________