Abstract:
Recombinant gene coding for a protein having endochitinase activity or for a precursor thereof which comprises the sequence of SEQ ID NO:1 below: 
     Gly Gly Asp Leu Gly Ser VaL Ile Ser Asn Ser Met Phe Asp Gln Met Leu Lys His Arg Asn Glu Asn Ser Cys Gln Gly Lys Asn Asn Phe Tyr Ser Tyr Asn Ala Phe Ile Thr Ala Ala Arg Ser Phe Pro Gly, Phe Gly Thr Ser Gly Asp Ile Asn Ala Arg Lys Arg Glu Ile Ala Ala Phe Phe Ala Gln Thr Ser His Glu Thr Thr Gly Gly Trp Pro Ser Ala Pro Asp Gly Pro Phe Ala Trp Gly Tyr Cys Phe Leu Arg Gly Arg Gly Asn Pro Gly Asp Tyr Cys Ser Pro Ser Ser Gln Trp Pro Cys Ala Pro Gly Arg Lys Tyr Phe Gly Arg Gly Pro Ile Gln Ile Ser His Asn Tyr Asn Tyr Gly Pro Cys Gly Arg Ala Ile Gly Val Asp Leu Leu Asn Asn Pro Asp Leu Val Ala Thr Asp Pro Val Ile Ser Phe Lys Thr Ala Ile Trp Phe Trp Met Thr Pro Gln Ser Pro Lys Pro Ser Cys His Asp Val Ile Ile Gly Arg Trp Asn Pro Ser Ala Gly Asp Arg Ser Ala Asn Arg Leu Pro Gly Phe Gly Val Ile Thr Asn Ile Ile Asn Gly Gly Leu Glu Cys Gly Arg Gly Asn Asp Asn Arg Val Gln Asp Arg Ile Gly Phe Tyr Arg Arg Tyr Cys Gly Ile Leu Gly Val Ser Pro Gly Asp Asn Leu Asp Cys Gly Asn Gln Arg Ser Phe Gly Asn Gly Leu Leu Val Asp Thr Met. 
     Application: For obtaining plants resisting to pathogenic agents.

Description:
This application is a continuation of application Ser. No. 07/842,165, filed May 1, 1992. 
    
    
     FIELD OF THE INVENTION 
     The invention relates to a new recombinant gene coding for a new protein having endochitinase activity or for a precursor thereof, to a bacterium containing this recombinant gene, to a plant cell, a plant or a plant part, especially a plant seed, which contain a recombinant gene of this type, and to a method for rendering plants resistant to pathogenic agents such as fungi and bacteria as well as arthropods, in particular insects, and nematodes, which comprises a step of transformation with this gene, as well as to this new protein and to a method for preparing it. 
     Crop plants are subjected to attacks by pathogenic agents such as fungi and bacteria, which are responsible for substantial harvest losses. At present, the principal means of controlling these agents lies in the use of chemical substances having fungicidal or bactericidal activity. It is now known that plants react naturally to such attack by various defence mechanisms, which are unfortunately in general triggered too late and at too low an intensity to be sufficiently effective. One of these mechanisms comprises the induction of an enzyme known as chitinase EC 3.2.1.14 (A. Toppan et al., 1982, Agronomie, 2, 829-834). This induction may be artificially stimulated with substances such as ethylene, and results in an increase in resistance of the treated plant to pathogenic agents (Boller T., 1988, Oxford Surveys of Plant Molecular and Cell Biology, 5, 145-174). 
     Chitin is a linear polysaccharide polymer consisting of N-acetylglucosamineB units linked via β-(1→4) bonds. It is a structural compound present in the walls of most pathogenic fungi, in the exoskeleton of arthropods, especially insects, and in the external sheath of the eggs and cysts of nematodes. The enzymes known as chitinases are capable of degrading chitin. Among these, two different groups are distinguished, defined according to their mode of attack of chitin: exochitinases capable of liberating the N-acetylglucosaimine unit located at the non-reducing ends of the chains, and endochitinases capable of fragmenting the chains, which are the only chitinases capable of inhibiting in vitro the growth of mycelial hyphae (Roberts W. K. et al., 1988, Gen. Microbiol., 134, 169-176). The great majority of known plant chitinases are of the endo type, in contrast to the known bacterial chitinases which are of the exo type (Roberts W. K. et al., 1988, Gen. Microbiol., 134, 169-176). 
     A large number of plant endochitinases, in particular those of tomato and tobacco (P. AUDY et al., 1990, Phytochem, 29, 4, 1143-1159), also exhibit a lysozyme activity, a capacity to cleave the β-(1→4) bonds between the N-acetylglucosamine and the N-acetylmuramic acid of the peptidoglycan of bacterial walls. It may hence be acknowledged that lysozyme and endochitinase activities are fairly closely related (Roberts W. K. et al., 1988, Gen. Microbiol., 134, 169-176), and that a new protein having endochitinase activity, especially one of structures intermediate between tomato endochitinase and tobacco endochitinase, probably exhibits lysozyme activity. 
     DNA sequences coding for bacterial exochitinases have already been isolated and cloned (Jones J. D. G. et al., 1986, EMBO J., 5, 467-473 and Sundheim L. et al., 1988, Physiol. Molec. Plant Pathol., 33, 483-491). U.S. Pat. No. 4,751,081 describes the isolation and cloning of the complete gene coding for Serratia marcescens chitinase, as well as the transformation of Pseudomonas fluorescens NZ130 and Pseudomonas putida MK280 bacteria with this gene. These transformed bacteria are capable of slightly degrading a colloidal chitin dispersed in the bacterial culture medium. The work of Harpster M. H. et al., 1989, Nucl. Ac. Res., 17, 5395 has shown that this gene codes for an exochitinase, thereby explaining the low efficiency of degradation observed (see Table 2, col. 13 and 14 of this document). The publication of Jones J. D. G. et al., (1988), Mol. Gen. Gen,et., 212, 536-542, mentions the transformation of tobacco plants with Agrobacterium tumefaciens containing a chimeric gene comprising the coding portion of Serratia marcescens exochitinase under the control of different plant promoters. This document gives no information about the possible increase in resistance to pathogens conferred by the expression of this exochitinase. 
     Genomic DNA and/or complementary DNA sequences coding for some plant endochitinases have, moreover, been isolated and cloned (Broglie K. E., 1986, Proc. Ntl. Acad. Sci. USA, 83, 6820-6824 and Headrick S. A., 1988, Plant Physiol., 86, 182-186). 
     International application WO 90/07001 discloses the construction of a plasmid bearing a cDNA of the endochitinase of bean Phaseolus vulgaris under the control of a strong promoter, the conversion with the aid of Agrobacterium tumefaciens, the regeneration of the transformed tobacco, test showing the increased resistance to fungi Rhizoctonia solani and Botrytis cinerea of the regenerated plants, the obtention of transgenic tomato plants expressing the bean chitinase as well as the obtention, by means of this gene, of colza transgenic plants having a chitinase activity and an increased resistance to Rhizoctonia solani with regard to the non-transformed colza plants. 
     SUMMARY OF THE INVENTION 
     The invention hence relates to a new recombinant gene, characterized in that it codes for a protein having endochitinase activity or a precursor thereof which comprises the sequence (1) below (SEQ ID NO: 1) 
     Gly Gly Asp Leu Gly Ser Val Ile Ser Asn Ser Met Phe Asp Gln Met Leu Lys His Arg Asn Glu Asn Ser Cys Gln Gly Lys Asn Asn Phe Tyr Ser Tyr Asn Ala Phe Ile Thr Ala Ala Arg Ser Phe Pro Gly Phe Gly Thr Ser Gly Asp Ile Asn Ala Arg Lys Arg Glu Ile Ala Ala Phe Phe Ala Gln Thr Ser His Glu Thr Thr Gly Gly Trp Pro Ser Ala Pro Asp Gly Pro Phe Ala Trp Gly Tyr Cys Phe Leu Arg Glu Arg Gly Asn Pro Gly Asp Tyr Cys Ser Pro Ser Ser Gln Trp Pro Cys Ala Pro Gly Arg Lys Tyr Phe Gly Arg Gly Pro Ile Gln Ile Ser His Asn Tyr Asn Tyr Gly Pro Cys Gly Arg Ala Ile Gly Val Asp Leu Leu Asn Asn Pro Asp Leu Val Ala Thr Asp Pro Val Ile Ser Phe Lys Thr Ala Ile Trp Phe Trp Met Thr Pro Gln Ser Pro Lys Pro Ser Cys His Asp Val Ile Ile Gly Arg Trp Asn Pro Ser Ala Gly Asp Arg Ser Ala Asn Arg Leu Pro Gly Phe Gly Val Ile Thr Asn Ile Ile Asn Gly Gly Leu Gly Cys Gly Arg Gly Asn Asp Asn Arg VaL Gln Asp Arg Ile Gly Phe Tyr Arg Arg Tyr Cys Gly ILe Leu Gly Val Ser Pro Gly Asp Asn Leu Asp Cys Gly Asn Gln Arg Ser Phe Gly Asn Gly Leu Leu Val Asp Thr Met 
     This recombinant gene preferably codes for a protein which comprises, immediately upstream of the sequence (1), the sequence (2) below (SEQ ID NO: 2): 
     Gln Asn Cys Gly Ser Gln Gly Gly Gly Lys Val Cys Ala Ser Gly Gln Cys Cys Ser Lys Phe Gly Trp Cys Gly Asn Th, Asn Asp His Cys Gly Ser Gly Asn Cys Gln Ser Gln Cys Pro Gly Gly Gly Pro Gly Pro Gly Pro Val Thr 
     which is designed to be cleaved off during the maturation of the protein, or a sequence exhibiting a substantial degree of homology with the sequence (2). 
     Preferably, this recombinant gene codes for a protein whose sequence comprises, upstream of the sequence (1) and preferably separated from the sequence (1) by a sequence designed to be cleaved off, a sequence coding for a signal peptide. An especially advantageous gene of this type is that which codes for a protein whose sequence comprises, immediately upstream of the sequence (2) or of a sequence exhibiting a substantial degree of homology with the sequence (2), the sequence (3) below (SEQ ID NO: 3): 
     Met Arg Arg Thr Ser Lys Leu Thr Thr Phe Ser Leu Leu Phe Ser Leu Val Leu Leu Ser Ala Ala Leu Ala 
     or a sequence exhibiting a substantial degree of homology with the sequence (3). 
     The invention also relates to a recombinant gene coding for a protein having endochitinase activity or for a precursor thereof, which comprises a sequence exhibiting a substantial degree of homology with the sequence (1). The coding portion of this recombinant gene comprises at least one portion 5&#39; of the genomic DNA or complementary DNA of tomato endochitinase and at least one portion 3&#39; of the genomic DNA or complementary DNA of tobacco endochitinase. Preferably, the coding portion of the recombinant gene possesses at least one intron. In effect, it is known that the presence of introns in the coding portion of a gene increases expression of the latter (see, for example, the work of J. CASSIS et al., 1987, Genes and development, 1, 1183-1200). 
     An example of such a recombinant gene is the recombinant gene in which the coding portion is the sequence below (SEQ ID NO: 4): 
     
         __________________________________________________________________________ATGAGGCGAA   CTTCTAAATT           GACTACTTTT                   TCTTTGCTGT                           TTTCTCTGGTTTTGCTGAGT   GCTGCCTTGG           CACAGAATTG                   TGGTTCACAG                           GGCGGAGGCAAAGTTTGTGC   GTCGGGACAA           TGTTGCAGCA                   AATTCGGGTG                           GTGCGGTAACACTAATGACC   ATTGTGGTTC           TGGCAATTGT                   CAAAGTCAGT                           GTCCAGGTGGCGGCCCTGGT   CCTGGTCCTG           TTACTGGTGG                   GGACCTCGGA                           AGCGTCATCTCAAATTCTAT   GTTTGATCAA           ATGCTTAAGC                   ATCGTAACGA                           AAATTCTTGTCAAGGAAAGA   ATAATTTCTA           CAGTTACAAT                   GCCTTTATTA                           CTGCTGCTAGGTCTTTTCCT   GGCTTTGGTA           CAAGTGGTGA                   TATCAATGCC                           CGTAAAAGGGAAATTGCTGC   TTTCTTTGCC           CAAACCTCCC                   ATGAAACTAC                           TGGTATGTGTATAACCATTC   ACATCGAACC           ATTAAAATAT                   AATTTCATTT                           TATTTTATTTAGTAATTGAT   TATATATGTA           GGAGGATGGC                   CTTCCGCACC                           TGATGGACCATTCGCATGGG   GTTACTGTTT           CCTTAGAGAA                   CGAGGTAACC                           CCGGTGACTACTGTTCACCA   AGTAGTCAAT           GGCCTTGTGC                   ACCTGGAAGG                           AAATATTTCGGACGAGGCCC   AATCCAAATT           TCACAGTAAG                   CTACATAAAT                           CTATATATGGTAAAATTTGA   TGAACTTGTA           GTGTCTAATT                   ACGTGTATTT                           TGACATTTCAAAACAGCAAC   TACAACTATG           GGCCATGTGG                   AAGAGCCATC                           GGAGTGGACCTTTTAAACAA   TCCTGATTTA           GTAGCCACAG                   ACCCAGTCAT                           CTCATTCAAGACTGCTATCT   GGTTCTGGAT           GACCCCTCAA                   TCACCAAAGC                           CTTCTTGCCACGATGTCATC   ATTGGAAGAT           GGAACCCATC                   TGCCGGTGAC                           CGATCAGCCAATCGTCTTCC   TGGATTTGGT           GTCATCACAA                   ACATCATCAA                           TGGGGGCCTGGAATGTGGTC   GTGGCAATGA           CAATAGGGTC                   CAGGATCGCA                           TTGGGTTTTACAGGAGGTAT   TGCGGTATTC           TTGGTGTTAG                   TCCTGGTGAC                           AATCTTGATTGCGGAAACCA   GAGATCTTTT           GGAAACGGAC                   TTTTAGTCGA                           TACTATGTAATGA__________________________________________________________________________ 
    
     This coding sequence is preferably preceded by a promoter sequence containing a strong viral promoter such as the 35S promoter of cauliflower mosaic virus (see ODELL J. T. et al., 1985, NATURE, 313, 810-812), and followed by a termination sequence containing the nopaline synthase terminator of Agrobacterium tumefaciens (see BEVAN M. et al., 1983, Nucl. Ac. Res., 11, 369). 
     The invention also relates to a bacterium, for example of the species E. coli, which contains the recombinant gene defined above in a nucleotide environment or context permitting its replication and can hence be used for the cloning of this gene, as well as to a bacterium capable of infecting a plant with transfer of genetic material, for example of one of the species Agrobacterium rhizogenes and Agrobacterium tumefaciens, which contains this gene in a context permitting its replication and can hence be used for transforming plant cells. The transformation of plant cells by the above gene may also be performed by another biological method such as the pollen tube technique (Zhong-xun Luo et al., Plant Molec. Biol. Rep., 1988, 6, 165-176) and the direct transformation of germinating seeds (Toepfer R. et al., 1989, The Plant Cell., 1, 133-139), or by a physical method such as the use of polyethylene glycol, electroporation (Chistou P. et al., 1987, Proc. Ntl. Acad. Sci. USA, 84, 3662-3699) and bombardment using microprojectiles (Klein T. M. et al., 1988, Proc. Ntl. Acad. Sci. USA, 85, 8502-8505). 
     The invention also relates to a plant cell, characterised in that it is transformed by the recombinant gene as hereinabove defined, inserted in a context capable of permitting its expression. This plant cell can originate from a major crop species such as, for example, maize, soya bean, beet, wheat, barley, poppy, rape, sunflower, alfalfa and sorghum, from a floral species such as the rose, carnation and gerbera or from an edible species such as carrot, tomato, lettuce, chicory, capsicum, melon and cabbage. Species given particular consideration are Brassica napus rape, Helianthus annuus sunflower and Nicotiana tabacum tobacco. 
     The transformation step which involves one or a few cells is followed by a step of multiplication of transformed cells so as to obtain calluses, which can give rise to transformed plants by processes of organogenesis or embryogenesis. A part of the descendants of these transformed plants contains and expresses the recombinant gene. 
     The invention hence also relates to a plant or a plant part, characterized in that it contains, in a context capable of permitting its expression, the recombinant gene as hereinabove defined. A plant part given particular consideration is the seed: grain or some other part of a plant capable of forming a complete new plant, in particular after sowing or burying in the ground. These plants can be any one of the above species, and more especially of the species Nicotiana tabacum, Helianthus annuus and Brassica napus. 
     The invention also relates to a method for obtaining plants resistant to pathogenic agents such as fungi and bacteria as well as arthropods, especially insects, and nematodes, characterized in that it comprises a step of transformation of plant cells by the recombinant gene as hereinabove defined, followed by a step of multiplication of the transformed cells and a step of regeneration of the plants. 
     Preferably, the step of transformation of the plant cells is performed in vitro using an agrobacterium (that is to say a bacterium of the genus Agrobacterium) which has integrated the recombinant gene as hereinabove defined. 
     The invention also relates to the plants resistant to pathogenic agents, capable of being obtained using the method defined above. 
     The invention also relates to the use of a plant falling within the category of the plants defined in the preceding paragraph, or of a plant containing, in a context capable of permitting its expression, the recombinant gene as hereinabove defined, as a parent in a selection programme for creating new plant varieties. 
     The invention also relates to a new protein having endochitinase activity which comprises the sequence (1), as well as to a method for obtaining it which comprises the culturing of plant cells or calluses transformed by the recombinant gene, lysis of these cells or calluses, and isolation and purification of the recombinant protein. This protein can be of interest as an active principle of a new medicinal product intended for treating conditions such as, for example, mycoses. 
     A better understanding of the invention will be gained from the examples below: 
     A large part of the collective techniques below, which are well known to those skilled in the art, is described in detail in the work by Maniatis et al. &#34;Molecular cloning: a laboratory manual&#34; published in 1989 by Cold Spring Harbor Press publications, New York (2nd edition). 
     The biological material (strains, phages, plasmids or plants) used in the examples below is commercially available and described, respectively, in the documents below: 
     phage lambda CHARON 4A: MANIATIS et al. Op. Cit. 
     shuttle vector pBIN19: BEVAN et al., 1984, Nucl. Ac. Res., 12, 8711-8721; 
     plasmide pBI121: JEFFERSON R. A. et al., 1987, E.M.B.O.J., 6, 3901; 
     E. coli strain MC1061: MEISSNER P. S. et al., 1987, Proc. Natl. Acad. Sci. USA, 84 4171; 
     E. coli strain HB101: MANIATIS et al., Op. Cit.; 
     Agrobacterium tumefaciens strain LBA4404: HOEKEMA et al., 1983, NATURE, 303, 179-180; 
     Nicotiana tabacum plant var. Wisconsin Havana 38: SCHNEIDER M., 1990, Plant Molec. Biol., 14, 935-947; 
     Chalara elegans fungus: RAWLINGS R. E., 1940, Ann. Mo-Bot. Gdn., 27, 561-598; 
     Nicotiana tabacum plant var. Paraguay 49 obtained from the Tobacco Institute, Bergerac, France. 
     Alternaria brassicae fungus: BAINS and TEWARI Physiol. Mol.Plant. Pathol. 30, 259, 1987 
     Helianthus annuus plant: Euroflor variety of RUSTICA seeds 
     Sinapis alba: BAIN and TEWARI above cited reference 
     The following abbreviations are used in the examples below: 
     alpha32-dCTP: deoxycitidine 5&#39;- alpha- 32  P!triphosphate marketed boy AMERSHAM under the reference 10205; 
     0.2×SSC: 30 mM NaCl, 3 mM trisodium citrate pH 7.0 (described by MANIATIS et al., op. cit.); 
     SDS: sodium dodecyl sulphate; 
     FPLC: fast protein liquid chromatography; 
     PVDF: polyvinylidene difluoride. 
    
    
     BRIEF DESCRIPTION OF THE DRAWINGS 
     FIG. 1 represents a restriction map of the genomic DNA fragment of tomato endochitinase, having 3.5 kbs, inserted into plasmid pCH3.5. 
     FIG. 2 (SEQ ID NO: 5) represents the genomic DNA sequence, and the deduced peptide sequence (SEQ ID NO: 6), of endochitinase of tomato having 3.5 k b  s, inserted into plasmid pCH3.5. 
     FIG. 3 represents the alignment on the basis of maximum homology of tomato endochitinase genomic DNA devoid of introns (lower line (SEQ ID NO: 14)) and tobacco endochitinase complementary DNA (upper line (SEQ ID NO: 15)). 
     FIG. 4 (SEQ ID NO: 12) represents the coding sequence of the chimeric gene flanked by the BamHI and SacI sites, and the deduced amino acid sequence (SEQ ID NO: 13). 
     FIG. 5 (SEQ ID NO: 9) represents the sequence of the complete chimeric gene. 
     FIG. 6 (SEQ ID NO: 1) represents the sequence of the mature recombinant endochitinase. 
    
    
     DETAILED DESCRIPTION OF THE INVENTION 
     EXAMPLE 1 
     Construction of the shuttle vector pBR1 containing a tomato-tobacco recombinant gene for endochitinase 
     1) Preparation of the coding sequence of the recombinant gene 
     a) Preparation of the 5&#39; portion of the coding sequence of the recombinant gene from tomato endochitinase gDNA (genomic DNA): 
     A clone containing tomato endochitinase gDNA was obtained in the following manner (see Doctoral Thesis, special field: plant molecular biology, 1986, of M. DURANT-TARDIF --Paris Sud University): 
     A tomato genomic DNA library was constructed in phage lambda Charon 4A by cloning fragments emanating from the partial digestion with EcoRI endonuclease of Lycopersicon esculentum tomato genomic DNA. When the genomic library had been amplified, 6.6×10 5  clones were screened after transfer of the phage DNA onto nitrocellulose by techniques well known to those skilled in the art (Maniatis et al., Molecular cloning: a laboratory manual, Cold Spring Harbor Laboratory, 1984) using a cDNA probe coding for a bean endochitinase (Broglie et al., 1986, PNAS, 83, 6820-6824). 
     The clone, referred to as clone 10.2, which hybridises with this probe contains a 3.5-kb tomato genomic DNA fragment containing a portion of the tomato endochitinase gene. This fragment was then inserted into plasmid pEMBL8 (Dente et al., (1983), Nucl. Ac. Res., 11, 1645-1655) between the EcoRI and HindIII sites. The plasmid obtained, referred to as pCH3.5, was cloned into E. coli. This plasmid was then extracted and purified by the alkaline lysis method (BIRNBOIM and DOLY in Maniatis et al., op. cit.). 
     The use of several restriction endonucleases made it possible to establish the restriction map of the approximately 3.5-kb genomic DNA fragment inserted into plasmid pCH3.5, shown in FIG. 1. 
     The various EcoRI-HincII, HincII-PvuII, PvuII-EcoRV and EcoRV-HindIII fragments were prepared by digestion with the corresponding endonucleases, and were purified by agarose gel electrophoresis and isolated by electroelution (Maniatis et al., op. cit.). Each of these fragments was cloned into the DNA of the replicative form of the single-stranded phage M13mp19 (Pharmacia) between the compatible restriction sites. These fragments were then sequenced according to the dideoxyribonucleotide method (Sanger et al., PNAS-USA, 14, 5463-5467, 1977). 
     The sequence (SEQ ID NO: 5), as deduced from the above experiments, is shown in FIG. 2, which also indicates the restriction sites used for cloning into pEMBL8 and the important restriction sites for the next steps of the construction. The translated amino acid sequence is also shown in this figure on the line below the coding sequence, the introns being hatched . 
     This sequence possesses a promoter portion of 1940 nucleotides followed by a coding portion, coding for 302 amino acids, in which two introns are inserted. This coding portion is incomplete in its 3&#39; region (no stop codon). 
     By the use of the Styl (position 2006) and HindIII (position 3007) restriction sites, a 1001-bp fragment was obtained; it was purified by electrophoresis on low-melting temperature agarose gel. Chemical synthesis of a 71-bp oligonucleotide, referred to as fragment 1, whose sequence is given below, enabled the 5&#39; portion removed upstream of the StyI site to be re-formed and a BamHI restriction site to be inserted upstream of the translation initiation ATG codon. The 1071-bp BamHI-HindIII fragment was subcloned into the vector pUC 19 (Pharmacia) in the corresponding sites using T4 DNA ligase. The plasmid obtained is referred to as pCH1. ##STR1## 
     b) Preparation of the Lacking 3&#39; portion of the coding sequence of the chimeric gene: 
     A comparison of sequences using suitable software (University of Wisconsin software UWGCG: Devereux et al., 1984, Nucl., Ac. Res., 12, 8711-8721 - Option GAP: optimal alignment of sequences according to the method of Needleman and Wunsch, 1970 J. mol. Biol., 48, 443-453) between the coding portion, incomplete in its 3&#39; region, of the clone pCH3.5 and the published sequence of tobacco endochitinase cDNA comprising 329 amino acids (Hideaki Shinshi et al. (1987), Proc. Ntl. Acad. Sci. USA, 84, 89-93 and (1990) Plant Mol. Biol.,, 14, 357-368) shows a substantial homology between the sequences, especially in the 3&#39; portion of the latter (see FIG. 3, which shows an alignment performed with this software on the basis of maximum homology of these two sequences, that of the tomato endochitinase gDNA devoid of its introns being located on the lower line). 
     Oligonucleotides synthesised on an Applied Biosystems 4600 DNA synthesiser were assembled so as to obtain a fragment, referred to as fragment 2, whose sequence reproduces, in respect of 71 nucleotides, the tomato endochitinase gDNA sequence located downstream of the DraII site (2), and in respect of 92 nucleotides, a sequence closely resembling the 3&#39; portion of the published sequence of tobacco endochitinase cDNA, to which a second stop codon and the sequence of the SacI restriction site have been added. This sequence is shown below: the sequence closely resembling the 3&#39; portion of the tobacco endochitinase cDNA sequence being underlined and the SacI site being indicated (SEQ ID NO: 7) ##STR2## 
     Plasmid pCH1 was subjected to a partial hydrolysis with the restriction enzymes BamHI and DraII, and a 999-bp fragment, referred to as fragment 3, whose ends consist of the BamHI site at the 5&#39; end and the DraII site (2) at the 3&#39; end (see FIG. 2), was then isolated and purified after agarose gel electrophoresis; the fragments 2 and 3 were ligated using T4 DNA ligase in plasmid pUC 19 opened at the BamHI and SacI restriction sites. The plasmid obtained is referred to as pCH1.2. It was checked by sequencing that the BamHI-SacI portion of this plasmid contained the expected sequence. The latter, as well as the deduced amino acid sequence, is shown in FIG. 4. This sequence comprises the coding sequence of the chimeric gene flanked by the BamHI and SacI restriction sites. This sequence codes for a protein of 329 amino acids comprising an assumed signal peptide of 24 amino acids (determined using a software which employs the method described by G. von Heijne, 1986, Nucl. Ac. Res., 14, 483-490). The expected molecular mass on the basis of the sequence of this protein when its assumed signal peptide has been cleaved off is approximately 32 kDa. 
     2) Preparation of the complete chimeric gene and cloning of the latter into the shuttle vector pBIN 19. 
     The coding sequence obtained above was inserted between a promoter sequence comprising the so-called 35S promoter of cauliflower mosaic virus (35S CaMV) and a termination sequence comprising the nopaline synthase (NOS) terminator of Agrobacterium tumefaciens. 
     a) Preparation of the promoter sequence comprising the 35S promoter of cauliflower mosaic virus: 
     Starting with plasmid pBI121 (Clontech), by cleavage using HindIII and BamHI endonucleases followed by electrophoresis, the approximately 900-bp HindIII-BamHI fragment containing the 35S promoter is isolated. This fragment is recut with HindII. The approximately 410-bp fragment carrying the BamHI site is treated with T4 DNA ligase in the presence of a HindIII linker (synthetic sequence containing a HindIII site). After cleavage with HindIII endonuclease and electrophoresis, the resulting HindIII-BamHI fragment (of approximately 420-bp) is isolated and purified. 
     b) Preparation of the termination sequence comprising the nopaline synthase (NOS) terminator of Agrobacterium tumefaciens. 
     Starting with plasmid pBI121 (Clontech), by cleavage using the restriction enzymes SacI and EcoRI followed by agarose gel electrophoresis, an approximately 250-bp fragment containing the nopaline synthase terminator was isolated. 
     The promoter sequence, the coding sequence of the chimeric gene for chitinase and the termination sequence were ligated using T4 DNA ligase in the shuttle vector pBIN19 opened using HindIII and EcoRI endonucleases. The portion of this vector which may be transferred to plants comprises a canamycin resistance gene immediately upstream of the complete chimeric gene (see BEVAN (1984), Nucl. Ac. Res., 12, 8711-8721). The canamycin resistance gene will serve as a selection marker during the steps of transformation and analysis of the progeny of the transformed plants. 
     The vector obtained is referred to as pBR1. The sequence of the complete chimeric gene (SEQ ID NO: 9) checked by sequencing, is shown in FIG. 5. The plasmid is cloned into E. coli strain MC1061 (Clontech). 
     EXAMPLE 2 
     Transfer into Agrobacterium tumefaciens or Agrobacterium rhizogenes of plasmid pBR1 containing the tomato-tobacco chimeric gene for endochitinase 
     a) Transfer into Agrobacterium tumefaciens 
     This transfer is carried out as described below by triparental conjugation between E. coli strain MC1061 containing the vector pBRl and Agrobacterium tumefaciens strain LBA4404 (Clontech) using E. coli strain HB101 containing the mobilisation plasmid pRK2013. 
     E. coli strain MC1061 containing plasmid pBR1 and an E. coli strain HB101 (Clontech) containing the mobilisation plasmid pRK2013 are cultured at 37° C. in Luria medium (Gibco) in the presence of 25 mg/l of canamycin. 
     Agrobacterium tumefaciens strain LBA4404 is cultured at 28° C. in Luria medium in the presence of 100 mg/l of rifampicin (it is resistant to this antibiotic); 200 μl of each of the three cultures are mixed, plated on Luria agar medium (Gibco) and incubated over-night at 28° C. The bacteria are then resuspended in 5 ml of Luria medium and aliquot portions are plated on Petri dishes containing an agar minimum medium (described in &#34;Plant molecular biology manual&#34; GELVIN et al., Kluwer Academic Press, 1988) in the presence of 100 mg/l of rifampicin and 25 mg/l of canamycin. Under these conditions, only the Agrobacterium tumefaciens colonies which have integrated the plasmid pBR1 grow. These colonies contain the chimeric gene in a context permitting its replication. 
     Resistance of the selected colonies to both antibiotics is checked by subculturing these colonies on the same selection medium twice in succession. The presence of the chimeric gene for endochitinase in Agrobacterium tumefaciens is checked by Southern&#39;s method on a total DNA preparation. (Lysis of the cells, purification of the DNA by extraction using a phenol/chloroform mixture, according to the protocol described by GELVIN in the work cited above, cleavage of the purified DNA using restriction enzymes, agarose gel electrophoresis, transfer onto a membrane and hybridisation according to techniques well known to those skilled in the art). 
     b) Transfer into Agrobacterium rhizogenes 
     This transfer is carried out in the same manner as the transfer into Agrobacterium tumefaciens described in a), with Agrobacterium rhizogenes strain A4 described by GUERCHE et al. (1987) Mol. gen. genet. 206, 382. 
     EXAMPLE 3 
     Production of transformed tobacco plants 
     Nicotiana tabacum tobacco cultured in vitro was infected with Agrobacterium tumefaciens containing plasmid pBR1 according to the procedure of Horsch et al., well known to those skilled in the art (HORSCH R. B. et al. 1985, Science 227, 1229-1231), the main steps of which are described below. 
     Discs of leaves of axenic N. tabacum tobacco plants (variety Wisconsin Havana 38, sensitive to pathogenic fungi) are incubated in a culture of A. tumefaciens harbouring plasmid pBR1. The discs, drained on Whatman paper, were transferred onto culture media in Petri dishes in order to multiply the transformed cells so as to obtain calluses, and then to produce shoots in the presence of cefotaxime (500 μg/ml) and canamycin (100 μg/ml). The canamycin-resistant shoots were then transferred onto a medium permitting the induction of roots in the presence of cefotaxime and canamycin. The plantlets are then transplanted into pots in a substrate composed of peat and compost, and left to grow in the greenhouse. All the transformed plants (Ro generation) which survived the steps of regeneration and acclimatisation in the greenhouse proved morphologically normal and fertile. They were self-fertilised and gave seeds (R 1  generation). 
     EXAMPLE 4 
     Analysis of the genomic DNA of the transformed tobacco plants (Ro generation) according to the SOUTHERN Blot technique 
     The high molecular weight genomic DNA was isolated from mature leaves of transgenic plants of the Ro generation according to the method of extraction using cetyltrimethylammonium bromide and purification by precipitation, described in the work &#34;Plant Molecular Biology Manual&#34; already cited. 
     10 μg of this genomic DNA were digested overnight at 37° C. with 20 units of the restriction enzymes HindIII and EcoRI. The restriction fragments obtained were separated by agarose gel (1%) electrophoresis. The DNA was transferred according to the SOUTHERN Blot method onto a nitrocellulose filter and hybridised with a nucleotide probe comprising the sequence of the recombinant chimeric gene labelledt with α32-dCTP by random labelling (random priming). Washing under highly stringent conditions was carried out in the presence of 0.2×SSC, 0.1% SDS at 68° C. before autoradiography. Analysis of the autoradiogram enables the following conclusions to be drawn: 
     some plants do not possess copies of the transferred gene (absence of signal). 
     most of the plants tested contain at least one copy without rearrangement of the construction: CaMV 35S promoter--endochitinase chimzeric gene--NOS terminator. 
     some profiles suggest that there are internal rearrangements in construction, but these events are rare. 
     EXAMPLE 5 
     Determination for the transformed tobacco plants (Ro, R 1 , and R 2  generations) of the expression of the recombinant endochitinase 
     1) Analysis of the messenger RNA according to the Northern Blot technique. 
     The total RNA of the transformed plants of the Ro generation was isolated according to the protocol of VERWOERD et al., NAR, 17, 2362, 1989. Portions of leaves are removed and ground, then treated with a phenol/Tris-HCl pH 8.0/0.1M LiCl mixture. 
     The RNAs are purified by treatment with chloro-form and then with 2M LiCl and precipitated. 
     15 μg of RNA of each plant are separated by agarose gel (1.2%) electrophoresis under denaturing conditions (Maniatis op. cit.) and then transferred onto a nitrocellulose membrane (Hybond C-extra Amersham). The messenger RNAs (mRNAs) corresponding to the gene introduced are identified using an oligonucleotide probe of sequence (SEQ ID NO: 10) 
     5&#39; AGGGCCGCCACCTGGACACTGA 3&#39; 
     labelled beforehand by means of α32-dCTP, and terminal transferase (Boehringer Mannheim) according to the protocol described in Maniatis et al. (op. cit.). 
     This analysis enabled the presence of a hybridisation signal corresponding to a messenger RNA of approximately 1,500 nucleotides, absent from the untransformed plants, to be detected for the transformed plants. 
     2) Determination of the expression of the endochitinase. 
     The method used employs visualisation of the recombinant endochitinase by immunological techniques. 
     a) Preparation of antibodies: a tomato endochitinase was purified to homogeneity from tomato calluses as described below: tomato calluses were cultured in vitro on a Murashige and Skoog medium (Murashige T. and Skoog F., 1962, Physiol. Plant., 15, 473-497) containing 0.1 mg/l of NAA (naphthaleneacetic acid) and 1 mg/l of BAP (benzylaminopurine). 
     Cell extracts are obtained by grinding the plant material in a 50 mM Tris-HCl buffer solution pH 8.4 containing 15 mM β-mercaptoethanol and 5% of polyvinyl-pyrrolidone. 
     The protein is purified from this extract by ammonium sulphate precipitation, liquid chromatography according to the FPLC technique of PHARMACIA on the cation exchange column based on synthetic polymer (Mono S of Pharmacia) and exclusion chromatography (molecular sieving) on a crosslinked agarose according to the protocol described below: 
     Protocol for purification of tomato endochitinase 
     STEP 1 
     The protein extract is precipitated with ammonium sulphate (60% saturation). The proteins which have precipitated are recovered by centrifugation (15,000 g for 30 min), solubilised in a buffer solution (100 mM ammonium acetate pH 5.2) and dialysed overnight at 4° C. against 100 mM ammonium acetate buffer solution pH 5.2 
     Immediately before proceeding, the concentration of the buffer solution in the protein extract is brought down to 10 mM by passage through ready-to-use minicolumns (PD10, Pharmacia). 
     STEP 2 
     The protein extract is then purified by ion exchange chromatography based on synthetic polymer (Mono-S column of Pharmacia) using an FPLC technique (Pharmacia). 
     The extract is placed on the Mono-S column equilibrated with 10 mM ammonium acetate buffer pH 5.2. The proteins retained on the column are eluted with a linear gradient from 10 to 500 mM ammonium acetate. 
     STEP 3 
     The fractions containing tomato endochitinase are concentrated by ultrafiltration on a Centricon 10 membrane (Amicon). Purification of the protein is continued by chromatography (molecular sieving) on a crosslinked agarose (SUPEROSE 12 column, Pharmacia); elution is carried out with 500 mM ammonium acetate buffer solution pH 5.2. 
     At each step, the tomato endochitinase is identified by its molecular weight (polyacrylamide gel electrophoresis in the presence of SDS--visualisation with silver), and its endochitinase activity measured by a radiochemical method (see Example 9 below) using labelled chitin as substrate (MOLANO et al. (1977) Anal. Biochem 83, 648-656). 
     25 μg of tomato endochitinase were then injected into rabbits in 500 μl of Freund&#39;s complete adjuvant. 
     Three booster injections of 25 μg in Freund&#39;s incomplete adjuvant (500 μl) were carried out at 3-week intervals. The immune serum was drawn after the last injection. 
     b) Preparation of crude protein extracts of transformed tobacco plants (Ro generations: 
     The crude protein extracts were prepared from various tissues of the plant (root, stem, leaf, and the like). The tissue fragments were frozen in liquid nitrogen, reduced to powder and stored at -20° C. The powder was extracted at 4° C. in the presence of 0.1M ammonium acetate buffer pH 5.2 and subjected to centrifugation at 10,000 g. The concentration of total proteins was determined on the supernatants, hereinafter referred to as the crude protein extracts, according to the technique of Bradford (Bradford, M. M., (1976) Anal. Biochem., 72, 248-254). 
     c) Detection by immunoblotting (WesternBlot.) 
     The crude protein extracts of various transformed plants and untransformed plants (controls) were subjected to Western Blot, a technique well known to those skilled in the art and described, in particular, by H. TOWBIN et al.: Proc. Ntl. Acad. Sci. USA, 76, 1972, 4350-4354, which comprises the following steps: 
     denaturation by boiling for 10 min in a buffer, designated loading buffer, consisting of 0.125M Tris-HCl pH 6.8, 4% SDS, 0.002% bromophenol blue, 20% glycerol and 10% β-mercaptoethanol, according to the protocol described by LAEMMLI (U. K. LAEMMLI, Nature, 227 (1970), 680-685); 
     electrophoretic separation of the different proteins contained in the solubilisate according to the protocol described by LAEMMLI (U. K. LAEMMLI, Nature, 227 (1970), 680-685); 
     electrotransfer of the said proteins contained in the gel onto a PVDF membrane (according to the technique of H. TOWBIN et al. Proc. Natl. Acad. Sci. USA 76 (1979) 4350-4354). 
     Immunodetection is carried out according to a protocol comprising the following steps: 
     saturation of the PVDF membrane onto which the proteins have been transferred by incubation for at least 2 hours at 37° C. in a 3% gelatin solution 
     3 washes in phosphate-buffered saline containing 0.05% of Tween 20 detergent 
     incubation (1 hour at 37° C.) in the presence of the immune serum prepared above (containing polyclonal antibodies recognising the recombinant protein), diluted to 1/10,000 in phosphate-buffered saline 
     3 washes in phosphate-buffered saline containing 0.05% of Tween 20 detergent. 
     The antigen-antibody complex is then visualised using a streptavidin-biotin system conjugated to alkaline phosphatase with AMERSHAM kit BN 23 (Blotting-detection kit) used according to the manufacturer&#39;s directions. 
     The blot obtained shows the presence of a protein of approximately 26 kDa for the transformed plants, absent from the control plants. (The protein deduced from the sequence of the chimeric gene, when its assumed signal peptide has been cleaved off, has a molecular mass of approximately 32 kDa). 
     Analysis according to the Northern Blot technique and according to the Western Blot technique was performed on 30 transformed plants (responding positively to Southern Blot). 28 plants showed an expression of the messenger RNA of the chimeric gene in Northern Blot and an expression of the recombinant endochitinase in Western Blot. The non-expression in the case of 2 plants probably results from insertion of the chimeric gene in an untranscribed context. 
     Analysis according to the Northern Blot technique and according to the Western Blot technique was also performed on the plants of the R 1  generation derived from transformed plants of the Ro generation expressing the recombinant protein, and on plants of the R 2  generation derived from plants of the R 1  generation expressing the recombinant protein. In keeping with Mendelian segregation (see Example 6 below), most but not all of the plants of the R 1  generation and of the R 2  generation express the recombinant protein. 
     These results hence show the stability of the insertion of the gene in the tobacco plants, and of its expression during successive generations. 
     EXAMPLE 6 
     Genetic analysis of the transformed tobacco plants (R 1  generation) 
     Tobacco plants regenerated (Ro generation) in the presence of canamycin were self-pollinated. The mature seeds (R 1  generation) are harvested and stored in Eppendorf tubes at 4° C. The seeds are surface-sterilised using 2% aqueous calcium hypochlorite solution. The seeds are then rinsed with sterile water, dried for 24 h in a laminar-flow hood on filter paper and left to germinate on Murashige and Skoog agar medium supplemented with 100 μg/ml of canamycin (the Kanamycin resistance gene linked to the complete chimeric gene and transferred to the tobacco plant at the same time as the latter serves here as a selection marker). 
     Genetic analysis was performed on the progeny of 16 transformed plants (of the Ro generation) chosen from the 28 plants expressing the recombinant endochitinase (see Example 4), designated by the abbreviation Tn (n being the No. assigned to the plant) and of one untransformed control Nicotiana tabacum var. Wisconsin Havana 38 plant, designated by the abbreviation WH 38. 
     The number of individuals observed (total population) varies according to the progeny from 27 to 139. The germination rate is high (of the order of 95%), and comparable for all the plants studied. 
     Two types of phenotypes are observed at the time of germination of the seeds: 
     Kanamycin-resistant plantlets which grow well in the presence of 100 μg/ml of canamycin and possess a developed root system and green leaves, 
     Kanamycin-sensitive plantlets, corresponding either to plants which do not develop roots and which produce white leaves, or to plants for which the root system is reduced and which produce leaves with white areas. 
     The genetic segregation is defined as the ratio of the number of plants resistant to the number of plants sensitive to Kanamycin. 
     Table 1 below collates the results obtained: 
     
                                           TABLE 1__________________________________________________________________________SEGREGATIONS OBSERVED IN THE PROGENY OF TRANSFORMEDTOBACCO PLANTS AND INTERPRETATION                                   Conclu-                                   sion:     Km.sup.r        Km.sup.s           Total       Km.sup.r                          Km.sup.s actual     observed           popu-               Tested theoretical                       theoretical segre-PLANT     populations           lations               segregation                       populations                             Chi Square                                   gation__________________________________________________________________________Transformed T1  62 27 89  3:1     66.75                          22.25                             1.35  3:1plants T2  66 14 80  3:1     60 20 2.40  3:1 T4  66 25 91  3:1     68.25                          22.75                             0.30  3:1 T6  86 5  91  15:1    85.31                          5.69                             0.09  15:1 T11 48 11 59  3:1     44.25                          14.75                             1.27  3:1 T12 61 31 92  3:1     69 23 3.71  3:1 T14 85 3  88  15:1    82.5                          5.5                             1.21  15:1 T16 73 21 94  3:1     70.5                          23.5                             0.35  3:1 T19 74 19 93  3:1     69.75                          23.25                             1.04  3:1 T27 35 13 48  3:1     36 12 0.11  3:1 T28 51 19 70  3:1     52.5                          17.5                             0.17  3:1 T29 59 26 85  3:1     63.75                          21.25                             1.42  3:1 T30 17 10 27  3:1     20.25                          6.75                             1.59  3:1 T31 139        0  139 --      -- -- --    &gt;2loci T36 65 25 90  3:1     67.50                          22.50                             0.37  3:1 T37 71 25 96  3:1     72 24 0.06  3:1Control WH138     0  89 89  --      -- -- --    --plant__________________________________________________________________________ WH38: untransformed Nicotiana tabacum var. Wisconsin Havana 38 plant Tn: progeny of the transformed plant expressing the recombinant endochitinase Km.sup.r : number of Kanamycinresistant plants; Khi2 at the 5% level = 3.84 Km.sup.s : number of Kanamycinsensitive plants When the observed Khi2 is less than 3,84, the observed and assumed segregations coincide. 
    
     Statistical analysis of the results collated in Table 1 above shows that the character of canamycin resistance, genetically linked to the character conferred by the endochitinase chimeric gene, behaves as a single dominant Mendelian character (Mendelian segregation 3:1 or 15:1) present at a single :Locus (one or several similar copies of the gene T1, T2, T4, T11, T12, T16, T.19, T27, T28, T29, T30, T36 and T37--3:1), at two loci (two assemblies genetically far apart each comprising one or several genetically similar copies of the gene T6 and T14 15:1) or at more than two loci (in the case of the plant T31). 
     The number of loci in each plant was confirmed by analysis of the progeny of the R 2  generation. 
     EXAMPLE 7 
     Measurement of the resistance of the transformed plants (R 1  generation) to pathogenic fungi 
     Canamycin-resistant plantlets of the R 1  generation derived from the 16 chosen transformed plants, from one Nicotiana tabacum var. Wisconsin Havana 38 plant sensitive to Chalara elepans (also known as Thielaviopsis basicola), designated by the abbreviation WH38, and from one Nicotiana tabacum var. Paraguay 49 plant, designated by the abbreviation P49, genetically tolerant to this fungus, were transferred to the greenhouse for assessment of their resistance to this fungus. The latter was chosen since it is representative of the pathogenic fungi of tobacco possessing chitin in their wall. The study covered populations of plantlets varying from 15 to 36 according to the plants. The protocol chosen in this study is described below: 
     The plantlets are cultivated in small pots (3×3 cm). On appearance of the 5th leaf, the plants are inoculated by depositing a suspension of endoconidia (5×10 5  spores/ml) on the hypocotyl. The endoconidia are taken from mycelia cultures of this fungus maintained on potato dextrose agar medium (Difco) at 22° C. and in darkness. Resistance to Chalara elegans is assessed by assigning a score 45 days after inoculation. The plants are scored according to the symptoms of infection and according to their level of vegetative development relative to an uninoculated control (this control is an uninoculated WH38 plant for the plants derived from the 16 chosen transformed plants and from the WH38 plant, and an uninoculated P49 plant for the plants derived from the P49 plant). The classes are defined according to the following criteria: 
     Score 0: plant dead; score 1: terminal bud still green, root system destroyed; score 2: plant development not exceeding 25% of that of the control, root system completely necrotic; score 3: plant development attaining 50% of the development of the control, root system exhibiting healthy parts; score 4: plant development identical to the control. 
     The index of resistance of the progeny of a transformed plant represents the mean of the scores assigned to the plantlets derived from this plant. 
     Table 2 below collates the results obtained. 
     
                       TABLE 2______________________________________MEASUREMENT OF THE RESISTANCE OF PROGENYOF TRANSFORMED TOBACCO PLANTS TOPATHOGENIC FUNGI           Population                    Index of resistance    Plant  tested   of the progeny______________________________________Transformed      T1       32       2.030plants     T2       31       0.065      T4       36       1.200      T6       34       0.743      T11      35       2.514      T12      33       1.632      T14      26       1.769      T16      36       1.750      T19      36       1.416      T27      20       0.050      T28      27       1.444      T29      36       1.750      T30      15       2.666      T31      36       2.888      T36      36       1.686Control    WH38     34       0.044plants     P49      34       2.823______________________________________ WH38: untransformed Nicotiana tabacum var. Wisconsin Havana 38 plant P39: Nicotiana tabacum var. Paraguay 49 plant Tn: progeny of the transformed plant expressing the recombinant endochitinase. 
    
     It is observed on reading the above table that all the progenies of the transformed plants Tn possess an index of resistance greater than that of the progeny of the WH38 control plant (untransformed plant), and sometimes close to or even greater than that of the progeny of the genetically resistant P49 control plant. 
     EXAMPLE 8 
     Production of transformed rape plants 
     The transformation is carried out according to the protocol of P. GUERCHE et al. (P. GUERCHE et al. 1987, Mol. Gen. Genet., 206, 382). The various culture media are those described by Pelletier et al. (Pelletier et al., 1983, Mol. gen. genet., 191, 244). Details of their composition will be given later (Table 3). 
     a) Production of transformed roots 
     Stem segments are removed from the apical tip of rape plants (Brassica napus: spring varieties Brutor and Westar and winter variety) approximately 1 m high. These segments are surface-sterilised, rinsed in sterile water, cut into segments approximately 1.5 cm long and placed in a tube containing medium A. 
     Inoculation of the tip of this segment is performed by depositing a suspension of the Agrobacterium rhizogenes strain containing plasmid pBR1. 
     Transformed roots appear on the stem segment after 1 to 2 weeks; they are removed and placed on medium B containing agar (15 g/l) and supplemented with 500 μg of cefotaxime/ml. 
     b) Production of transformed calluses 
     Root fragments are incubated for 15 days on medium D containing 3 mg/l of 2,4-dichlorophenoxyacetic acid, and then transferred onto the same medium containing agar (15 g/l) for the purpose of multiplication of the transformed cells so as to obtain calluses and to yield crude extracts intended for purification of the recombinant protein (see Example 10 below). 
     c) Regeneration of transformed plants 
     Root fragments are incubated for 15 days on medium D containing 3 mg/l of 2,4-dichlorophenoxyacetic acid, and then placed on RCC medium for induction of buds. Rooted plants are then obtained by transfer of the buds to media F and G. 
     
                       TABLE 3______________________________________Composition of the various media used for the production oftransformed rape plantsComposition    Medium(mg/l)   A       B       D     RCC   F     G______________________________________NH.sub.4 NO.sub.3    1,650           200   1,650 1,650 825KNO.sub.3    1,900   2,500   1,250 1,900 1,900 950(NH.sub.4).sub.2 SO.sub.4            134     67NaH.sub.2 PO.sub.4            150     75KH.sub.2 PO.sub.4    170             35    170   170   85CaCl.sub.2.2H.sub.2 OO    440     750     525   440   440   220MgSO.sub.4.7H.sub.2 O    370     250     250   370   370   185H.sub.3 BO.sub.3    12.4    3       12.4  12.4  6.2   6.2MnSO.sub.4.4H.sub.2 O    33.6    10      33.6  33.6  22.3  22.3ZnSO.sub.4.7H.sub.2 O    21      2       21    21    8.6   8.6KI       1.66    0.75    1.66  1.66  0.83  0.83Na.sub.2 MoO.sub.4.    0.5     0.25    0.5   0.5   0.25  0.252H.sub.2 OCuSO.sub.4.5H.sub.2 O    0.05    0.025   0.05  0.05  0.025 0.025CoCl.sub.2.6H.sub.2 O    0.05    0.025   0.05  0.05  0.025 0.025FeSO.sub.4.7H.sub.2 O    22.24   27.8    27.8  27.8  27.8  22.24Na.sub.2 EDTA    29.84   37.3    37.3  37.3  37.3  29.84Inositol 100     100     100   100   100   100Nicotinic acid    0.5     1       1     0.5   1     0.5Pyridoxine HCl    0.5     1       1     0.5   1     0.5Thiamine         10      10          10Glycine  2                     2           2Glucose  10,000  20,000                    10,000Sucrose  10,000          20,000                          10,000                                10,000D-Mannitol       70,000        10,000NAA              1             1     0.1   0.01BA               1             0.5   0.52,4D             0.25    1Adenine                  30sulphateIPA                            0.5GA                             0.02Tween 80         10Agar     8,000                 8,000 8,000 8,000pH       5.8     5.8     5.8   5.8   5.8   5.8Gentamicin    10(sulphate)______________________________________ NAA = naphthaleneacetic acid BA = 6benzylaminopurine acid 2,4D = 2,4dichlorophenoxyacetic acid IPA = N.sup.6(Δ.sup.2isopentenyl)adenine GA.sub.3 = gibberellic acid EDTA = ethylenediaminetetraacetic acid. 
    
     EXAMPLE 9 
     Analysis of the genomic DNA of the transformed rape plants (Ro generation) and determination for the latter and their progeny of the expression of the recombinant endochitinase 
     1) Analysis of the genomic DNA according to the Southern Blot technical 
     Analysis of the genomic DNA according to the Southern Blot technique, performed under the conditions described in Example 4, enabled it to be established that most of the plants tested contain at least one copy without rearrangement of the construction CaMV 35S promoter--enochitinase chimeric gene--NOS terminator. 
     2) Analysis of the messenger RNA according to the Northern Blot technique 
     Analysis of the messenger RNA according to the Northern Blot technique, performed under the conditions described in Example 5, was performed only for a few plants, analysis according to the Western Blot technique being faster for yielding the expected information. It enabled the presence of a messenger RNA of approximately 1,500 nucleotides, absent from the untransformed plants, to be detected for the transformed plants analysed. 
     3) Determination of the expression of the recombinant endochitinase by Western Blot 
     Western blot analysis, performed under the conditions and using the antibodies described in Example 5 on the crude protein extracts of transformed rape plants (prepared as described in Example 5 for the crude protein extracts of transformed tobacco plants) enabled the recombinant protein to be visualised. 
     The blot obtained shows the presence of a protein of approximately 26 kDa for the transformed plants, absent from the control plants (the protein deduced from the sequence of the chimeric gene, when its signal peptide has been cleaved off, has a molecular mass of approximately 32 kDa), and also the presence of a protein of approximately 38 kDa recognised by the antibodies, also present in untransformed plants. The latter protein is an endogenous endochitinase (Atta K. K. et al., 1988, Abstracts of the Second International Congress of Plant Molecular Biology, Jerusalem) which exhibits serological features in common with those of the recombinant endochitinase. 
     Analysis according to the Western Blot technique was performed on 42 transformed plants (responding positively to Southern Blot). 38 plants showed an expression of the recombinant endochitinase. The non-expression observed in the case of 4 plants probably results from insertion of the chimeric gene in an untranscribed context. 
     Analysis according to the Western Blot technique was also performed on plants of the R 1  generation derived from transformed plants of the Ro generation expressing the recombinant endochitinase. In keeping with the laws of genetics applying to heredity of diploids, most but not all of these plants expressed the recombinant protein. 
     These results show the stability of the insertion of the gene in the rape plants, and of its expression during the generations. 
     EXAMPLE 10 
     Purification of the recombinant endochitinase of transformed rape calluses (Ro generation), measurement of its enzymatic activity and determination of its amino-terminal sequence 
     1) Purification of the recombinant endochitinase: 
     The recombinant protein was purified from the crude protein extracts of transformed rape calluses, by ammonium sulphate precipitation, FPLC liquid chromatography on a cation exchange column based on synthetic polymer and exclusion chromatography (molecular sieving) on a crosslinked agarose, according to the protocol described below: 
     Protocol for purification of the recombinant endochitinase 
     STEP 1 
     The protein extract is precipitated with ammonium sulphate (60% saturation). The proteins which have precipitated are recovered by centrifugation (15,000 g for 30 min), solubilised in a buffer solution (100 mM ammonium acetate pH 5.2) and dialysed overnight at 4° C. against 100 mM ammonium acetate buffer solution pH 5.2 
     Immediately before proceeding, the concentration of the buffer solution in the protein extract is brought down to 10 mM by passage through ready-to-use minicolumns (PD10, Pharmacia). 
     STEP 2 
     The protein extract is then purified by ion exchange chromatography based on synthetic polymer (Mono-S column of Pharmacia) using an FPLC technique (Pharmacia). 
     The extract is placed on the Mono-S column equilibrated with 10 mM ammonium acetate buffer pH 5.2. The proteins retained on the column are eluted with a linear gradient from 10 to 500 mM ammonium acetate. 
     STEP 3 
     The fractions containing the recombinant endochitinase are concentrated by ultrafiltration on a Centricon 10 membrane (Amicon). Purification of the protein is continued by exclusion chromatography (molecular sieving) on a crosslinked agarose (SUPEROSE 12 column, Pharmacia), elution being carried out with 500 mM ammonium acetate buffer solution pH 5.2. 
     At each step, the tomato endochitinase is identified by its molecular weight (polyacrylamide gel electrophoresis in the presence of SDS--visualisation with silver), by its immunoblot (see Example 5 c)) and its endochitinase activity, measured by a radiochemical method described below using labelled chitin as substrate (MOLANO et al. (1977) Anal. Biochem 83, 648-656). 
     2) Measurement of the enzymatic activity of the recombinant endochitinase. 
     a) Method 
     The endochitinase activity is measured by a radiochemical method employing tritium-labelled chitin as substrate, according to a protocol described by MOLANO et al., 1977, Anal. Biochem 83, 648-656, summarised below. 
     To 50 μl of tritiated chitin (50 kBq/ml), washed beforehand by 4 successive centrifugations and renewal of the solvent, 50 μl of fraction containing the recombinant endochitinase are added, followed by 250 μl of 0.2M sodium acetate buffer solution pH 4.5. After incubation for 45 min at 20° C., the reaction is stopped by adding 100 μl of 20% trichloroacetic acid. After centrifugation (10,000 g for 10 min), the quantity of radioactivity solubilised in 100 μl of supernatant is measured by liquid scintillation. 
     At each step of purification according to the method described above, the recombinant protein (identified by means of its molecular weight and its positive reaction with polyclonal antibodies to tomato endochitinase) shows an endochitinase activity. 
     b) Results 
     The specific activities, measured at the end of step 1, step 2 and step 3, are 135, 7,416 and 32,193 cpm/μg of protein, respectively. 
     3) Determination of the amino-terminal sequence of the mature recombinant endochtitinase. 
     After purification of the recombinant endochitinase according to the protocol described above, sequencing of the amino-terminal end was carried out. The samples to be treated are carried to the surface of a PVDF (polyvinylidene difluoride) filter by electrotransfer according to the method described by H. TOWBIN et al., Proc. Ntl. Acad. Sci. USA (1979), 4350-4354, after polyacrylamide gel electrophoresis in the presence of SDS. The filter is introduced into a protein sequencer (model 470 A marketed by the company Applied Biosystems (USA)) equipped with a chromatograph (Applied Biosystems model 430) which analyses continuously the phenylthio-hydantoin derivatives formed, after each degradation cycle. 
     The amino-terminal sequence determined (SEQ ID NO: 11) is shown below, the symbol Xaa representing an undetermined amino acid: 
     Gly-Gly-Xaa-Leu-Gly-Ser-VaL-Ile-Ser-Asn-Xaa-Met-Phe-Xaa-Gln-Met-Leu-Lys-Xaa-Arg 
     It is seen that the beginning of the sequence of the mature protein (SEQ ID NO: 1) shown in FIG. 6 corresponds to the 76th amino-acid from amino-terminal methionine deduced from the sequence of the chimeric gene (SEQ ID NO: 12), such as shown in FIG. 4 and SEQ ID NOs. 12 and 13. 
     The protein translated from the messenger RNA encoded by the chimeric gene undergoes a cleavage of its assumed signal peptide of 24 amino acids (G. von Heijne, 1986, Nucl. Ac. Res., 14, 483-490), followed by a maturation producing the cleavage of an amino-terminal peptide of 51 amino acids. 
     The sequence of the chimeric gene hence contains the information necessary for the synthesis of a protein of the prepro-enzyme type, which is matured to active endochitinase. 
     EXAMPLE 11 
     Genetic analysis of the transformed rape plants (R 1  generation) 
     The regenerated rapes (R 0  generation) were self-pollinated. The mature seeds (R 1  generation) are collected and stored in bags. Seeds are then sown in boxes on vermiculite, then the young plants are replanted individually in 2-liter pots containing horticultural compost. The expression of the recombinant protein is emphasized by the Western Blot technique on young leaves (see paragraph 3 of Example 9) after extraction of the proteins according to the protocole described in Example 5b). 
     In accordance with the laws of genetics applying to heredity of diploids, most but not all of these plants express the recombinant protein. 
     The progeny of 15 of the transformed rape plants were statistically analyzed according to the protocole described in Example 7. The obtained results show that the expression character of the endochitinase chimeric gene behaves as a single dominant Mendelian character present at a single locus (12 progenies out of 15 exhibit the Mendelian segregation 3:1) or at two loci (3-progenies out of 15 exhibit the Mendelian segregation 15:1). 
     EXAMPLE 12 
     Measurement of the resistance of the transformed rape plants (R 2  generation) to pathogenic fungi 
     The R 1  generation plants, expressing the recombinant protein are self-pollinated. the R 2  generation seeds obtained are germinated as described in Example 11. 
     The resistance of the rape plants expressing the recombinant protein is determined on the R 2  generation plants by inoculation in culture chamber using Alternaria brassicae, a fungus representative of the pathogenic fungi of the rape plant, according to the protocole described by Bains and Tewari, 1987, Physiol. Mol. Plant. Pathol. 30: 259 summarized hereafter. 
     Young rape plants, 21 days old, are inoculated with a suspension of spores deposited on the central vein of the first leaf, previously pricked with a needle. Two weeks later, the extent of the necrosis resulting from the growth of the parasitic fungus is measured. 
     The results obtained from the progeny of 10 transformed plants, show that the progeny of three plants exhibit a considerably increased resistance, close to that of a mustard variety Sinapis alba, Bains and Tewari, referenced above, genetically resistant to Alternaria brassicae. 
     EXAMPLE 13 
     Obtention of transformed roots of sunflower 
     Segments of petioles are taken from Helianthus annuus sunflower plants (Euroflor Rustica seeds variety between 6 and 10 weeks old. The segments are disinfected by soaking for 30 mins. in a 1% solution of calcium hypochlorite. 
     The segments of petioles are then placed in a tube containing a quantity of the gelose-containing Murashige and Skoog culture :medium. The inoculation of the end of these segments is carried out by depositing a suspension of the Agrobacterium rhizogenes strain containing the pBR1 plasmid. 
     Transformed roots appear on the segment of petiole after about 1 month . These roots are taken out and placed on the agar medium M (medium M to which 6 g/l of agarose have been added), containing 500 μg of cefotaxime/ml. The composition of the medium M is given hereinafter (Table 4). These roots are replanted every week for 4 weeks in the same medium. Then they are transferred on the liquid medium M, in order to obtain the production of roots in quantity sufficient to analyze the expression of the recombinant protein by the Western Blot technique according to the protocole described in paragraph 3 of Example 9. The crude protein extracts to be used for this analysis are prepared according to the technique described in Example 5. The blots obtained show the presence of a protein of expected molecular weight (26 kDa) for the transformed roots, absent from the control roots and leaves of sunflower plants (non-transformed plants). 
     
                       TABLE 4______________________________________Composition of the culture medium M used for the cultureof transformed roots of sunflower.         Composition         mg/l______________________________________NH.sub.4 NO.sub.3           330KNO.sub.3       380K.sub.2 PO.sub.4           170MgSO.sub.4      370CaCl.sub.2      440H.sub.3 BO.sub.3           6.3MnSO.sub.4, 4H.sub.2 O           22.3ZnSO.sub.4, 7H.sub.2 O           1.6KI              0.83Na.sub.2M oO.sub.4, 2H.sub.2O           0.25CuSO.sub.4, 5H.sub.2 O           0.025CoCl2, 6H.sub.2 O           0.025Pyridoxine HCl  0.1Nicotinic acid  0.1Glycine         0.4Inositol        20Thiamine        0.02Sucrose         30,000Iron citrate    200______________________________________ 
    
     
         __________________________________________________________________________SEQUENCE LISTING(1) GENERAL INFORMATION:(iii) NUMBER OF SEQUENCES: 15(2) INFORMATION FOR SEQ ID NO:1:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 254 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: protein(xi) SEQUENCE DESCRIPTION: SEQ ID NO:1:GlyGlyAspLeuGlySerValIleSerAsnSerMetPheAspGlnMet151015LeuLysHisArgAsnGluAsnSerCysGlnGlyLysAsnAsnPheTyr202530SerTyrAsnAlaPheIleThrAlaAlaArgSerPheProGlyPheGly354045ThrSerGlyAspIleAsnAlaArgLysArgGluIleAlaAlaPhePhe505560AlaGlnThrSerHisGluThrThrGlyGlyTrpProSerAlaProAsp65707580GlyProPheAlaTrpGlyTyrCysPheLeuArgGluArgGlyAsnPro859095GlyAspTyrCysSerProSerSerGlnTrpProCysAlaProGlyArg100105110LysTyrPheGlyArgGlyProIleGlnIleSerHisAsnTyrAsnTyr115120125GlyProCysGlyArgAlaIleGlyValAspLeuLeuAsnAsnProAsp130135140LeuValAlaThrAspProValIleSerPheLysThrAlaIleTrpPhe145150155160TrpMetThrProGlnSerProLysProSerCysHisAspValIleIle165170175GlyArgTrpAsnProSerAlaGlyAspArgSerAlaAsnArgLeuPro180185190GlyPheGlyValIleThrAsnIleIleAsnGlyGlyLeuGluCysGly195200205ArgGlyAsnAspAsnArgValGlnAspArgIleGlyPheTyrArgArg210215220TyrCysGlyIleLeuGlyValSerProGlyAspAsnLeuAspCysGly225230235240AsnGlnArgSerPheGlyAsnGlyLeuLeuValAspThrMet245250(2) INFORMATION FOR SEQ ID NO:2:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 51 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(xi) SEQUENCE DESCRIPTION: SEQ ID NO:2:GlnAsnCysGlySerGlnGlyGlyGlyLysValCysAlaSerGlyGln151015CysCysSerLysPheGlyTrpCysGlyAsnThrAsnAspHisCysGly202530SerGlyAsnCysGlnSerGlnCysProGlyGlyGlyProGlyProGly354045ProValThr50(2) INFORMATION FOR SEQ ID NO:3:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 24 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(xi) SEQUENCE DESCRIPTION: SEQ ID NO:3:MetArgArgThrSerLysLeuThrThrPheSerLeuLeuPheSerLeu151015ValLeuLeuSerAlaAlaLeuAla20(2) INFORMATION FOR SEQ ID NO:4:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 1153 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(xi) SEQUENCE DESCRIPTION: SEQ ID NO:4:ATGAGGCGAACTTCTAAATTGACTACTTTTTCTTTGCTGTTTTCTCTGGTTTTGCTGAGT60GCTGCCTTGGCACAGAATTGTGGTTCACAGGGCGGAGGCAAAGTTTGTGCGTCGGGACAA120TGTTGCAGCAAATTCGGGTGGTGCGGTAACACTAATGACCATTGTGGTTCTGGCAATTGT180CAAAGTCAGTGTCCAGGTGGCGGCCCTGGTCCTGGTCCTGTTACTGGTGGGGACCTCGGA240AGCGTCATCTCAAATTCTATGTTTGATCAAATGCTTAAGCATCGTAACGAAAATTCTTGT300CAAGGAAAGAATAATTTCTACAGTTACAATGCCTTTATTACTGCTGCTAGGTCTTTTCCT360GGCTTTGGTACAAGTGGTGATATCAATGCCCGTAAAAGGGAAATTGCTGCTTTCTTTGCC420CAAACCTCCCATGAAACTACTGGTATGTGTATAACCATTCACATCGAACCATTAAAATAT480AATTTCATTTTATTTTATTTAGTAATTGATTATATATGTAGGAGGATGGCCTTCCGCACC540TGATGGACCATTCGCATGGGGTTACTGTTTCCTTAGAGAACGAGGTAACCCCGGTGACTA600CTGTTCACCAAGTAGTCAATGGCCTTGTGCACCTGGAAGGAAATATTTCGGACGAGGCCC660AATCCAAATTTCACAGTAAGCTACATAAATCTATATATGGTAAAATTTGATGAACTTGTA720GTGTCTAATTACGTGTATTTTGACATTTCAAAACAGCAACTACAACTATGGGCCATGTGG780AAGAGCCATCGGAGTGGACCTTTTAAACAATCCTGATTTAGTAGCCACAGACCCAGTCAT840CTCATTCAAGACTGCTATCTGGTTCTGGATGACCCCTCAATCACCAAAGCCTTCTTGCCA900CGATGTCATCATTGGAAGATGGAACCCATCTGCCGGTGACCGATCAGCCAATCGTCTTCC960TGGATTTGGTGTCATCACAAACATCATCAATGGGGGCCTGGAATGTGGTCGTGGCAATGA1020CAATAGGGTCCAGGATCGCATTGGGTTTTACAGGAGGTATTGCGGTATTCTTGGTGTTAG1080TCCTGGTGACAATCTTGATTGCGGAAACCAGAGATCTTTTGGAAACGGACTTTTAGTCGA1140TACTATGTAATGA1153(2) INFORMATION FOR SEQ ID NO:5:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 3012 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(ix) FEATURE:(A) NAME/KEY: intron(B) LOCATION: 2384..2462(D) OTHER INFORMATION: /number=1(ix) FEATURE:(A) NAME/KEY: intron(B) LOCATION: 2617..2697(D) OTHER INFORMATION: /number=2(ix) FEATURE:(A) NAME/KEY: CDS(B) LOCATION: join(1942..2383, 2463..2616, 2698..3007)(ix) FEATURE:(A) NAME/KEY: sig.sub.-- peptide(B) LOCATION: 1942..2166(ix) FEATURE:(A) NAME/KEY: mat.sub.-- peptide(B) LOCATION: join(2167..2383, 2463..2616, 2698..3007,2698)(xi) SEQUENCE DESCRIPTION: SEQ ID NO:5:GAATTCATATTTATTTTAAAAAAATATTTTCAACTTCAAAAATATATTTTTTTCACGCCT60ACCCTCGACCCCCCTCCCGCACCCTTACCCGCCCTCTACCAACCCCCCCCCCCCCAAAAA120AAAATAAATTAAAGTTTACTTTTAAAAATATTTTCAACTTCAAAATTTCATTTTTTTTCA180TCCCTACCCTCGACCACCCCCACCCTCCCGCTAAAAAATAAAAGTTTAAGTTTGTTTTTG240AAAAGTATTTTCAACTTCAAAAATTCATTTTTTCACCCCTAACCTCAACCCCCCACCCAC300ATTCCCACCCCAATTTTTTTTTTTAAGTTTGTTGTTAAAAAATATTTTCTACTTCAAAAT360TTCATTTCACCCTTTCCCCCCCCCCTCCCCAAACCCCACCCCACCCCCCCACCCCCCAAA420AAAAATATTTAAATTTGTTTTTAAAAAATATTTTCAATTTCAAAATTTTATTTTCTATTC480TAGTAAAAATAAAAGATATATCTCAAAAACATTTTTTACTTATTCAAAAACCAAACACTC540TTTTCCAGAAAAAATTTCTATTCACCAACCAAATATGAGAAAATAAATCAAAATCTAGTT600ATTTTAGAAAATGTTTTCCTACATATCAAACACACCCAATGTCTTCATTAATGTGTTCAG660ATTTATTTTATGTCAACTTGGTCGCTATGTTATATGAATTAGCCACACAAATTCAATTTA720ATTGCACATTACCACTATTTTGTAGTTCACGTAGAAATTAAAGTTCATCACAACAAAATA780AATATTGGGCGCACGGGCGACTCCCCACTAGTATCACTCAGAAATCACAATAAAGTATTA840AATTTTGTCAAAATTCTTTATCCGTATTAAGAAATCTTTGAAGTCTGAATACATATAAAT900TCATAATTCATAAATTTCAAATTTCTCTTAGTAATTTTTATTGAGTTATTAATTTCATTT960AAACAAATTCATTGTACTTTGTAAATACTCCTAATTTGTATGATTTTGGACTCATGTAAG1020GAAACCTTATCAAATTAAGTATGGAGTTAAAGGGGAAGAGTAGAATTAGCAGCCCAAAGA1080TACACTTTCAAATTATGTAAGTTTGACCCAGCCTGCCCTATTTCTTCTAGCACCAGCTGC1140TACCTTATATAATTACTTTAATTTGAAAATGTCATCAATATCATGCAAAATTTACCGGCC1200CTATTTCTTCTAGCACTAGCTACTACCTTATATAATTACTTTAATTTGTAAGTGTCATCA1260ATATCATGCAAAATTTAGTCAAAATATTTATCTCGATGTCTTTGGTTCTCAAATAGAGCA1320AATAGACTCAGACTCGAACCTACGCAAGTGTAAAAGCAAGGAATGATTACCAAACAAGAC1380AGTTCTCAACAAGCAACAAAATAAACAAGGCAAAACTAGTTAGAAAACGAATGCTATTGT1440CATTCCAGCCGAACTAACAATAACCTACATACAAACCAGTTCAACCTTTAGCTTTACTTT1500TACCATTTTTGGCTCTTTTGTTAATTGAGATTTGAAATAAATCTCAACAATAATTTATTT1560ATGATCCACATGACATTAGTCTAAGAGGTGATTGAACATTACTTGAGAGATATTGCTATT1620CGATGAGTTACATAGTTTTCCACTACAAATTTAATTTACTCTAACTATGAATATTATAAT1680TTGTAGTACAGTTTTTATTTAATAGGTAAATTTAATAAGAGTAAACAAAAAATATCCAGC1740AACTATAGTCTCCAGTCCAAATTATGTAGAGAAAAGTCTGGAATAACGTCCAAAGCCGCC1800CGTCTCTTTTACTTATAACTGAATTAAATTCTGGATACGACAGGGTGGACTATCAATTTT1860GTCATAAAAGTCACTGATTCCTCACAACCACTTGCCTATAAATAGCTTTCACTTTAGCAT1920TTGTTTGCCATCACATTCAAAATGAGGCGAACTTCTAAATTGACTACTTTT1971MetArgArgThrSerLysLeuThrThrPhe75-70TCTTTGCTGTTTTCTCTGGTTTTGCTGAGTGCTGCCTTGGCACAGAAT2019SerLeuLeuPheSerLeuValLeuLeuSerAlaAlaLeuAlaGlnAsn65-60-55-50TGTGGTTCACAGGGCGGAGGCAAAGTTTGTGCGTCGGGACAATGTTGC2067CysGlySerGlnGlyGlyGlyLysValCysAlaSerGlyGlnCysCys45-40-35AGCAAATTCGGGTGGTGCGGTAACACTAATGACCATTGTGGTTCTGGC2115SerLysPheGlyTrpCysGlyAsnThrAsnAspHisCysGlySerGly30-25- 20AATTGTCAAAGTCAGTGTCCAGGTGGCGGCCCTGGTCCTGGTCCTGTT2163AsnCysGlnSerGlnCysProGlyGlyGlyProGlyProGlyProVal15-10-5ACTGGTGGGGACCTCGGAAGCGTCATCTCAAATTCTATGTTTGATCAA2211ThrGlyGlyAspLeuGlySerValIleSerAsnSerMetPheAspGln151015ATGCTTAAGCATCGTAACGAAAATTCTTGTCAAGGAAAGAATAATTTC2259MetLeuLysHisArgAsnGluAsnSerCysGlnGlyLysAsnAsnPhe202530TACAGTTACAATGCCTTTATTACTGCTGCTAGGTCTTTTCCTGGCTTT2307TyrSerTyrAsnAlaPheIleThrAlaAlaArgSerPheProGlyPhe354045GGTACAAGTGGTGATATCAATGCCCGTAAAAGGGAAATTGCTGCTTTC2355GlyThrSerGlyAspIleAsnAlaArgLysArgGluIleAlaAlaPhe505560TTTGCCCAAACCTCCCATGAAACTACTGGTATGTGTATAACCATTCAC2403PheAlaGlnThrSerHisGluThrThr6570ATCGAACCATTAAAATATAATTTCATTTTATTTTATTTAGTAATTGATTATATATGTAGGA2464GlyGGATGGCCTTCCGCACCTGATGGACCATTCGCATGGGGTTACTGTTTC2512GlyTrpProSerAlaProAspGlyProPheAlaTrpGlyTyrCysPhe758085CTTAGAGAACGAGGTAACCCCGGTGACTACTGTTCACCAAGTAGTCAA2560LeuArgGluArgGlyAsnProGlyAspTyrCysSerProSerSerGln9095100105TGGCCTTGTGCACCTGGAAGGAAATATTTCGGACGAGGCCCAATCCAA2608TrpProCysAlaProGlyArgLysTyrPheGlyArgGlyProIleGln110115120ATTTCACAGTAAGCTACATAAATCTATATATGGTAAAATTTGATGAAC2656IleSerHisTTGTAGTGTCTAATTACGTGTATTTTGACATTTCAAAACAGCAACTACAACTAT2710AsnTyrAsnTyr125GGGCCATGTGGAAGAGCCATCGGAGTGGACCTTTTAAACAATCCTGAT2758GlyProCysGlyArgAlaIleGlyValAspLeuLeuAsnAsnProAsp130135140TTAGTAGCCACAGACCCAGTCATCTCATTCAAGACTGCTATCTGGTTC2806LeuValAlaThrAspProValIleSerPheLysThrAlaIleTrpPhe145150155160TGGATGACCCCTCAATCACCAAAGCCTTCTTGCCACGATGTCATCATT2854TrpMetThrProGlnSerProLysProSerCysHisAspValIleIle165170175GGAAGATGGAACCCATCTGCCGGTGACCGATCAGCCAATCGTCTTCCT2902GlyArgTrpAsnProSerAlaGlyAspArgSerAlaAsnArgLeuPro180185190GGATTTGGTGTCATCACAAACATCATCAATGGGGGCCTAGAATGTGGT2950GlyPheGlyValIleThrAsnIleIleAsnGlyGlyLeuGluCysGly195200205CGTGGTAATGACAACAGGGTACAAGATCGAATTGGATTTTACAGGAGG2998ArgGlyAsnAspAsnArgValGlnAspArgIleGlyPheTyrArgArg210215220TATTGCGGAAGCTT3012TyrCysGly225(2) INFORMATION FOR SEQ ID NO:6:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 302 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: protein(xi) SEQUENCE DESCRIPTION: SEQ ID NO:6:MetArgArgThrSerLysLeuThrThrPheSerLeuLeuPheSerLeu75-70-65-60ValLeuLeuSerAlaAlaLeuAlaGlnAsnCysGlySerGlnGlyGly55-50-45GlyLysValCysAlaSerGlyGlnCysCysSerLysPheGlyTrpCys40-35- 30GlyAsnThrAsnAspHisCysGlySerGlyAsnCysGlnSerGlnCys25-20-15ProGlyGlyGlyProGlyProGlyProValThrGlyGlyAspLeuGly10- 515SerValIleSerAsnSerMetPheAspGlnMetLeuLysHisArgAsn101520GluAsnSerCysGlnGlyLysAsnAsnPheTyrSerTyrAsnAlaPhe253035IleThrAlaAlaArgSerPheProGlyPheGlyThrSerGlyAspIle404550AsnAlaArgLysArgGluIleAlaAlaPhePheAlaGlnThrSerHis556065GluThrThrGlyGlyTrpProSerAlaProAspGlyProPheAlaTrp70758085GlyTyrCysPheLeuArgGluArgGlyAsnProGlyAspTyrCysSer9095100ProSerSerGlnTrpProCysAlaProGlyArgLysTyrPheGlyArg105110115GlyProIleGlnIleSerHisAsnTyrAsnTyrGlyProCysGlyArg120125130AlaIleGlyValAspLeuLeuAsnAsnProAspLeuValAlaThrAsp135140145ProValIleSerPheLysThrAlaIleTrpPheTrpMetThrProGln150155160165SerProLysProSerCysHisAspValIleIleGlyArgTrpAsnPro170175180SerAlaGlyAspArgSerAlaAsnArgLeuProGlyPheGlyValIle185190195ThrAsnIleIleAsnGlyGlyLeuGluCysGlyArgGlyAsnAspAsn200205210ArgValGlnAspArgIleGlyPheTyrArgArgTyrCysGly215220225(2) INFORMATION FOR SEQ ID NO:7:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 71 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:7:GGATCCATGAGGCGAACTTCTAAATTGACTACTTTTTCTTTGCTGTTTTCTCTGGTTTTG60CTGAGTGCTGC71(2) INFORMATION FOR SEQ ID NO:8:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 163 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:8:GGCCTGGAATGTGGTCGTGGCAATGACAATAGGGTCCAGGATCGCATTGGGTTTTACAGG60AGGTATTGCGGTATTCTTGGTGTTAGTCCTGGTGACAATCTTGATTGCGGAAACCAGAGA120TCTTTTGGAAACGGACTTTTAGTCGATACTATGTAATGAGCTC163(2) INFORMATION FOR SEQ ID NO:9:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 1863 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:9:AAGCTTGCACGACACACTTGTCTACTCCAAAAATATCAAAGATACAGTCCTCAGAAGACC60AAAGGGCCAATTGAGACTTTTCAACAAAGGGTAATATCCGGAAACCTCCTCGGATTCCAT120TGCCCAGCTATCTGTCACTTTATTGTGAAGATAGTGGAAAAGGAAGGTGGCTCCTACAAA180TGCCATCATTGCGATAAAGGAAAGGCCATCGTTGAAGATGCCTCTGCCGACAGTGGTCCC240AAAGATGGACCCCCACCCACGAGGAGCATCGTGGAAAAAGAAGACGTTCCAACCACGTCT300TCAAAGCAAGTGGATTGATGTGATATCTCCACTGACGTAAGGGATGACGCACAATCCCAC360TATCCTTCGCAAGACCCTTCCTCTATATAAGGAAGTTCATTTCATTTGGAGAGAACACGG420GGGACTCTAGAGGATCCATGAGGCGAACTTCTAAATTGACTACTTTTTCTTTGCTGTTTT480CTCTGGTTTTGCTGAGTGCTGCCTTGGCACAGAATTGTGGTTCACAGGGCGGAGGCAAAG540TTTGTGCGTCGGGACAATGTTGCAGCAAATTCGGGTGGTGCGGTAACACTAATGACCATT600GTGGTTCTGGCAATTGTCAAAGTCAGTGTCCAGGTGGCGGCCCTGGTCCTGGTCCTGTTA660CTGGTGGGGACCTCGGAAGCGTCATCTCAAATTCTATGTTTGATCAAATGCTTAAGCATC720GTAACGAAAATTCTTGTCAAGGAAAGAATAATTTCTACAGTTACAATGCCTTTATTACTG780CTGCTAGGTCTTTTCCTGGCTTTGGTACAAGTGGTGATATCAATGCCCGTAAAAGGGAAA840TTGCTGCTTTCTTTGCCCAAACCTCCCATGAAACTACTGGTATGTGTATAACCATTCACA900TCGAACCATTAAAATATAATTTCATTTTATTTTATTTAGTAATTGATTATATATGTAGGA960GGATGGCCTTCCGCACCTGATGGACCATTCGCATGGGGTTACTGTTTCCTTAGAGAACGA1020GGTAACCCCGGTGACTACTGTTCACCAAGTAGTCAATGGCCTTGTGCACCTGGAAGGAAA1080TATTTCGGACGAGGCCCAATCCAAATTTCACAGTAAGCTACATAAATCTATATATGGTAA1140AATTTGATGAACTTGTAGTGTCTAATTACGTGTATTTTGACATTTCAAAACAGCAACTAC1200AACTATGGGCCATGTGGAAGAGCCATCGGAGTGGACCTTTTAAACAATCCTGATTTAGTA1260GCCACAGACCCAGTCATCTCATTCAAGACTGCTATCTGGTTCTGGATGACCCCTCAATCA1320CCAAAGCCTTCTTGCCACGATGTCATCATTGGAAGATGGAACCCATCTGCCGGTGACCGA1380TCAGCCAATCGTCTTCCTGGATTTGGTGTCATCACAAACATCATCAATGGGGGCCTGGAA1440TGTGGTCGTGGCAATGACAATAGGGTCCAGGATCGCATTGGGTTTTACAGGAGGTATTGC1500GGTATTCTTGGTGTTAGTCCTGGTGACAATCTTGATTGCGGAAACCAGAGATCTTTTGGA1560AACGGACTTTTAGTCGATACTATGTAATGAGCTCGAATTTCCCCGATCGTTCAAACATTT1620GGCAATAAAGTTTCTTAAGATTGAATCCTGTTGCCGGTCTTGCGATGATTATCATATAAT1680TTCTGTTGAATTACGTTAAGCATGTAATAATTAACATGTAATGCATGACGTTATTTATGA1740GATGGGTTTTTATGATTAGAGTCCCGCAATTATACATTTAATACGCGATAGAAAACAAAA1800TATAGCGCGCAAACTAGGATAAATTATCGCGCGCGGTGTCATCTATGTTACTAGATCGAA1860TTC1863(2) INFORMATION FOR SEQ ID NO:10:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 22 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO:10:AGGGCCGCCACCTGGACACTGA22(2) INFORMATION FOR SEQ ID NO:11:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 20 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: peptide(xi) SEQUENCE DESCRIPTION: SEQ ID NO:11:GlyGlyXaaLeuGlySerValIleSerAsnXaaMetPheXaaGlnMet151015LeuLysXaaArg20(2) INFORMATION FOR SEQ ID NO:12:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 1163 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(ix) FEATURE:(A) NAME/KEY: intron(B) LOCATION: 449..527(D) OTHER INFORMATION: /number=1(ix) FEATURE:(A) NAME/KEY: intron(B) LOCATION: 682..762(D) OTHER INFORMATION: /number=2(ix) FEATURE:(A) NAME/KEY: CDS(B) LOCATION: join(7..448, 528..681, 763..1153)(ix) FEATURE:(A) NAME/KEY: sig.sub.-- peptide(B) LOCATION: 7..231(ix) FEATURE:(A) NAME/KEY: mat.sub.-- peptide(B) LOCATION: join(232..448, 528..681, 763..1153)(xi) SEQUENCE DESCRIPTION: SEQ ID NO:12:GGATCCATGAGGCGAACTTCTAAATTGACTACTTTTTCTTTGCTGTTT48MetArgArgThrSerLysLeuThrThrPheSerLeuLeuPhe75-70-65TCTCTGGTTTTGCTGAGTGCTGCCTTGGCACAGAATTGTGGTTCACAG96SerLeuValLeuLeuSerAlaAlaLeuAlaGlnAsnCysGlySerGln60-55-50GGCGGAGGCAAAGTTTGTGCGTCGGGACAATGTTGCAGCAAATTCGGG144GlyGlyGlyLysValCysAlaSerGlyGlnCysCysSerLysPheGly45-40-35-30TGGTGCGGTAACACTAATGACCATTGTGGTTCTGGCAATTGTCAAAGT192TrpCysGlyAsnThrAsnAspHisCysGlySerGlyAsnCysGlnSer25-20-15CAGTGTCCAGGTGGCGGCCCTGGTCCTGGTCCTGTTACTGGTGGGGAC240GlnCysProGlyGlyGlyProGlyProGlyProValThrGlyGlyAsp10-51CTCGGAAGCGTCATCTCAAATTCTATGTTTGATCAAATGCTTAAGCAT288LeuGlySerValIleSerAsnSerMetPheAspGlnMetLeuLysHis51015CGTAACGAAAATTCTTGTCAAGGAAAGAATAATTTCTACAGTTACAAT336ArgAsnGluAsnSerCysGlnGlyLysAsnAsnPheTyrSerTyrAsn20253035GCCTTTATTACTGCTGCTAGGTCTTTTCCTGGCTTTGGTACAAGTGGT384AlaPheIleThrAlaAlaArgSerPheProGlyPheGlyThrSerGly404550GATATCAATGCCCGTAAAAGGGAAATTGCTGCTTTCTTTGCCCAAACC432AspIleAsnAlaArgLysArgGluIleAlaAlaPhePheAlaGlnThr556065TCCCATGAAACTACTGGTATGTGTATAACCATTCACATCGAACCAT478SerHisGluThrThr70TAAAATATAATTTCATTTTATTTTATTTAGTAATTGATTATATATGTAGGAGGA532GlyGlyTGGCCTTCCGCACCTGATGGACCATTCGCATGGGGTTACTGTTTCCTT580TrpProSerAlaProAspGlyProPheAlaTrpGlyTyrCysPheLeu75808590AGAGAACGAGGTAACCCCGGTGACTACTGTTCACCAAGTAGTCAATGG628ArgGluArgGlyAsnProGlyAspTyrCysSerProSerSerGlnTrp95100105CCTTGTGCACCTGGAAGGAAATATTTCGGACGAGGCCCAATCCAAATT676ProCysAlaProGlyArgLysTyrPheGlyArgGlyProIleGlnIle110115120TCACAGTAAGCTACATAAATCTATATATGGTAAAATTTGATGAACTTGTAGTGTC731SerHisTAATTACGTGTATTTTGACATTTCAAAACAGCAACTACAACTATGGGCCATGT784AsnTyrAsnTyrGlyProCys125130GGAAGAGCCATCGGAGTGGACCTTTTAAACAATCCTGATTTAGTAGCC832GlyArgAlaIleGlyValAspLeuLeuAsnAsnProAspLeuValAla135140145ACAGACCCAGTCATCTCATTCAAGACTGCTATCTGGTTCTGGATGACC880ThrAspProValIleSerPheLysThrAlaIleTrpPheTrpMetThr150155160CCTCAATCACCAAAGCCTTCTTGCCACGATGTCATCATTGGAAGATGG928ProGlnSerProLysProSerCysHisAspValIleIleGlyArgTrp165170175AACCCATCTGCCGGTGACCGATCAGCCAATCGTCTTCCTGGATTTGGT976AsnProSerAlaGlyAspArgSerAlaAsnArgLeuProGlyPheGly180185190195GTCATCACAAACATCATCAATGGGGGCCTGGAATGTGGTCGTGGCAAT1024ValIleThrAsnIleIleAsnGlyGlyLeuGluCysGlyArgGlyAsn200205210GACAATAGGGTCCAGGATCGCATTGGGTTTTACAGGAGGTATTGCGGT1072AspAsnArgValGlnAspArgIleGlyPheTyrArgArgTyrCysGly215220225ATTCTTGGTGTTAGTCCTGGTGACAATCTTGATTGCGGAAACCAGAGA1120IleLeuGlyValSerProGlyAspAsnLeuAspCysGlyAsnGlnArg230235240TCTTTTGGAAACGGACTTTTAGTCGATACTATGTAATGAGCTC1163SerPheGlyAsnGlyLeuLeuValAspThrMet245250(2) INFORMATION FOR SEQ ID NO:13:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 329 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: protein(xi) SEQUENCE DESCRIPTION: SEQ ID NO:13:MetArgArgThrSerLysLeuThrThrPheSerLeuLeuPheSerLeu75-70-65-60ValLeuLeuSerAlaAlaLeuAlaGlnAsnCysGlySerGlnGlyGly55-50-45GlyLysValCysAlaSerGlyGlnCysCysSerLysPheGlyTrpCys40-35- 30GlyAsnThrAsnAspHisCysGlySerGlyAsnCysGlnSerGlnCys25-20-15ProGlyGlyGlyProGlyProGlyProValThrGlyGlyAspLeuGly10- 515SerValIleSerAsnSerMetPheAspGlnMetLeuLysHisArgAsn101520GluAsnSerCysGlnGlyLysAsnAsnPheTyrSerTyrAsnAlaPhe253035IleThrAlaAlaArgSerPheProGlyPheGlyThrSerGlyAspIle404550AsnAlaArgLysArgGluIleAlaAlaPhePheAlaGlnThrSerHis556065GluThrThrGlyGlyTrpProSerAlaProAspGlyProPheAlaTrp70758085GlyTyrCysPheLeuArgGluArgGlyAsnProGlyAspTyrCysSer9095100ProSerSerGlnTrpProCysAlaProGlyArgLysTyrPheGlyArg105110115GlyProIleGlnIleSerHisAsnTyrAsnTyrGlyProCysGlyArg120125130AlaIleGlyValAspLeuLeuAsnAsnProAspLeuValAlaThrAsp135140145ProValIleSerPheLysThrAlaIleTrpPheTrpMetThrProGln150155160165SerProLysProSerCysHisAspValIleIleGlyArgTrpAsnPro170175180SerAlaGlyAspArgSerAlaAsnArgLeuProGlyPheGlyValIle185190195ThrAsnIleIleAsnGlyGlyLeuGluCysGlyArgGlyAsnAspAsn200205210ArgValGlnAspArgIleGlyPheTyrArgArgTyrCysGlyIleLeu215220225GlyValSerProGlyAspAsnLeuAspCysGlyAsnGlnArgSerPhe230235240245GlyAsnGlyLeuLeuValAspThrMet250(2) INFORMATION FOR SEQ ID NO:14:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 905 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(xi) SEQUENCE DESCRIPTION: SEQ ID NO:14:ATGAGGCGAACTTCTAAATTGACTACTTTTTCTTTGCTGTTTTCTCTGGTTTTGCTGAGT60GCTGCCTTGGCACAGAATTGTGGTTCACAGGGCGGAGGCAAAGTTTGTGCGTCGGGACAA120TGTTGCAGCAAATTCGGGTGGTGCGGTAACACTAATGACCATTGTGGTTCTGGCAATTGT180CAAAGTCAGTGTCCAGGTGGCGGCCCTGGTCCTGGTCCTGTTACTGGTGGGGACCTCGGA240AGCGTCATCTCAAATTCTATGTTTGATCAAATGCTTAAGCATCGTAACGAAAATTCTTGT300CAAGGAAAGAATAATTTCTACAGTTACAATGCCTTTATTACTGCTGCTAGGTCTTTTCCT360GGCTTTGGTACAAGTGGTGATATCAATGCCCGTAAAAGGGAAATTGCTGCTTTCTTTGCC420CAAACCTCCCATGAAACTACTGGAGGATGGCCTTCCGCACCTGATGGACCATTCGCATGG480GGTTACTGTTTCCTTAGAGAACGAGGTAACCCCGGTGACTACTGTTCACCAAGTAGTCAA540TGGCCTTGTGCACCTGGAAGGAAATATTTCGGACGAGGCCCAATCCAAATTTCACACAAC600TACAACTATGGGCCATGTGGAAGAGCCATCGGAGTGGACCTTTTAAACAATCCTGATTTA660GTAGCCACAGACCCAGTCATCTCATTCAAGACTGCTATCTGGTTCTGGATGACCCCTCAA720TCACCAAAGCCTTCTTGCCACGATGTCATCATTGGAAGATGGAACCCATCTGCCGGTGAC780CGATCAGCCAATCGTCTTCCTGGATTTGGTGTCATCACAAACATCATCAATGGGGGCCTG840GAATGTGGTCGTGGCAATGACAATAGGGTCCAAGATCGCATTGGGTTTTACAGGAGGTAT900TGCGG905(2) INFORMATION FOR SEQ ID NO:15:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 943 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(xi) SEQUENCE DESCRIPTION: SEQ ID NO:15:TCTCTCCTACTCCTCTCTGCCTCGGCAGAACAATGTGGTTCGCAGGCGGGAGGTGCGCGT60TGTGCCTCGGGTCTCTGCTGCAGCAAATTTGGTTGGTGTGGTAACACCAATGACTATTGT120GGCCCTGGCAATTGCCAGAGCCAGTGCCCTGGTGGTCCCACACCACCCGGTGGTGGGGAT180CTCGGCAGTATCATCTCAAGTTCCATGTTTGATCAGATGCTTAAGCATCGCAACGATAAT240GCATGCCAAGGAAAGGGATTCTACAGTTACAATGCCTTTATCAATGCTGCTAGGTCTTTT300CCTGGCTTTGGTACTAGTGGTGATACCACTGCCCGTAAAAGAGAAATCGCGGCTTTCTTC360GCCCAAACCTCCCATGAAACTACAGGAGGATGGGCAACAGCACCAGATGGTCCATACGCG420TGGGGTTACTGCTGGCTTAGAGAACAAGGTAGCCCCGGCGACTACTGTACACCAAGTGGT480CAGTGGCCTTGTGCTCCTGGTCGGAAATATTTCGGACGAGGCCCCATCCAAATTTCACAC540AACTACAACTACGGACCTTGTGGAAGAGCCATAGGAGTGGACCTCCTAAACAATCCTGAT600TTAGTGGCCACAGATCCAGTAATCTCATTCAAGTCAGCTCTCTGGTTTTGGATGACTCCT660CAATCACCAAAACCTTCTTGCCACGATGTCATCATTGGAAGATGGCAACCATCGTCTGCT720GACCGCGCAGCCAATCGTCTCCCTGGATTTGGTGTCATCACGAACATCATCAATGGTGGC780TTGGAATGTGGTCGTGGCACTGACTCAAGGGTCCAGGATCGCATTGGGTTTTACAGGAGG840TATTGCAGTATTCTTGGTGTTAGTCCTGGTGACAATCTTGATTGCGGAAACCAGAGGTCT900TTTGGAAACGGACTTTTAGTCGATACTATGTAATTTTATGGTC943__________________________________________________________________________