Abstract:
The present invention relates to a plant promoter which comprises the sequence (B)  SEQ ID NO: 4! below: ##STR1## or a sequence having a high degree of homology with the sequence (B). Application: Protection of plants by genetic engineering and especially defense of plants in stress conditions

Description:
The present invention relates to a novel plant promoter and to the microorganisms and plant cells containing a unit for the expression of a protein of interest comprising said promoter. The promoter according to the invention is a strong constitutive promoter enabling said protein to be expressed in microorganisms and plant cells irrespective of the stage of development of the plant. 
     Furthermore, the promoter according to the invention has a particular application in the field of the protection of plants by genetic engineering and especially that of the defense of plants in stress conditions. 
     BACKGROUND OF THE INVENTION 
     The applications of plant transformation have increased over recent years. Numerous genes of prokaryotic or eukaryotic (animal or vegetable) origin, coding especially for proteins which confer a novel agronomic property when expressed, have been isolated and then transferred to plants. 
     In a very large number of cases, the genes which have been introduced into plants by genetic engineering are chimeric, associating regulatory elements of different origins. Thus, very often, the gene coding for a protein of interest is placed under the control of a strong constitutive promoter enabling said protein to be expressed in the whole plant (or the major part thereof) throughout its life, irrespective of the stage of development. The promoter of the 35S transcript of the cauliflower mosaic virus (35S CaMV), which is the most widely used in constructions of chimeric genes, corresponds to this description. 
     Now, for a number of applications, it is not necessary for the gene coding for the protein of interest, supporting the agronomic property, to have a continuous expression or an expression distributed throughout the whole plant. In certain cases, such characteristics can even reduce or annul the beneficial effects of the transferred gene. In fact, the continuous expression of a protein at a high level can divert part of the metabolism towards this expression and ultimately cause a loss of yield. 
     Very soon, the search for et more specific gene expression was undertaken; it led for example to the isolation of tissue- or organ-specific promoters. 
     It can be of interest to induce the expression of a given gene only in a precise situation or, preferably, to ensure a base expression level throughout the life of a plant while at the same time allowing the superexpression of the gene in a given situation. 
     Several inducible promoters have already been described, some of which respond both to infection by pathogenic microorganisms and to chemical compounds or plant hormones, such as ethylene (Roby et al., 1990, Plant Cell, 2, 999) or auxin. 
     A plant promoter isolated from tobacco has been described by Takahashi et al., Proc. Natl. Acad. Sci. USA, 1990, 87, 8013-8016. 
     In another publication, these authors state that this promoter reacts specifically only to auxins and not to other hormones or to stress (Takahashi et al., The Plant Journal, 1991, 1(3), 327-332). 
     SUMMARY OF THE INVENTION 
     The present invention relates to a promoter which is expressed at a sustained level in the different organs and tissues of a plant, and especially the roots and meristem of a plant, and which is very strongly inducible in stress situations such as, in particular, after a heat shock, a wound, a hormone shock, a biotic or abiotic elicitor or a bacterial, fungal or viral infection. 
     The invention further relates to the microorganisms (bacteria) and plant cells which have integrated a unit for the expression of a protein of interest, said unit comprising the promoter according to the invention. 
     It further relates to the plants or parts of plants and the seeds which comprise the plant cells of the invention. 
     Finally, it further relates to the use of one of the above plants or parts of plants for selecting molecules with plant protection activity which are capable of inducing natural defense reactions in plants against the aggressions of phytopathogenic or phytophagic organisms (fungi, bacteria, viruses, insects and nematodes). 
     The promoter according to the invention comprises the DNA sequence (B)  SEQ ID NO: 4! or a sequence having a high degree of homology with the sequence (B). 
     In one variant, the promoter according to the invention contains, upstream from the sequence (B), a sequence (C)  SEQ ID NO: 5! or a sequence having a high degree of homology with the sequence (C). 
     Finally, in a preferred variant of the invention, the promoter of the invention contains, upstream from the sequence (B), a sequence (D)  SEQ ID NO: 6! or a sequence having a high degree of homology with the sequence (D). 
     Here a high degree of homology denotes a homology (ratio of the identical nucleotides to the total number of nucleotides) of at least 70%, and preferably of at least 80%, of the nucleotide sequences when they are aligned according to the maximum homology by the optimal sequence alignment method of Needleman and Wunsch, 1970; J. Mol. Biol., 48, 443-453. This method is used especially in the UWGCG software of the University of Wisconsin: Devereux et al. , 1984, Nucl. Ac. Res. , 12, 387-395--option GAP. 
     The elements necessary for the function of this promoter and for the expression of its characteristics (transactivating factors etc. ) are present in other dicotyledonous or monocotyledonous plants. Their presence therefore enables this promoter to be used in numerous cultivated plants such as, in particular, tobacco, potato, tomato, maize, sunflower, barley and colza plants, or other plants such as yeasts and fungi. 
     Any DNA sequences coding for proteins of interest can be placed under the control of the promoter according to the invention, particularly sequences coding for proteins which make it possible to ensure the protection of a plant, for example against viral, bacterial or fungal infections and against the other stress conditions. Examples of such proteins which may be mentioned in particular are the tomato-tobacco endochitinases such as that described in EP-A-493 581, whose coding sequence is  SEQ ID NO: 16!. 
     The promoter according to the invention was obtained by screening a tobacco gene library with the aid of a DNA probe having the sequence  SEQ ID NO: 1!. 
     A clone corresponding to the sequence  SEQ ID NO: 1! was obtained by the differential screening of cDNA clones derived from poly(A) +   mRNAs specifically synthesized during the infection of Nicotiana tabacum tobacco leaves with Pseudomonas solanacearum strain GMI1000. This bacterial strain is well known for causing a hypersensitivity reaction on tobacco of the Bottom Special variety. In this connections reference may be made to the work by Message et al. , 1978, Proc. 4th Intl. Conf. of Plant Pathogenic Bacteria, pp. 823-833. The clone containing the sequence  SEQ ID NO: 1! will hereafter be called the &#34;246 clone&#34;. 
     The 246 clone then made it possible, by the screening of a tobacco gene library, to isolate a clone, hereafter called the 246C clone  SEQ ID NO: 7!, which contains the DNA sequence (D)  SEQ ID NO: 6!, the DNA sequence (C)  SEQ ID NO: 5!, the DNA sequence (B)  SEQ ID NO: 4! and a sequence containing 2 open reading frames separated by an intron. 
     Following the procedure described in section 9 below, association of the promoter (sequences B+C+D) with the β-glucuronidase gene gave expression vector pSG123. The promoter consisting of the sequences B+C+D is called the 246C promoter. 
     Expression vector pSG123 was used to test the transient expression of the glucuronidase gene in tobacco protoplasts, said protoplasts being placed in a stress situation either by infection with Pseudomonas solanacearum or by treatment with an elicitor or a hormone. 
     Following the procedure described in section 13, expression vector pSG123 was used to prepare an expression vector stable in plant cells, namely binary vector pSG246. 
     This binary vector pSG246, was transferred to Agrobacterium tumefaciens or Agrobacterium rhizogenes cells, which were then used to obtain transgenic tobacco, colza and sunflower plants. Expression vector pSG123 was used for the transformation of tissues of monocotyledons (barley and maize). The behavior of these plants or tissues in stress conditions was studied. 
     The promoter according to the invention, comprising the sequence (B), (C) and (D), was also associated with the gene coding for tomato-tobacco chitinase. The resulting chimeric genes were used for transforming Agrobacterium cells. 
     The DNA sequence  SEQ ID NO: 1! can easily be synthesized by the techniques well known to those skilled in the art (L. J. MacPRIDE and H. M. CARUTHURS, Tetrahedron Letters (1983) vol. 24, 245). 
     A study of the transgenic plants obtained by the transformation of plants with the aid of Agrobacterium cells obtained above made it possible to demonstrate the base promoting activity of the promoter according to the invention, and the superexpression of the proteins of interest (β-glucuronidase and chitinase) in stress situations. 
     The results included in the illustrative part below clearly show that the promoter according to the invention has a base promoting activity which is greatly enhanced when the transgenic plants containing this promoter and a gene coding for a protein of interest are placed in stress conditions: heat shock, wound, infection with pathogens (fungi, bacteria), elicitors (biotic and abiotic). 
     Different deletions of plasmid pSG123, carried out in the 5&#39; region of the promoter with the aid of restriction enzymes and/or nuclease Exo3, demonstrated the existence of vectors pSG251 and pSG33, the respective sequences of which are the sequence (B) (pSG33)  SEQ ID NO: 4! or the sequence (B) containing the sequence (C) (pSG251)  SEQ ID NO: 5! upstream. 
     Easy visualization of the expression of glucuronidase (Jefferson et al. , 1987, Plant Molec. Biol. Reporter, 5, 387), or of its superexpression in the case of induction of the promoter of the invention, makes it possible to use plants which express this chimeric gene for the selection of inducer molecules. 
     Plants possess defense mechanisms against aggressions, especially parasitic aggressions (fungi, bacteria, viruses or insects); these mechanisms which depend on induction phenomena are not well known and often come into play too late to be effective. Early triggering of these mechanisms (Roby et al. , 1988, Physiol. Molec. Plant Pathol. , 33, 409), especially by elicitor-type compounds in cascade reactions, enables the plant to resist aggressions. 
     Second-generation fungicides, which are active on the plant&#39;s defenses while being inactive on the parasite, have already been marketed. 
     Plants which express glucuronidase under the control of the promoter of the invention, induced early and specifically in a hypersensitivity reaction to a bacterial infection, constitute a preferred tool for selecting molecules capable of inducing the expression or superexpression of defense gene. 
     The invention will be understood more clearly with the aid of the following description divided into sections, which comprises experimental results and a discussion thereof. Some of these sections refer to experiments performed for the purpose of carrying out the invention; others refer to Examples of the invention, which of course are given purely by way of illustration. 
     Most of the techniques below, which are well known to those skilled in the art, are described in detail in the work by Sambrook et al.: &#34;Molecular Cloning: A laboratory manual&#34; published in 1989 by Cold Spring Harbor Press in New York (2nd edition). 
     The biological material (strains, phages, plasmids or plants) used in the sections below is commercially available and/or is described respectively in the following documents: 
     
         ______________________________________binary vector pBIN19:           BEVAN et al., 1984, Nucl. Ac.           Res., 12, 8711-8721, obtained           from Clontech (Palo Alto,           California, USA)vector 101.3:   JEFFERSON, 1987, Plant Molec.           Biol. Reporter, 5, 387-405,           obtained from Clontechvector pBI221:  JEFFERSON, 1987, Plant Molec.           Biol. Reporter, 5, 387-405,           obtained from Clontechvector pBIl2l:  JEFFERSON, 1987, Plant Molec.           Biol. Reporter, 5, 387-405,           obtained from ClontechPseudomonas     MESSAGE et al., 1978, Proc.solanacearum strain           4th Intl. Conf. of PlantGMI1000:        Pathogenic Bacteria, pp. 823-           833Pseudomonas     MESSAGE et al., 1978, Proc.solanacearum strain           4th Intl. Conf. of PlantGMI1178:        Pathogenic Bacteria, pp. 823-           833Pseudomonas     MESSAGE et al., 1978, Proc.solanacearum strain           4th Intl. Conf. of PlantK60:            Pathogenic Bacteria, pp. 823-           833NOS terminator: nopaline synthase terminatorvector pTZ19R:  obtained from PharmaciaE. coli strain MC1061:           MANIATIS et al., 1982,           Molecular Cloning: A labora-           tory manual, Cold Spring           Harbor, New York, obtained           from ClontechE. coli strain HB101:           MANIATIS et al., 1982,           Molecular Cloning: A labora-           tory manual, Cold Spring           Harbor, New York, obtained           from ClontechAgrobacterium   LBA4404, obtained from Clon-tumefaciens strain:           tech, HOEKEMA et al., 1983,           NATURE, 303, 179-180Agrobacterium   pRIA.sub.4rhizogenes strain:Nicotiana tabacum           Wisconsin Havana 38 variety:plant:          SCHNEIDER M., 1990, Plant           Molec. Biol., 14, 935-947Chalara elegans RAWLINGS R. E., 1940, Ann. Mo.fungus:         Bot. Gdn., 27, 561-598Alternaria brassicae           BAINS and TEWARI, 1987,fungus:         Physiol. Mol. Plant Pathol.,           30, 259Nicotiana tabacum           Paraguay 49 variety, obtainedplant:          from the Institut du tabac,           Bergerac, FranceBrassica napus plant:           Brutor and Westar spring           varieties and winter line           (selection line, Rustica           Semences)Rhizoctonia solani           ACHARYA et al., 1984, Can. J.pathogen:       Plant Pathol., 6, 325-328sunflower plants:           genotype 2603B (selection           line, Rustica Semences)maize:          line LH132barley:         GERBEL variety, obtained from           the Institut National de la           Recherche Agronomique (INRA),           Paris, France______________________________________ 
    
     Strains GMI1000 and K60 can be obtained from the Collection Nationale des Bacteries Phytopathogenes (CNBP) INRA, Pathologie Vegetale, Rue Georges MOREL, 49070 BEAUCOUZE, FRANCE. 
     Strain GMI1178 can be obtained from INRA, Pathologie Vegetale, Chemin de Borde-Rouge, AUZEVILLE BP 27, 31326 CASTANET TOLOSAN Cedex, FRANCE. 
     The following abbreviations are used in the Examples below: 
     32P-dCTP: deoxycytidine 5&#39;- 32  P-triphosphate marketed by AMERSHAM under the reference 10205; 
     2 SSC: NaCl 0.3M, trisodium citrate 30 mM; pH 7.0 (described by MANIATIS et al., op. cit.); 
     SDS: sodium dodecylsulfate; 
     FPLC: fast protein liquid chromatography; 
     PVDF: polyvinylidene difluoride; 
     EDTA: ethylenediaminetetraacetic acid; 
     DEPC: diethyl pyrocarbonate; 
     NAD: nicotinamide adenine dinucleotide. 
    
    
     BRIEF DESCRIPTION OF THE DRAWINGS 
     FIG. 1 represents the mapping of the 246C genomic DNA clone, established with the aid of the restriction enzymes shown. 
     FIG. 2A-2B represent the alignment, according to the optimal alignment method of Needleman and Wunsch, 1970, J. Mol. Biol., 48, 443-453, applied by the UWGCG software of the University of Wisconsin (Devereux et al., 1984, Nucl. Ac. Res., 12, 387-395), option GAP, of the 3&#39; part of 700 bp of the promoter of the 246C gene and the promoter described by Takahashi et al., 1989, Proc. Natl. Acad. Sci. USA, 87, 8013. 
     FIG. 3 represents the different expression vectors tested in which, relative to full-length plasmid pSG123, there is a variable deletion of the 5&#39; part of the promoter. 
    
    
     DETAILED DESCRIPTION OF THE INVENTION 
     Section 1: Infection of tobacco, Nicotiana tabacum, with two strains of the pathogenic bacterium Pseudomonas solanacearum 
     The bacteria of the Pseudomonas solanacearum strain are cultivated for 72 h on BG agar medium (Boucher et al., 1985, J. Gen. Microbiol., 131, 2449); a colony is taken for inoculating 40 ml of the same medium. After 16 to 24 h of incubation at 28° C., the bacterial suspension is centrifuged for 10 min at 6000 g and 4° C.; the supernatant is discarded to leave the polysaccharide layer present on the surface of the residue. After washing with sterile water, the bacteria are resuspended in 20 ml of water. Their concentration is then determined by densitometry. 
     Young tobacco plant leaves are detached from the plant, washed with distilled water and immersed in a desiccator containing 1.2 of bacterial suspension at a concentration of 3×10 6  bacteria/ml. A vacuum is created for 10 min by means of a vacuum pump and is then let down slowly. Each infiltrated leaf is then placed in a beaker containing 10 mM sodium phosphate buffer of pH 6.0, and transferred to a culture chamber. The leaves are removed after different incubation times and stored at -70° C. 
     Two bacterial strains were used, namely strain GMI1000, which causes a hypersensitivity reaction on tobacco of the Bottom Special variety, and strain GMI1178 (Message et al., 1978, Proc. 4th Intl. Conf. of Plant Pathogenic Bacteria, pp. 823-833), a mutant which is derived from the previous strain and has lost the capacity to induce the hypersensitivity reaction in tobacco. 
     Section 2: Extraction and isolation of the total RNAs from Nicotiana tabacum infected with Pseudomonas solanacearum strains 
     10 g of plant material are ground in the presence of liquid nitrogen and then taken up in a mixture of 3 ml of phenol, 3 ml of chloroform/isoamyl alcohol (24:1, v:v) and 6 ml of the lysis buffer of composition Tris-HCl 200 mM pH 7.0, EDTA 200 mM, SDS 1%. 
     After agitation on a Vortex, the phases can be separated by centrifugation for 10 min at 6000 g and 4° C. The aqueous phase is removed and re-extracted with 6 ml of a phenol/chloroform/isoamyl alcohol mixture (25:24:1, v:v) and then with 6 ml of phenol. 16 ml of absolute ethanol and 400 μl of 3M sodium acetate of pH 5.5 are added to the aqueous phase; the mixture is precipitated for 2 h at -20° C. The residue obtained is dissolved in 5 ml of sterile water containing 0.1% of diethyl pyrocarbonate (DEPC), after which the RNAs are precipitated for 12 h at 4° C. following the addition of 5 ml of 4M LiCl. After centrifugation for 20 min at 6000 g, the residue of RNA is washed with 75% ethanol, dried and taken up in 800 μl of sterile distilled water containing 0.1% of DEPC. The solution is precipitated for 2 h at -20° C. following the addition of 0.1 vol of 3M sodium acetate of pH 5.5 and 2.5 vol of absolute ethanol. After centrifugation for 15 min at 12,000 g, the residue of RNA is washed with 75% ethanol and dissolved in 200 μl of distilled water containing 0.1% of DEPC. 
     The total RNAs are then determined by spectrophotometry at 260 nm. 
     Section 3: Preparation of the poly(A) -   messenger RNAs 
     1 g of oligo d(T) cellulose gel (Collaborative Research Inc.) is resuspended in 2 ml of the buffer Tris-HCl 10 mM pH 7.4, EDTA 1 mM, NaCl 0.4M, SDS 0.1%. This gel is introduced into a Pasteur pipette whose end is plugged with glass wool. The RNA solution is heated at 65° C. for 4 min and then left to cool slowly to room temperature. A final NaCl concentration of 0.4M is obtained by adding a 5M NaCl solution. 
     The solution of total RNAs is then deposited on the oligo d(T) cellulose gel. This is then rinsed with about 12 ml of the buffer of composition Tris-HCl 10 mM pH 7.4, NaCl 0.4M, EDTA 1 mM, SDS 0.5%. 
     The poly(A) +   RNAs are subsequently eluted with 7 ml of the buffer of composition Tris-HCl 10 mM pH 7.4, SDS 0.1%, and then precipitated overnight at -20° C. following the addition of 2.5 volumes of 95% ethanol and 0.1 volume of 3.3M sodium acetate of pH 5.5. The residue of poly(A) +   RNAs obtained by centrifugation at 35,000 g for 1 h is washed 3 times with 75% ethanol, dried, taken up in 0.5 ml of sterile distilled water and reprecipitated under the conditions described above. After centrifugation, the residue is then washed with 75% ethanol, dried and dissolved in sterile distilled water. The poly(A) +   RNAs are then determined by spectrophotometry at 260 nm. 
     Section 4: Synthesis of double-stranded DNA from poly(A) +   messenger RNAs isolated from leaves of tobacco infected with Pseudomonas solanacearum strain GMI1000, and cloning into E. coli 
     This synthesis is effected by the method of Gubler and Hoffman (1983, Gene, 25, 263) using the D. Scribe kit from Genofit (Geneva, Switzerland) in accordance with the manufacturer&#39;s instructions. 
     Synthesis of the first strand: 
     2.5 μg of poly(A) +   RNAs isolated from tobacco leaves infected with Pseudomonas solanacearum strain GMI1000 and removed 6 h after inoculation are incubated at 44° C. for 30 to 60 min in the presence of Tris-HCl 40 mM pH 8.3, NaCl 80 mM, MgCl 2  6 nM, DTT 5 mM, dATP 0.5 mM, dTTP 0.5 mM, dGTP 0.5 mM, dCTP 0.5 mM, 1.5 μg of oligo d(pT) 12-18 and 10 to 15 units of AMV (avian myeloblastosis virus) reverse transcriptase in a total volume of 25 μl. 
     Synthesis of the second strand: 
     The reaction medium derived from the synthesis of the first strand is diluted to 100 μl with the buffer of composition Tris-HCl 40 mM pH 7.5, MgCl 2  10 mM, NaCl 80 mM; 2 units of RNase H are added and the mixture is incubated at 37° C. for 5 min. 
     After cooling to 12° C., 25 units of DNA polymerase I, 0.5 Weiss unit of E. coli ligase and NAD in a final concentration of 0.1 mM are added. 
     After incubation for 60 min at 12° C. and then 60 min at 18° C., the reaction is stopped by the addition of EDTA and SDS in final concentrations of 20 mM and 1% respectively, followed by heating for 2 min at 60° C. 
     Purification of the cDNA: 
     This purification is effected by chromatography on a Sephadex G100 column in the buffer Tris-HCl 50 mM pH 7.5, NaCl 300 mM, EDTA 1 mM. The addition of alpha32P-dCTP in the synthesis step affords easier identification of the chromatographic fractions containing the double-stranded DNA. The latter is precipitated by the addition of ammonium acetate (final concentration 0.3M) and 2.5 vol of absolute ethanol. 
     Digestion with nuclease S1: 
     The precipitate obtained is washed with 75% ethanol, dried and taken up in sterile water. The cDNA is then treated with nuclease S1 in a total volume of 300 μl, at 30° C. for 10 min, in the presence of 20 U of enzyme in the buffer of composition sodium acetate 30 mM pH 4.4, NaCl 0.25M, ZnCl 2  1 mM. 
     When the reaction has ended, the mixture is extracted once with a phenol/chloroform/isoamyl alcohol mixture (50:48:2, v:v) and then three times with ethyl ether before being precipitated with ethanol. 
     The DNA precipitate obtained after centrifugation is then dried and taken up in 20 μl of sterile water. 
     Addition of a poly dC tail at the 3&#39; end (dC tailing): 
     The following are added successively to the cDNA solution: 10 μl of the terminal transferase buffer of composition potassium cacodylate 70 mM pH 7.2, CoCl 2  0.5 mM, dithiothreitol 0.5 mM, 2 μl of 0.25 mM α-dCTP, 5 μl of α-32P-dCTP (370MBq/ml), 12 μl of H 2  O and 1.2 μl of terminal transferase (18 units). 
     The tailing reaction is performed by incubation at 37° C. for 30 min and is then stopped by the addition of 30 μl of 0.25M EDTA of pH 8.0. 
     Purification of the double-stranded cDNAs after tailing: 
     The mixture derived from dC tailing is precipitated with ethanol and then centrifuged. The cDNA residue is taken up in 10 μl of the buffer of composition Tris-HCl 10 mM pH 7.5, NaCl 100 mM, EDTA 1 mM, 5% glycerol, 0.02% bromophenol blue. This solution is deposited on a Biogel A 0.5M column (1 ml of support). The column is eluted with the buffer of composition Tris-HCl 10 mM pH 7.5, NaCl 100 mM, EDTA 1 mM; fractions are collected, their radioactivity is measured and the size of the cDNAs they contain is analyzed by agarose gel electrophoresis. The fractions containing cDNAs with a size of more than 500 base pairs are combined and the cDNA is precipitated with ethanol. 
     Hybridization with pBR322-dG: 
     The cDNA collected after precipitation is redissolved in 50 μl of the annealing buffer of composition Tris-HCl 20 mM pH 7.5, NaCl 100 mM, EDTA 1 mM. 4 μl of pBR322-dG solution (21 ng, Clontech) and 46 μl of water are added. 
     After incubation for 15 min at 65° C. and then 2 h at 57° C., the hybridization is checked by agarose gel electrophoresis. 
     The double-stranded cDNA obtained is inserted at the PstI site of plasmid pBR322. After ligation, the DNA obtained is used to transform competent cells of E. coli strain HB101. Colonies of recombinant bacteria are obtained after the transformed competent cells have been plated out and cultured on a Petri dish. 
     Section 5: Selection, by differential screening, of cDNA clones derived from poly(A) +   mRNAs specifically synthesized during bacterial infection with Pseudomonas solanacearum strain GMI1000 
     The DNA of the recombinant bacterial colonies obtained by cloning cDNA synthesized from poly(A) +   messenger RNAs of tobacco leaves infected with strain GMI1000 was transferred to a Biodyne nylon membrane (Pall Corporation, USA) in accordance with the manufacturer&#39;s instructions. These DNAs are hybridized successively with the aid of 2 radioactive probes obtained by the synthesis of cDNA, in the presence of alpha-32P-dCTP, from messenger RNAs purified from plants infected with strains GMI1000 and GMI1178 respectively. 
     After washing and autoradiographic exposure of the membranes, the bacterial colonies which exhibit a stronger hybridization signal with the probe synthesized from leaves inoculated with strain GMI1000 are selected. The plasmid DNA of these colonies is prepared and the cDNA inserts of these plasmids are isolated and then labeled with alpha-32P-dCTP and used as a probe for revealing, by the dot-blot and then Northern blotting technique, the equivalent amounts of corresponding mRNA purified from total RNA of tobacco leaves inoculated with strain GMI1000or GMI1178. 
     The colonies whose insert, used as a probe, gives a more intense signal during the revealing of the total RNAs purified from tobacco leaves inoculated with strain GMI1000 are retained. 
     Section 6: Characterization of a cDNA clone derived from an mRNA specifically synthesized during bacterial infection with Pseudomonas solanacearum strain GMI1000 
     14 bacterial clones were isolated from the cDNA library constructed from messenger RNAs of tobacco leaves infected with Pseudomonas solanacearum strain GMI1000. 
     One of said clones, called 246, with an insert length of 750 base pairs, enables a transcript of about 800 nucleotides to be revealed by Northern blotting. The accumulation of this transcript starts 4 to 9 h after inoculation and reaches a maximum between 12 and 15 h. In the tobacco leaves infected with strain GMI1178, a slight accumulation of the transcript is observed between 12 and 15 h. 
     A study of the sequence of the cDNA of the 246 clone  SEQ ID NO: 1! demonstrates the existence of a first, incomplete open reading frame coding for a peptide of 59 amino acids, and a second, potential reading frame coding for a peptide of 88 amino acids. The sequence of these two peptides is represented by  SEQ ID NO: 2!. Intron splicing consensus sequences (Brown, 1986, Nucl. Ac. Res., 14, 9549) are present between these two reading frames. Cloning of a cDNA from an immature messenger RNA has therefore probably taken place. The cDNA sequence of the 246 clone without the intron is the sequence A 1   SEQ ID NO: 3!. 
     Section 7: Screening of a tobacco gene library with the aid of the characterized cDNA 
     A tobacco DNA gene library was obtained by partial digestion, with the enzyme MboI, of DNA isolated from the germination of Nicotiana tabacum, NK326 variety, and cloning of the restriction fragments into phage EMBL-3 (Clontech). 500,000 recombinant phages were screened after plating at a rate of 10,000 phages per Petri dish by the technique known to those skilled in the art and described in Sambrook et al. (Molecular Cloning, A laboratory manual, Cold Spring Harbor Laboratory Press, 1989). 
     The phage DNA is transferred to a nitrocellulose membrane (BA85, Schleicher and Schull), denatured for 2 min in the solution NaOH 0.5M, NaCl 1.5M and then soaked in the neutralizing solution NaCl 1.5M, Tris-HCl 0.5M pH 7.4 for 5 min. After rapid rinsing in 2 SSC (NaCl 0.3M, sodium citrate 30 mM), the filters are dried for 30 min at 37° C. and the DNA is then fixed by treatment at 80° C. under vacuum for 1 h 30 min. 
     The membranes are then prehybridized for 4 h at 37° C. in the buffer of composition 5 SSC (NaCl 0.75M, sodium citrate 75 mM), 50% formamide, 0.3% skimmed milk. 
     The hybridization is carried out in the same buffer for 18 h at 37° C. after addition of the probe labeled with alpha-32P-dCTP, which consists of the insert of 750 base pairs of the 246 cDNA clone. 
     The membranes are then washed 3 times for 20 min at 37° C. in the solution 5 SSC, SDS 0.1%, then twice for 30 min at 37° C. in the solution 2 SSC, SDS 0.1% and finally for 30 min at 42° C. in the solution 2 SSC, SDS 0.1%; they are then autoradiographed. 
     After developing of the autoradiograms, each lysis plate exhibiting a positive signal is isolated and the phages are eluted in SM medium (NaCl 100 mM, Tris-HCl 50 mM pH 7.5, MgSO 4  5 mM, gelatin 0.01%) and then purified by a further screening effected under the same conditions. 
     12 clones were thus isolated and purified. The DNA of each clone was produced and purified by the technique well known to those skilled in the art, and then digested with the enzyme SalI, which enables the genomic DNA insert to be isolated after agarose gel electrophoresis. 
     Transfer to a nylon membrane, followed by hybridization with the probe consisting of the cDNA of the 246 clone, shows a positive signal, confirming the presence of a sequence complementary to the 246 cDNA in this genomic DNA. 
     These clones were then mapped using a series of restriction enzymes. One clone, which exhibits a hybridization signal in the central region of the fragment inserted into phage DNA, was selected from said clones. This clone was called 246C. 
     Section 8: Sequencing and analysis of the sequence of the 246C genomic DNA clone 
     A fragment of the insert contained in this phage was isolated by digestion with the enzyme SstI and then cloned into phage pBluescript® 11 KS +/- (Stratagene) to give phagemid pKS246. Its mapping was established and is shown in FIG. 1. The sequence of this insert  SEQ ID NO: 7! was then determined by the method of Sanger et al. (PNAS-US. A, 14, 5463, 1977) after the creation of progressive deletions with the aid of the enzymes ExoIII, mung bean and nuclease S1 by Henikoff&#39;s technique (Gene, 28, 351, 1984). 
     This insert of 3046 base pairs, called the 246C gene, consists of a coding region of 853 bp starting with an ATG in position 2146 and terminating with a TGA codon in position 2998; this region is interrupted by an intron starting in position 2464and terminating in position 2653. Three potential transcription initiation sites were determined by primer extension using the technique described in Sambrook et al. (op. cit., 1989); the most probable site is in position 2068. 
     The promoter region of the 246C gene upstream from position 2146 is called the 246C promoter. A study of the sequence of the 246C promoter shows the presence of several elements known to be involved in gene regulation. 
     Two consensus sequences CAAT corresponding to this element for regulating the transcription of eukaryotic genes, and a complementary and inverted sequence ATTG, are present in positions 2051, 2101 and 1967. 
     Two consensus sequences TATAA are present in positions 2089 and 2111 and a complementary sequence AATAT in position 2020. These three elements are all located between 10 and 50 base pairs downstream from the elements CAAT and 30 to 50 base pairs upstream from the potential transcription sites. 
     A sequence TGACG was identified in position 1950; this sequence, whose existence is demonstrated in the 35S promoter of CaMV, seems to be responsible for the expression of chimeric genes in the roots and leaves (LAM et al., 1989, Proc. Natl. Acad. Sci. USA, 86, 7890). 
     Three regions exhibit a considerable homogeneity with the HSEs (heat shock elements) of plants (GURLEY and KEY, 1991, Biochemistry, 30, 1). These regions are homologous with the consensus sequence GAANNGAANNTTCNNTTC or TTCNNTTCNNGAANNGAA; they are close to the TATA and CAAT boxes and duplicated  SEQ ID NO: 17 and NO: 18!. 
     A sequence homologous with the element CCGTCC characterized as being involved in the response to elicitors of fungal origin (LOIS et: al., 1989, EMBO J., 8, 1641) was located in position 1822. 
     Over about 30% of its length, the promoter of the 246C gene has a high homology (&gt;90%) over 700 base pairs with the plant promoter isolated from tobacco, having the sequence  SEQ ID NO: 8!, described by TAKAHASHI et al., 1990, Proc. Natl. Acad. Sci. USA, vol. 87, pp. 8013-8016. FIG. 2 represents the alignment of the DNA sequence of this promoter  SEQ ID NO: 9, 10 and 11! (top line) with the corresponding part of the DNA sequence of the promoter of the invention  SEQ ID NO: 12 and 13! (bottom line). 
     Section 9: Construction of expression vector pSG123 associating the promoter of the 246C gene with the β-glucuronidase gene 
     Starting from phasmid pKS246, digestion with the enzymes HindIII and BalI makes it possible to isolate an insert of about 2200 base pairs containing the promoter part of the 246C gene, the translation initiation codon and 11 codons coding for the aminoterminal part of the protein. 
     Plasmid pBI101.3 (Clontech) is digested with the enzymes HindIII and EcoRI; the fragment of about 2100 base pairs containing the gene of β-glucuronidase coded by the uidA locus of E. coli, followed by the nopaline synthase terminator of Agrobacterium tumefaciens, is ligated to plasmid pUC19, opened at the same sites, to give a plasmid called pBI201.3. 
     The HindIII-BalI insert carrying the promoter sequences of the 246C gene is cloned into plasmid pBI201.3, opened at the HindIII and SmaI sites. 
     The vector obtained, called pSG123, therefore contains the glucuronidase gene under the control of the promoter of the 246C gene. The nucleotide sequence of the complete chimeric gene is the sequence  SEQ ID NO: 14!. 
     Section 10: Protocol of the transient expression of the glucuronidase gene under the control of the promoter of the 246C gene in tobacco protoplasts 
     Preparation of tobacco protoplasts Leaves of 4- to 5-week-old tobacco plants (Nicotiana tabacum, var. Samsun NN) are removed, cut into thin strips and incubated in medium TO (Table 1, adapted from Chupeau et al., 1974, C. R. Acad. Sci. (Paris), 278 D, 1565) containing 1 g/liter of Onozuka cellulase R100, 200 mg/l of Onozuka macerozyme (Yakult Honsha, Nishinoniya, Japan) and 500 mg/l of pectolyase Y23 (Sheishin Pharmaceutical Ind., Japan), for 15 h at 22° C. 
     The protoplasts are separated from the cellular debris by sieving on a nylon sieve of 85 μm mesh, followed by centrifugation for 5 min at 50 g on a 19% (weight/volume) sucrose solution. The protoplasts floating on this medium are washed once in medium T0 and counted and their number is adjusted to a density of 1.5×106 protoplasts/ml. 
     Preparation of vector pSG123 
     The E. coli strain containing vector pSG123 is cultivated on Luria medium (Gibco) containing 50 mg/l of ampicillin. The plasmid is amplified according to the protocol described in Sambrook et al., 1989 (op. cit. ). Plasmid pSG123 is then purified by centrifugation on a cesium chloride gradient and by two successive precipitations with ethanol. The plasmid residue is then redissolved in 10 mM Tris-HCl buffer of pH 8.0. 
     Transformation with polyethylene glycol 
     The protoplast suspensions (320 μl per aliquot) are incubated at 45° C. for 5 min and then rapidly cooled on ice. 50 μg of plasmid pSG123 and 160 μl of a polyethylene glycol solution (40% polyethylene glycol, 0.4M mannitol, 30 mM MgCl 2 , 0.1% Mes pH 5.8) are then added. After 10 min, the protoplasts are collected by centrifugation, resuspended by gentle agitation in 500 μl of buffer TO and incubated in the dark at 28° C. 
     Measurement of the transient expression 
     After 24 h of incubation, 50 μl of β-glucuronidase 10× extraction buffer are added and the protoplasts are then lyzed by freezing at -80° C. followed by thawing at 37° C. (Jefferson, 1987, Plant Molec. Biol. Reporter, 5, 387). 
     The supernatant obtained after centrifugation at 10,000 g is used to measure the β-glucuronidase activity by fluorimetry (Jefferson, , 1987, Plant Molec. Biol. Reporter, 5, 387). 
     In parallel, the amount of proteins present in the extracts is measured by Bradford&#39;s method using the Bio Rad kit (Bio Rad Lab.). 
     
                       TABLE 1______________________________________Composition of medium T0 (per liter)______________________________________NH.sub.4 NO.sub.3         825    mgKNO.sub.3                 950    mgCaCl.sub.2.2H.sub.2 O     220    mgMgSO.sub.4.7H.sub.2 O     185    mgKH.sub.2 PO.sub.4         85     mgH.sub.3 BO.sub.3          1      mgMnSO.sub.4.4H.sub.2 O     100    μgZnSO.sub.4.7H.sub.2 O     1      mgKI                        100    μgAlCl.sub.3                30     μgNiCl.sub.2.6H.sub.2 O     30     μgCuSO.sub.4.5H.sub.2 O     30     μgFeSO.sub.4. 7H.sub.2 O    27.8   mgNa.sub.2 EDTA.2H.sub.2 O  37.2   mgThiamine                  100    μgNicotinic acid            200    μgPyridoxine                1      mgBiotin                    10     μgCa pantothenate           1      mgSucrose                   20     gInositol                  100    mgMannitol                  80     g2- N-Morpholino!ethanesulfonic acid (MES)                     200    mg______________________________________ pH adjusted to 5.8 before autoclaving 
    
     Section 11: Transient expression of the glucuronidase gene under the control of the promoter of the 246C gene in tobacco protoplasts infected with Pseudomonas solanacearum 
     This transient expression, determined according to the protocol of section 10, is measured after incubation for 24 h of the protoplasts prepared according to the above protocol in medium T0 (described in section 10) containing a suspension of Pseudomonas solanacearum bacteria (10 bacteria/protoplast) obtained as described in section 1. 
     The β-glucuronidase activity is expressed in pmol of methylumbelliferone formed/min/mg of protein. 
     No activity is detected in the protoplasts of plants which have not received DNA of vector pSG123. An activity of 450 pmol/min/mg of protein is measured on protoplasts treated with vector pBI221 (Clontech) containing the β-glucuronidase gene under the control of the 35S constitutive promoter of CaMV; this activity is reduced to 300 pmol/min/mg of protein after infection with Pseudomonas solanacearum strains GMI1000 and GMI1178. 
     An activity of 600 pmol/min/mg of protein is measured on protoplasts treated with plasmid pSG123; this activity is largely unmodified after inoculation with strain GMI1178; it increases to a value of 1000 pmol/min/mg of protein after inoculation with strain GMI1000. 
     The promoter of the 246C gene therefore permits a substantial base expression of the glucuronidase gene, said expression being more substantial than that governed by the 35S promoter of CaMV, which is used here as the control. This promoter further exhibits a strong inducibility since the expression of β-glucuronidase increases by 40% after infection with bacterial strain GMI1000. 
     Section 12: Transient expression of the glucuronidase gene under the control of the promoter of the 246C gene of tobacco protoplasts treated with an elicitor (chitin heptasaccharides) or a hormone 
     The expression is measured after incubation of the protoplasts for 24 h as described above in medium TO containing an elicitor at a concentration of 25 μM or a hormone, namely 2,4-D (2,4-dichlorophenoxyacetic acid), at a concentration of 4 μM. The elicitors used (glycosidic compounds derived from the wall of pathogenic fungi) are chitin heptasaccharides with the property of inducing defense reactions in plants (Roby et al., 1987, BBRC, 143, 885). 
     No activity is detected in untreated protoplasts used as the control. An activity of the order of 400 pmol of methylumbellifercone formed/min/mg of protein is measured on protoplasts which have received DNA of vector pBI221; this activity is not affected by the treatment (elicitors or hormone). 
     Protoplasts which have received DNA of vector pSG123 have an activity of 450 pmol/min/mg of protein; this activity is increased by 50% if the protoplasts are treated with the hormone 2,4-D and by 70% if the protoplasts are treated with chitin heptasaccharide. 
     The characteristics of this promoter which are demonstrated when protoplasts are infected with bacterial strain GMI1000 (high base level and inducibility) can be reproduced using an inducer derived from the wall of phytopathogenic fungi. 
     Section 13: Construction of an expression vector stable in plant cells: binary vector pSG246 
     Cleavage of vector pSG123 with the restriction endonucleases HindIII and EcoRI, followed by agarose gel electrophoresis, makes it possible to isolate the chimeric gene associating the 246C promoter with the coding part of β-glucuronidase and the NOS terminator. The chimeric gene is introduced into and ligated to binary vector pBIN19 (Clontech), previously opened at the HindIII and EcoRI sites, to give vector pSG246. This binary vector possesses two kanamycin resistance genes, the one being capable of expression in bacteria and the other, located immediately upstream from the complete recombinant gene (Bevan, 1984, Nucl. Ac. Res., 12, 8711), being capable of transfer to plant cells. The kanamycin resistance gene will serve as a selectable marker during the steps involving transformation and analysis of the lineage of the transformed plants. 
     The vector obtained, called pSG246, is cloned into E. coli strain DH5α. 
     Section 14: Transfer to Agrobacterium of plasmid pSG246 containing β-glucuronidase under the control of the promoter of the tobacco 246C gene 
     a) Transfer to Agrobacterium tumefaciens 
     This transfer is effected by transformation using the freeze-thaw method described in Plant Molecular Biology Manual (Gelvin et al., eds., Kluwer Academic Publishers, 1988) and is summarized below. 
     Competent cells of Agrobacterium tumefaciens (strain LBA4404, Clontech) are prepared by the rapid ice-cooling of a culture in the exponential growth phase. The bacteria are then resuspended in 20 mM CaCl 2 . Aliquots of this suspension are distributed into Eppendorf tubes and then frozen in liquid nitrogen. 
     1 μg of plasmid pSG246 is added to the frozen cells contained in an Eppendorf tube. The suspension is then incubated at 37° C. for 5 min; 1 ml of Luria medium (Gibco) is then added and the tube is incubated at 28° C. for 4 h. Aliquots are plated out on Petri dishes containing a minimum agar medium described in Plant Molecular Biology Manual (op. cit.), in the presence of 100 mg of rifampicin and 25 mg/l of kanamycin. Under these conditions, only the Agrobacterium tumefaciens colonies which have integrated plasmid pSG246 grow. Said colonies contain the chimeric gene in a context which allows its replication. 
     The resistance of the selected colonies to the two antibiotics is verified by subculturing said colonies on the same selection medium twice in succession. The presence of the chimeric gene associating, the 246C promoter with the coding part of β-glucuronidase in Agrobacterium tumefaciens is verified by the Southern blotting method on a total DNA preparation (lysis of the cells, purification of the DNA by extraction with a phenol/chloroform mixture according to the protocol described by Gelvin in the work cited above, cleavage of the purified DNA with restriction enzymes, agarose gel electrophoresis, membrane transfer and hybridization by the techniques well known to those skilled in the art). 
     b) Transfer to Agrobacterium rhizogenes 
     This transfer is effected in the same manner as the transfer to Agrobacterium tumefaciens described in a), with Agrobacterium rhizogenes strain A4 described by Guerche et al., (1987) Mol. Gen. Genet., 206, 382. 
     Section 15: Production of tobacco plants transformed with Agrobacterium tumefaciens containing plasmid pSG246 
     Tobacco, Nicotiana tabacum, cultivated in vitro, was infected with Agrobacterium tumefaciens containing plasmid pSG246 according to the procedure of Horsch et al., which is well known to those skilled in the art (Horsch R. B. et al., 1985, Science, 227, 1229-1231) and the principal steps of which are described below. 
     Leaf disks from axenic tobacco plants, Nicotiana tabacum (Bottom Special variety), are incubated in a culture of A. tumefaciens containing plasmid pSG246. The disks, drained on Whatman paper, are transferred to culture media in Petri dishes for multiplication of the transformed cells to give calli (Murashige and Skoog, 1962, Physiol. Plant, 15, 473) and then to produce buds in the presence of cefotaxim (500 μg/ml), which is intended to eliminate Agrobacterium tumefaciens, and in the presence of kanamycin (100 μg/ml). 
     In parallel, transformations were carried out with Agrobacterium tumefaciens strains LBA4404 containing the following vectors: 
     pBI101 (Clontech), which consists of the coding part of glucuronidase preceding the nopaline synthase terminator in binary vector pBIN19. This construction, hereafter called construction pBI101, is devoid of a promoter. 
     pBI221 (Clontech), which consists of a fragment of 800 base pairs of the 35S promoter of the cauliflower mosaic virus, inserted in front of the coding part of glucuronidase in vector pBI101. This construction will hereafter be called construction pBI221. 
     The kanamycin-resistant buds were then transferred to a medium for the induction of roots in the presence of carbenicillin and kanamycin. The plantlets are then potted up into a substrate composed of peat and vegetable mold and are grown on in a greenhouse. All the transformed plants (R0 generation) which have survived the steps of regeneration and greenhouse acclimatization were found to be morphologically normal and fertile. They were self-fertilized and gave seeds (R1 generation). 
     Section 16: Analysis of the genomic DNA of tobacco plants transformed with Agrobacterium tumefaciens containing plasmid pSG246 (R0 generation) by the Southern blotting technique 
     The high-molecular tobacco genomic DNA was isolated from mature leaves of transgenic plants of the R0 generation by the method involving extraction with cetyltrimethylammonium bromide and purification by precipitation, described in the work &#34;Plant Molecular Biology Manual&#34; cited above. 
     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 electrophoresis on agarose gel (1%). The DNA was transferred to a nylon filter (Hybond N + , Amersham) by the Southern blotting method and hybridized with a nucleotide probe comprising part of the sequence of the recombinant gene, Labeled by coupling with peroxidase (ECL kit, Amersham). The membranes are then washed and developed according to the protocol recommended by Amersham. 
     Analysis of the films affords the following conclusions: 
     some plants do not possess copies of the transferred recombinant gene (absence of signal). 
     most of the plants tested contain at least one copy without rearrangement of the construction: 246C promoter/coding sequence of β-glucuronidase/NOS terminator, hereafter called construction pSG246. 
     some profiles suggest that internal rearrangements exist in this construction, but these events are rare. 
     Section 17: Study of the activation characteristics of the 246C promoter in transgenic tobacco plants 
     This study was performed on plants of the R1 generation which had previously been selected in vitro on Murashige and Skoog&#39;s agar medium containing 500 μg/ml of kanamycin. 
     10 plants per transformant lineage, selected for their kanamycin resistance, are pricked out into vegetable mold and then cultivated for 4 to 5 weeks in a culture chamber. 
     a) Activation by the phytopathogenic bacterium Pseudomonas solanacearum 
     Inoculation by infiltration 
     Inoculation tests are conducted according to the protocol described in section 1 on four leaves belonging to 2 different plants. The measurements of glucuronidase activity were made according to the method described by Jefferson (Plant Molecular Biology Reporter, 5, 387, 1987) using 4-methylumbelliferyl β-D-glucuronide as the substrate. 
     The results show that: 
     the plants containing construction pBI101 have no detectable glucuronidase activity. 
     the plants containing construction pBI121 have a glucuronidase activity of between 5000 and 70,000 pmol of methylumbelliferone/min/mg of protein, corresponding to an expected constitutive expression for this construction. A slight activation of this promoter in response to the stress of infiltration was found for some transformants. 
     the plants containing construction pSG246 have a low glucuronidase activity, in the non-inoculated plants, of between 2000 and 5000 pmol/mg of protein. A strong induction is measured in response to the bacterial infection, irrespective of the bacterial strain used (GMI1000 or K60 (Sequeira et al., Physiol. Plant Pathol., 10, 43, 1977), (compatible strain which causes symptoms). The induction factor (ratio of the activity measured after inoculation to the activity measured before inoculation) is of the order of 20 and the activity values sometimes exceed those obtained with the plants expressing construction pBI121. 
     Localized bacterial infection 
     A localized bacterial infection is produced by depositing a drop of a bacterial suspension of Pseudomonas solanacearum (3 μl containing 3×10 5  bacteria obtained as described in section 1) onto a wound obtained by perforating a leaf with a syringe needle. 
     The 246C promoter is activated around the lesion created by the infection and also in all parts of the infected plant (inoculated leaf, upper leaves and lower leaves of the plant, and roots). This systemic activation takes place as from the first few hours after inoculation. 
     No activation was observed in plants of the R1 generation derived from plants transformed with constructions pBI101 and pBI121. 
     The same type of localized infection produced in the roots of tobacco plants cultivated in vitro again results in a strong activation of the promoter at the inoculation site, but also throughout the root and in the aerial part of the plant. 
     b) Activation by the pathogenic fungus Chalara elegans 
     In vitro study 
     10 to 15 ml of Murashige and Skoog&#39;s liquid medium are poured into a Petri dish containing a 3-week culture of Chalara elegans in the process of sporulation (culture on PDA (potato dextrose agar) medium, Difco). 
     The spores can be collected by scratching the surface of the culture. After counting, appropriate dilution makes it possible to obtain suspensions of 10 4  and 10 5  spores per ml. 
     7 ml aliquots are distributed into Magenta dishes (Sigma). A transgenic tobacco plant (about 3 weeks old and cultivated in a sterile medium), transformed with the β-glucuronidase gene under the control of the 246C promoter, is introduced into each dish, their roots dipping into the spore suspension. The plants are then removed and frozen and the glucuronidase activity is determined. At the time of infection, the specific activity is 20,000 pmol of methylumbelliferone per mg of protein. Compared with non-inoculated references placed under the same conditions, this activity is increased by factors of 8 and 8.5 for infections with 10 4  and 10 5  spores per ml, respectively, as from 4 days after inoculation. 
     Greenhouse study 
     10 plants per transformant: lineage, selected for their kanamycin resistance, are pricked out into 3×3 cm pots. When the 5th leaf appears, the plants are inoculated by depositing a suspension of 5×10 5  endoconidia of Chalara elegans onto the neck. 
     c) Activation by the pathogenic fungus Sclerotinia sclerotiorum 
     Study on leaf disks 
     Leaf disks 20 mm in diameter, originating from plants expressing construction pSG246, are placed on an appropriate liquid survival medium. A cube of agar with a side length of about 5 mm, containing mycelium of Sclerotinia sclerotiorum, is placed on each of these disks. The glucuronidase activity, measured as a function of time, shows that the presence of mycelium induces the glucuronidase activity after 7 hours of contact. After 24 hours, the activity is increased by a factor of 4 compared with that of leaf disks not brought into contact with the mycelium. The same experiment carried out on leaf disks derived from reference tobaccos (not expressing construction pSG246) shows only a glucuronidase activity comparable to the background. 
     d) Activation by elicitors 
     Two types of elicitors were used, the one a biotic type corresponding to molecules derived from natural molecules or macromolecules, and the other an abiotic type corresponding to chemical molecules. 
     d1. Biotic elicitors of bacterial or fungal origin 
     The elicitors used are harpin, which is a protein isolated from Erwinia amylovora, and a protein isolated from Pseudomonas solanacearum culture supernatant. Protein elicitors such as cryptogeine isolated from Pseudomonas cryptogea and capsiceine isolated from Pseudomonas capsici (Ricci et al., 1989, Eur. J. Biochem., 183, 555-563) were similarly tested. 
     Using a syringe, appropriate concentrations of elicitors were infiltrated in all cases under the lower epidermis of tobacco leaves expressing construction pSG246. The induction of activity is induced in all cases by the presence of an elicitor in an approximately 5 mm ring immediately adjacent to the infiltration zone. The stimulation is very apparent 24 hours after infiltration but is visible after only 6 hours. The activity after 24 hours is often 5 to 6 times those of the reference plants (plants expressing construction pSG246 but without elicitors injected under the epidermis). 
     d2. Abiotic elicitors: salicylic acid, copper sulfate 
     Tobacco leaves expressing construction pSG246, which have been detached from the plant, are immersed in solutions with a salicylic acid concentration of 1 to 10 μg/ml or a copper sulfate concentration of 0.025 to 0.25 mM. 
     In the presence of salicylic acid, the glucuronidase activity is increased by a factor of 5 after 6 hours and 10 after 24 hours. In the case of copper sulfate, the glucuronidase activity is increased by a factor of 17 at 0.025 mM and 11 at 0.25 mM when compared with leaves of untreated reference plants. 
     d3. Induction by growth regulators 
     The application of an auxin in the form of 2,4-dichlorophenoxyacetic acid (2,4-D) was effected at concentrations of 1.5 and 10 μM. The application, effected by the immersion of petioles of detached tobacco leaves expressing construction pSG246, shows that induction in the leaf starts 6 hours after the application of auxin at a concentration of 5 μM and is stimulated 18-fold after 12 hours, compared with the leaves of reference plants not treated with auxin. 
     The glucuronidase activity is measured when the symptoms of the disease appear, i.e. about 15 days after inoculation. 
     The results of the activity measured on the aerial part of the whole plant show that: 
     the plants containing construction pBI101 have no detectable glucuronidase activity. 
     the plants transformed with construction pBI121 have an activity of 12,000 to 60,000 pmol of methylumbelliferone/min/mg of protein. This activity varies little after inoculation. 
     the plants transformed with construction pSG246 have a low glucuronidase activity in the healthy plants. This activity increases considerably in the plants which display symptoms, reaching values of 85,000 pmol of methylumbelliferone formed/min/mg of protein. 
     e) Activation by a wound 
     This activation was investigated on leaves of about 5-week-old plants of the R1 generation containing construction pSG246, previously selected for their kanamycin resistance. 
     The simple excision of a leaf causes a slow and weak activation of the promoter, both in the leaf and in the plant; however, the laceration of a leaf causes a very large (5-fold) and extremely rapid (30 min) increase in the glucuronidase activity of the lacerated leaf. 
     f) Heat-shock activation 
     About 5-week-old tobacco plants of the R1generation containing construction pSG246, previously selected for their kanamycin resistance, are transferred for 2 or 4 h to an enclosure at 40° C. in order to cause a heat shock. When the treatment has ended, the plants are immediately frozen in liquid nitrogen and their β-glucuronidase activity is determined on the whole of the aerial part. 
     The same protocol is applied to plants transformed with construction pBI121; the activity of these plants is not modified by heat shock. 
     By contrast, the plants containing construction pSG246 exhibit a large increase in glucuronidase activity after heat shock; the mean stimulation factor, determined on several plants, is of the order of 12. 
     g) Expression during development, and spatial distribution of the expression in the plant 
     The localization of the activity in the plant tissues can be visualized by using the histochemical substrate cyclohexylammonium 5-bromo-4-chloroindol-3-yl-β-D-glucuronide (X-gluc) for disclosing glucuronidase activity, according to the method described by Jefferson (Plant Molecular Biology Reporter, 5, 387, 1987). 
     Germination of the seeds 
     During the germination of tobacco seeds of the R1 generation expressing glucuronidase under the control of the 246C promoter, the expression is not detectable in the cotyledons, strong throughout the root and very strong in the root and cauline meristems. In the developed plant, the detection of glucuronidase activity was recorded in all the tissues tested, including the dry seed. 
     Section 18: Production of colza plants transformed with Agrobacterium rhizogenes containing plasmid pSG246 
     The transformation is effected according to the protocol of P. Guerche et al. (P. Guerche et al., 1987, Mol. Gen. Genet., 206, 382). The different culture media are those described by Pelletier et al. (Pelletier et al., 1983, Mol. Gen. Genet., 191, 244). Their composition will be given in detail below (Table 2). 
     a) Production of transformed roots 
     Stem segments are taken from the apical end of colza plants (Brassica napus: Brutor and Westar spring varieties and winter variety) about 1 m in height. These segments are sterilized on the surface, rinsed in sterile water, cut into segments of about 1.5 cm in length and placed in a tube containing medium A. 
     The end of this segment is inoculated by depositing a suspension of the Agrobacterium rhizogenes strain containing plasmid pSG246. 
     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 complemented with 500 μg of cefotaxim/ml. 
     b) Regeneration of transformed plants 
     Root fragments are incubated for 15 days in medium D containing 3 mg/l of 2,4-dichlorophenoxyacetic acid and are then placed on medium RCC for inducing buds. Rooted plants are then obtained by transferring the buds to media F and G. 
     
                       TABLE 2______________________________________Composition of the different media used for the production oftransformed colza plantsComposition    Medium(mg/l)   A       B       RCC   F     G     D______________________________________NH.sub.4 NO.sub.3    1650            1650  1650  825   200KNO.sub.3    1900    2500    1900  1900  950   1250(NH.sub.4).sub.2 SO.sub.4            134                       67NaH.sub.2 PO.sub.4            150                       75KH.sub.2 PO.sub.4    170             170   170   85    5CaCl.sub.2.2H.sub.2 O    440     750     440   440   220   525MgSO.sub.4.7H.sub.2 O    370     250     370   370   185   250H.sub.3 BO.sub.3    12.4    3       12.4  6.2   6.2   12.4MnSO.sub.4.4H.sub.2 O    33.6    10      33.6  22.3  22.3  33.6ZnSO.sub.4.7H.sub.2 O    21      2       21    8.6   8.6   21KI       1.66    0.75    1.66  0.83  0.83  1.66Na.sub.2 MoO.sub.4.    0.5     0.25    0.5   0.25  0.25  0.52H.sub.2 OCuSO.sub.4.5H.sub.2 O    0.05    0.025   0.05  0.25  0.25  0.05CoCl.sub.2.6H.sub.2 O    0.05    0.025   0.05  0.25  0.25  0.05FeSO.sub.4.7H.sub.2 O    22.4    27.8    27.8  27.8  22.24 27.8Na.sub.2 EDTA    29.84   37.3    37.3  37.3  29.84 37.3Inositol 100     100     100   100   100   100Nicotinic acid    0.5     1       0.5   1     0.5   1Pyridoxine.HCl    0.5     1       0.5   1     0.5   1Thiamine         10            10          10Glycine  2               2           2Glucose  10,000  20,000              10,000Sucrose  10,000          10,000                          10,000      20,000D-Mannitol       70,000  10,000NAA              1       1     0.1   0.1BA               1       0.5   0.52,4-D            0.25                      1Adenine sulfate                            30IPA                                        30GA                             0.02Tween 80         10Agar     8000            8000  8000  8000pH       5.8     5.8     5.8   5.8   5.8   5.8Gentamycin    10(sulfate)______________________________________ NAA: naphthaleneacetic acid BA: 6benzylaminopurine 2,4D: 2,4dichlorophenoxyacetic acid IPA: N.sup.6(2-isopentyl)adenine GA.sub.3 : gibberellic acid EDTA: ethylenediaminetetraacetic acid 
    
     Section 19: Characteristics of the expression of the glucuronidase gene under the control of the 246C promoter in colza plants 
     a) Activation by a wound 
     The leaves of colza plants of the R1 generation containing glucuronidase under the control of the 246C promoter were excised or excised and lacerated. 
     A weak activation of glucuronidase activity is observed in the excised leaves; a very strong (6 times the base activity) and extremely rapid (about 30 min) activation results from laceration. 
     b) Infection with phytopathogenic fungi 
     Leaf parasite (Alternaria brassicae): 
     Colza plants of the R1 generation possessing construction pSG246 are cultivated in vegetable mold for about 3 weeks in pots. The plants are then inoculated locally with a suspension of spores (10 ml containing 1000 spores obtained after culture on PDA medium) of the pathogenic fungus Alternaria brassicae, deposited on a wound made with a needle. Necrosis then develops around this wound. 
     A strong stimulation of the glucuronidase activity (detected by testing with X-gluc, section 17e) is then observed in the inoculated leaf, around the necrotic zone. 
     Root parasite (Rhizoctonia solani): 
     Colza seeds of the R1 generation, transformed with construction pSG246, are sown on a substrate consisting of a mixture of peat, vermiculite and sand (10:10:5, v:v), contained in a 1 liter pot. The seeds are covered with a 1 cm layer of substrate containing 10,000 viable propagules of Rhizoctonia solani per gram. These propagules are obtained by culturing a Rhizoctonia strain in a Roux flask on grains of rice for 15 days and then grinding it to a particle size of less than 1 mm. 
     During their development, the colza plants are attacked at the roots. 
     A strong stimulation of the glucuronidase activity (detected by testing with X-gluc&#39;, section 17e) is observed in the roots of infected plants, compared with the activity measured in the roots of control plants (same R1 lineage of transformed but not infected plants). Furthermore, a strong stimulation of the glucuronidase activity is induced systemically in the aerial parts. 
     c) Heat-shock activation of colza plants of the R1 generation 
     About 5-week-old colza plants of the R1 generation containing construction pSG246 are transferred for 2 or 4 h to an enclosure at 40° C. in order to cause a heat shock. When the treatment has ended, the plants are immediately frozen in liquid nitrogen and their β-glucuronidase activity is determined on the whole of the aerial part. 
     The same protocol is applied to plants transformed with construction pBI121; the activity of the latter plants is not affected by heat shock. 
     By contrast, the plants containing construction pSG246 exhibit a large increase in glucuronidase activity following heat shock; the mean stimulation factor, determined on several plants, is of the order of 12. 
     d) Expression during development 
     During the germination of colza seeds of the R1 generation containing glucuronidase under the control of the 246C promoter, an expression of this protein is observed in the cotyledons, a strong expression throughout the root and a very strong expression in the root and cauline meristems. 
     A very strong expression was also measured in the transformed roots and calli during the steps involving the regeneration of transgenic plants, as well as in the various parts of the plant (including the mature seeds). 
     Section 20: Production of sunflower calli transformed with Agrobacterium rhizogenes containing plasmid pSG246 
     The transformation is effected according to the protocol of Guerche et al. (Mol. Gen. Genet., 206, 382, 1987), which was initially developed for the transformation of colza. The different culture media are those described by Pelletier et al. (Mol. Gen. Genet., 191, 244, 1983); their composition has been described in detail (Table 2). 
     Sunflower hypocotyls are obtained by germinating seeds on vermiculite for 7 to 10 days. These seeds are placed in a culture clamber, the conditions being 16 h of illumination at 20° C./8 h of darkness at 17° C. The hypocotyls are sterilized on the surface, rinsed in sterile water and placed in a tube containing Murashige and Skoog&#39;s medium in which the concentration of macroelements has been reduced by half. 
     The end of this segment is inoculated by depositing a suspension of the Agrobacterium rhizogenes strain containing plasmid pSG246. 
     Transformed roots appear after one month; they are removed and placed on medium B containing agar (15 g/l) and complemented with 500 μg of cefotaxim/ml, for 4 weeks with weekly subculture. They are then cultivated in the same liquid medium, with agitation (100 rpm), and subcultured every month. Transfer of these roots to medium D enables calli to form from the transformed roots. 
     The glucuronidase activity of the roots cultivated in liquid medium B and calli cultivated on medium D, estimated by fluorimetry, has very high values of between 10 4  and 10 5  pmol of methylumbelliferone formed/min/mg of proteins. 
     Section 21: Transient expression of the glucuronidase gene under the control of the promoter of the 246C gene in immature sunflower embryos 
     The immature embryos of field mother plants of genotypc 105 were removed and cultured for 14 days on medium I (Table 3) at 25° C. in the dark. These embryos are then cultivated for 3 days on medium II at 25° C. under a photoperiod of 16 hours per day/8 hours per night. About twenty embryos, are then deposited side-by-side on medium III. 
     Preparation of vector pSG123: 
     This is carried out according to the protocol described in section 10. 
     Transformation of the plant material: 
     The plasmid DNA (vector pSG123) is introduced into the plant cells by using the particle gun constructed according to the principle described by Zumbrunn (Zumbrunn et al., 1989, Technique, 1(3), 204-216). The plasmid DNA is adsorbed onto tungsten microparticles at a rate of 4 μg/mg of tungsten. 2.5 mg of the tungsten/DNA mixture are then deposited onto a macroprojectile, which is accelerated by the explosion of a cartridge. 
     The break-up of the macroprojectile on a stop plate containing a hole enables the tungsten microparticles and the DNA to be projected into the cells. 
     Measurement of the transient expression: 
     The DNA adsorbed on the tungsten microparticles which have penetrated the plant cells is released; the chimeric gene associating the promoter of the 246C gene with the glucuronidase is then transcribed and subsequently translated. The glucuron: Ldase obtained is then visualized by the histochemical test described by JEFFERSON et al., 1987, Plant Molecular Biology Reporter, 5, 387, using the substrate cyclohexylammonium 5-bromo-4-chloroindol-3-yl-β-D-glucuronide (X-gluc). The cells expressing the gene then give a blue coloration. 
     Counting of the number of blue cells obtained per Petri dish during a transient expression experiment makes it possible to count the number of transformed cells and to estimate the expression of the chimeric construction tested. 
     The transient expression, measured using the substrate X-gluc 48 hours after bombardment with the microparticle gun, shows that the β-glucuronidase gene is expressed in the immature sunflower embryos. 
     The intensity is greater than that induced by using plasmid pBI221 (Clontech), in which the glucuronidase gene is placed under the control of the 35S promoter of the cauliflower mosaic virus. 
     The number of transformed cells expressing the glucuronidase gene under the control of the promoter of the 246C gene is of the order of 140 per dish (mean value over 4 experiments), whereas the number of transformed cells is 60 per dish (mean value over 4 experiments) in the presence of plasmid pBI221, in which the glucuronidase gene is placed under the control of the 35S promoter of the cauliflower mosaic virus. 
     The embryos are then drained on sterile filter paper and subsequently re-cultured on medium II in the dark for 3 days. The embryos are then briefly rinsed with Murashige and Skoog&#39;s liquid medium (Murashige and Skoog, 1962, Physiol. Plant, 15, 473) containing 500 mg/l of the antibiotic cefotaxim. They are then drained on sterile filter paper and cultured on medium III containing 250 mg/l of cefotaxim, 250 mg/l of carbenicillin and 50 mg/l of paromomycin. This culture is effected at 25° C. under a photoperiod of 16 h day/8 h night; the plant tissues are subcultured every 21 days on this same medium. 
     The buds newly formed from these tissues are transferred to medium IV under the same temperature and photoperiod conditions. The rooted plants are then grown on in a greenhouse. 
     Section 22: Expression of β-glucuronidase under the control of the 246C promoter in transformed sunflower plants 
     The plants expressing construction pSG246 have a glucuronidase expression which is at least equal to that obtained with plants transformed with construction pBI121. 
     
                       TABLE 3______________________________________Composition of the different media used for the production oftransformed sunflower plantsMedium           I       II      III   IV______________________________________KNO.sub.3        2500    2500    1900  1900NH.sub.4 NO.sub.3            --      --      1650  1650CaCl.sub.2.2H.sub.2 O            150     150     440   440MgSO.sub.4.7H.sub.2 O            250     250     370   370KH.sub.2 PO.sub.4            --      --      170   170(NH.sub.4).sub.2 SO.sub.4            134     134     --    --NaH.sub.2 PO.sub.4.H.sub.2 O            150     150     --    --ZnSO.sub.4.7H.sub.2 O            2       2       8.6   8.6H.sub.3 BO.sub.3 3       3       6.2   6.2KI               0.75    0.75    0.83  0.83CuSO.sub.4.5H.sub.2 O            0.025   0.025   0.025 0.025Na.sub.2 MoO.sub.4.2H.sub.2 O            0.25    0.25    0..25 0.25CoCl.sub.2.6H.sub.2 O            0.025   0.025   0.025 0.025MnSO.sub.4.4H.sub.2 O            10      10      22.3  22.3Na.sub.2 EDTA    37.3    37.3    37.3  37.3FeSO.sub.4.7H.sub.2 O            27.8    27.8    27.8  27.8Nicotinic acid   1       1       0.5   0.5Thiamine.HCl     10      10      0.1   0.1Pyridoxine.HCl   1       1       0.1   0.5Myoinositol      4000    4000    100   100L-Glycine        --      --      --    2L-Alanine        1000    1000    --    --L-Glutamine      800     800     --    --L-Serine         160     160     --    --L-Tryptophan     50      50      --    --L-Cysteine       10      10      --    --Ca D-pantothenate            --      --      0.8   --Folic acid       --      --      0.1   --Choline chloride --      --      0.1   --p-Aminobenzoic acid            --      --      0.05  --Riboflavine      --      --      0.05  --Sucrose          120,000 60,000  30,000                                  30,0002,4-Dichlorophenoxyacetic acid            2       --      --    --6-Benzylaminopurine            --      0.4     --    --Kinetin          --      --      1     --Indolacetic acid --      --      --    0.05Agar             7000    7000    7000  8000pH               5.7     5.8     5.7   5.7______________________________________ 
    
     Section 23: Protocol of the expression of the β-glucuronidase gene under the control of the 246C promoter in monocotyledon tissues 
     Production of the plant material: 
     Seeds of the GERBEL barley genotype are germinated on vermiculite in a greenhouse. After 7 days, the leaves and roots were removed and placed on a Petri dish containing Murashige and Skoog&#39;s agar medium for the transient expression experiments. 
     Immature maize embryos are removed, 10 to 14 days after pollination, from stools (line LH132) cultivated in a greenhouse. The embryos are placed with their embryonic axis in contact with the induction medium (composition given in Table 4 below) and then, 3 weeks later, on the maintenance medium (Table 5). The calli obtained are subcultured every week. The transient expression experiments are performed a few hours after subculture. 
     Preparation of vector pSG123: 
     This is carried out according to the protocol described in section 10. 
     Transformation of the plant material: 
     The plasmid DNA (vector pSG123) is introduced into the plant cells by using the particle gun constructed according to the principle described by Zumbrunn (Zumbrunn et al., 1989, Technique, 1(3), 204-216). The plasmid DNA is adsorbed onto tungsten microparticles at a rate of 4 μg/mg of tungsten. 2.5 mg of the tungsten/DNA mixture are then deposited onto a macroprojectile, which is accelerated by the explosion of a cartridge. 
     The break-up of the macroprojectile on a stop plate containing a hole enables the tungsten microparticles and the DNA to be projected into the cells. 
     Measurement of the transient expression: 
     The DNA adsorbed on the tungsten microparticles which have penetrated the plant cells is released; the chimeric gene associating the promoter of the 246C gene with the glucuronidase is then transcribed and subsequently translated. The glucuronidase obtained is then visualized by the histochemical test described by JEFFERSON et al., 1987, Plant Molecular Biology Reporter, 5, 387, using the substrate cyclohexylammonium 5-bromo-4-chloroindol-3-yl-β-D-glucuronide (X-gluc). The cells expressing the gene then give a blue coloration. 
     Counting of the number of blue cells obtained per Petri dish during a transient expression experiment makes it possible to count the number of transformed cells and to estimate the expression of the chimeric construction tested. 
     
                       TABLE 4______________________________________Medium for inducing maize calli from immatureembryos (in mg per liter)______________________________________MgSo.sub.4.7H.sub.2 O     370CaCl.sub.2.2H.sub.2 O     440KNO.sub.3                 1900NH.sub.3 NO.sub.3         1650KH.sub.2 PO.sub.4         170Na.sub.2 MoO.sub.4.2H.sub.2 O                     0.25CuSO.sub.4.5H.sub.2 O     0.025MnSO.sub.4.H.sub.2 O      16.75H.sub.3 BO.sub.3          6.2ZnSO.sub.4.7H.sub.2 O     8.6KI                        0.83CoCl.sub.2.6H.sub.2 O     0.025FeEDTA                    65.1Sucrose                   20,000Casein hydrolyzate        100L-Proline                 5800Glycine                   2Nicotinic acid            0.5Pyridoxine.HCl            0.5Inositol                  100Thiamine.HCl              0.1Abscisic acid             0.06Chloramben                4.12Phytagel                  3000______________________________________ pH = 5.7; autoclaving for 20 min at 12° C. 
    
     
                       TABLE 5______________________________________Medium for maintaining waize calli (in mg per liter)______________________________________MgSo.sub.4.7H.sub.2 O     370CaCl.sub.2.2H.sub.2 O     440KNO.sub.3                 1900NH.sub.3 NO.sub.3         1650KH.sub.2 PO.sub.4         170Na.sub.2 MoO.sub.4.2H.sub.2 O                     0.25CuSO.sub.4.5H.sub.2 O     0.025MnSO.sub.4.H.sub.2 O      16.75H.sub.3 BO.sub.3          6.2ZnSO.sub.4.7H.sub.2 O     8.6KI                        0.83CoCl.sub.2.6H.sub.2 O     0.025FeEDTA                    65.1Sucrose                   20,000Casein hydrolyzate        100L-Proline                 2900Glycine                   2Nicotinic acid            0.5Pyridoxine.HCl            0.5Inositol                  100Thiamine.HCl              0.1Dicamba (Banvel ®)    0.002Gelrite                   3000______________________________________ pH = 5.7; autoclaving for 20 min at 120° C. 
    
     Section 24: Transient expression of the β-glucuronidase gene under the control of the promoter of the 246C gene in barley tissues and maize calli 
     The transient expression, measured using the substrate X-gluc 48 hours after bombardment with the microparticle gun, shows that the β-glucuronidase gene is expressed in barley leaves and roots and also in maize calli. 
     The intensity of the expression is as great as that induced by using plasmid pBI221 (Clontech), in which the glucuronidase gene is placed under the control of the 35S promoter of the cauliflower mosaic virus. 
     The promoter of the tobacco 246C gene is therefore capable of directing the expression of a gene in monocotyledons. 
     Section 25: Construction of a plasmid placing the tomato-tobacco chitinase gene under the control of the inducible promoter, and expression thereof in tobacco 
     a) Preparation of the promoter sequence Plasmid pSG123, described above, is digested with the endonucleases HindIII and ScaI. After agarose gel electrophoresis, the HindIII-ScaI fragment of 2088 base pairs, containing the whole of the inducible promoter except for the 57 base pairs; located immediately upstream from the ATG, is purified 
     Ligation of this purified fragment, the synthetic ScaI-BamHI oligonucleotide of 62 base pairs of the sequence  SEQ ID NO: 15! and a vector pTZ19R (Pharmacia), linearized with the endonucleases HindIII and BamHI, produced plasmid pPH111. 
     The HindIII-BamHI fragment of 2150 base pairs, containing the inducible promoter in its entirety, is isolated from this plasmid pPH111 by cleavage with the endonucleases HindIII and BamHI, followed by agarose gel electrophoresis. 
     b) Preparation of the fragment carrying a hybrid gene coding for a protein with endochitinase activity 
     The BamHI-EcoRI fragment originating from plasmid pBR1 described in patent application EP-493 581, Example 1, and containing a chimeric gene coding for a protein with endochitinase activity  SEQ ID NO: 16!, which comprises the sequence coding for a tomato-tobacco hybrid endochitinase (in position 438-1587) and the NOS terminator, is purified. 
     c) Cloning into binary vector pBIN19 T4 DNA ligase was used to ligate the promoter sequence (cf. above), the sequence coding for chitinase and the terminator sequence to binary vector pBIN19 (Bevan, 1984, Nucl. Acids Res., 12, 8711-8721), opened with the endonucleases HindIII and EcoRI. This vector carries two kanamycin resistance genes, the one being capable of expression in bacteria and the other, located immediately upstream from the complete recombinant gene, being capable of transfer to plant cells. 
     The vector obtained, called pBR20, is cloned into E. coli strain HB101 (Clontech). 
     2) Transformation of Agrobacterium tumefaciens 
     The transformation of Agrobacterium tumefaciens strain LBA4404 (Clontech) is effected by the freeze-thaw method described in Plant Molecular Biology Manual (Gelvin et al., op. cit.) (summarized in section 14), starting from 1 mg of plasmid pBR20. 
     3) Transformation of tobacco 
     Tobacco, Nicotiana tabacum, cultivated in vitro, was infected with Agrobacterium tumefaciens containing plasmid pBR20 according to the procedure of Horsch et al., which is well known to those skilled in the art (Horsch R. B. et al., 1985, Science, 227, 1229-1231) and the principal steps of which are explained below. 
     Leaf disks from axenic tobacco plants, Nicotiana tabacum (Wisconsin Havana 38 variety), are incubated in a culture of A. tumefaciens containing plasmid pBR20. The disks, drained on Whatman paper, are cultured on culture media in Petri dishes for multiplication of the transformed cells to give calli. These calli are then transferred to a medium containing 500 mg/ml of cefotaxim for decontaminating the plant tissues (elimination of the Agrobacterium tumefaciens) and 100 mg/ml of kanamycin for selecting the transgenic material. 
     Demonstration of the expression of the protein with endochitinase activity in transgenic tobaccos 
     a) Preparation of the crude protein extracts from transformed tobacco 
     The crude protein extracts were prepared from different plant tissues (root, stem, leaf, etc.). 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 of pH 5.2 and centrifuged at 10,000 g. The concentration of total proteins was determined on the supernatants, hereafter called the crude protein extracts, by Bradford&#39;s technique (Bradford, M. M., 1976, Anal. Biochem., 72, 248-254). 
     b) Demonstration of the existence of the hybrid chitinase by immunoblotting (Western blotting) 
     The crude protein extracts are subjected to Western blotting, a technique well known to those skilled in the art and described by H. Towbin et al. (Proc. Ntl. Acad. Sci. USA, 76, 1979, 4350-4354). 
     The immunodetection of the protein of interest is effected by means of an immune serum containing polyclonal antibodies recognizing the hybrid protein with chitinase activity (cf. EP-493 581, section 5). 
     The antigen-antibody complex is then revealed by means of a streptavidin-biotin system conjugated with alkaline phosphatase, using the RPN23 kit from Amersham (blotting detection kit) in accordance with the manufacturer&#39;s instructions. 
     The blot obtained shows, for the leaves of tobacco plants transformed with plasmid pBR20, the presence of a protein with an apparent molecular weight of about 26±6 kDa, which is recognized by the polyclonal antibodies and is absent from the leaves of the reference tobacco plants. This protein has the same apparent molecular weight as the hybrid protein with chitinase activity described in patent application EP-493 581. 
     Section 26: Localization of the minimum sequences of the 246C promoter which are responsible for the described characteristics 
     Starting from vector pSG123 associating the promoter of the 246C gene with the β-glucuronidase gene, different deletions were generated in the 5&#39; region of this promoter by using either restriction enzymes and/or nuclease Exo3. The precise extent of the deletions was determined by sequencing according to Sanger&#39;s method. FIG. 3 shows the different vectors obtained with the aid of these deletions of the 5&#39; part of the promoter, counting from the transcription initiation site in position 2068. 
     a. Study of the strength of the 246C promoter by transient expression in tobacco protoplasts 
     These vectors were used in transient expression on tobacco protoplasts which do not receive any effector. Analysis of the results shows that the maximum expression is obtained with vectors pSG251 and pSG33, reaching 30,000 pmol of methylumbelliferone formed/min/mg of protein. Larger deletions generated in this promoter (corresponding to vectors pSG29, pSG23, pSG451, pSG2, pSG24, pSG3, pSG1) have the effect of reducing the glucuronidase expression in proportion to the size of the deletion (Table below). 
     
         ______________________________________Successive deletions of pSG123              GUS activity (pmol/min/mg)Reference          0______________________________________pBI221             ≈1000pSG123             5000pSG251             29000pSG33              31000pSG29              26000pSG23              22000pSG451             10000PSG2               4000PSG14              1000pSG3               0PSG1               0______________________________________ 
    
     Vectors pSG251 and pSG33 corresponding to the promoters comprising the sequence (B)  vector pSG33! and the sequence (C)  vector pSG251! respectively. 
     b. Study of the strength of the promoter by the stable expression of chimeric constructions containing deleted promoters in transgenic tobaccos For each of the vectors described in FIG. 3, the chimeric gene associating the promoter (complete or truncated) with the coding part of glucuronidase and the NOS terminator was purified on agarose gel after cleavage with the restriction endonucleases HindIII and EcoRI. In each case, the chimeric gene was introduced into and ligated to binary vector pBIN19 (Clontech), previously opened at the HindIII and EcoRI sites (section 13). 
     Tobacco, Nicotiana tabacum, cultivated in vitro, was infected with Agrobacterium tumefaciens containing the different constructions described above. The procedure followed is that described in section 15. 
     The glucuronidase activity is the mean of the measurements made on 10 to 20 independent transformants. In the absence of an inducer, the base glucuronidase activity of the different genotypes is not substantially affected by the deletions for the constructions ranging from pSG251 to pSG451: it is substantially identical to that of genotypes containing construction pSG123 (FIG. 3). For constructions pSG2, pSG24, pSG3 and pSG1, on the other hand, the expression becomes weaker as the length of the promoter becomes shorter, the expressions for pSG3 and pSG1 being zero. 
     In the presence of bacterial inducers (see section 17), the expression of the plants containing constructions pSG251 and pSG33 is stimulated by a factor of 3 relative to construction pSG123. This indicates that the deleted part corresponding to the sequence D  SEQ ID NO: 6! contains a sequence which reduces the inducibility of the 246C promoter; by contrast, the sequence B  SEQ ID NO: 4!, by itself or in the presence of the sequence C  SEQ ID NO: 5!, affords a greater inducibility than the sequence of the 246C promoter (sequences B+C+D). 
     On the other hand, the expression is unchanged for the genotypes containing constructions pSG29 and pSG23 relative to the genotypes containing constructions pSG123. 
     For the genotypes containing constructions pSG451, pSG2, pSG24, pSG3 and pSG1 , the inducibility is systematically less than those of the genotypes containing construction pSG123: it becomes weaker as the promoter becomes shorter and is zero for the plants containing constructions pSG3 and pSG1. 
     These results indicate that the sequence D  SEQ ID NO: 6! contains information of the silencer type, which partially inhibits the inducibility of the complete promoter (sequences B+C+D). 
     
         __________________________________________________________________________SEQUENCE LISTING(1) GENERAL INFORMATION:(iii) NUMBER OF SEQUENCES:18(2) INFORMATION FOR SEQ ID NO: 1:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 631 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(vii) IMMEDIATE SOURCE:(B) CLONE: 246(ix) FEATURE:(A) NAME/KEY: CDS(B) LOCATION:join(1..177, 368..631)(ix) FEATURE:(A) NAME/KEY: intron(B) LOCATION:178..367(ix) FEATURE:(A) NAME/KEY: misc.sub.-- signal(B) LOCATION:175..182(D) OTHER INFORMATION:/function=&#34;consensus spicingsequences&#34;(ix) FEATURE:(A) NAME/KEY: misc.sub.-- signal(B) LOCATION:323..333(D) OTHER INFORMATION:/function=&#34;consensus spicingsequences&#34;(ix) FEATURE:(A) NAME/KEY: misc.sub.-- signal(B) LOCATION:363..368(D) OTHER INFORMATION:/function=&#34;consensus spicingsequences&#34;(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 1:ATGAACCCTGTTCACAAAAAGATCCCTATTTTGATTCACAATAGTAAA48MetAsnProValHisLysLysIleProIleLeuIleHisAsnSerLys151015GCCATTTGTGAGTCTCTAAACATTCTTGAGTACATTGATGAAGTCTGG96AlaIleCysGluSerLeuAsnIleLeuGluTyrIleAspGluValTrp202530CATGACAAATGTCCATTACTTCCTTCTGATCCTTACGAAAAGTCACAA144HisAspLysCysProLeuLeuProSerAspProTyrGluLysSerGln354045GCCAGATTCTGGGCCGACTATATTGACAAGAAGGTAATAAACATCTCACAAAG197AlaArgPheTrpAlaAspTyrIleAspLysLys5055ACTTAACAGTCAATGTAACATGACCTTTACTAAGTTCATCTTGTGTAGTTTCACCGAGCT257GTTTAAGGTCGTCGTACATTTGAATATTAGGTGTTTCACATTTGAATTTTTTTATCCCCT317TGTTAGAATTCCTGATTCTGTCAATACTTATGGACGTTGGTTTAATGCAGATATAT373IleTyr60AGCACAGGAAGAAGAGTGTGGAGCGGTAAAGGTGAAGATCAAGAAGAA421SerThrGlyArgArgValTrpSerGlyLysGlyGluAspGlnGluGlu657075GCAAAGAAGGAATTCATAGAAATACTCAAGACTTTGGAAGGAGAGCTT469AlaLysLysGluPheIleGluIleLeuLysThrLeuGluGlyGluLeu808590GGAAATAAAACTTACTTTGGTGGTGATAATCTGGGTTTTGTGGATGTG517GlyAsnLysThrTyrPheGlyGlyAspAsnLeuGlyPheValAspVal95100105GCTTTGGTTCCCTTTACTAGTTGGTTTTATTCTTATGAGACTTGTGCA565AlaLeuValProPheThrSerTrpPheTyrSerTyrGluThrCysAla110115120125AACTTTAGTATAGAAGCAGAGTGTCCAAAGCTGGTGGTATGGGCAAAA613AsnPheSerIleGluAlaGluCysProLysLeuValValTrpAlaLys130135140ACATGTATGGAGAGCGAG631ThrCysMetGluSerGlu145(2) INFORMATION FOR SEQ ID NO: 2:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 147 amino acids(B) TYPE: amino acid(D) TOPOLOGY: linear(ii) MOLECULE TYPE: protein(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 2:MetAsnProValHisLysLysIleProIleLeuIleHisAsnSerLys151015AlaIleCysGluSerLeuAsnIleLeuGluTyrIleAspGluValTrp202530HisAspLysCysProLeuLeuProSerAspProTyrGluLysSerGln354045AlaArgPheTrpAlaAspTyrIleAspLysLysIleTyrSerThrGly505560ArgArgValTrpSerGlyLysGlyGluAspGlnGluGluAlaLysLys65707580GluPheIleGluIleLeuLysThrLeuGluGlyGluLeuGlyAsnLys859095ThrTyrPheGlyGlyAspAsnLeuGlyPheValAspValAlaLeuVal100105110ProPheThrSerTrpPheTyrSerTyrGluThrCysAlaAsnPheSer115120125IleGluAlaGluCysProLysLeuValValTrpAlaLysThrCysMet130135140GluSerGlu145(2) INFORMATION FOR SEQ ID NO: 3:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 441 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(vii) IMMEDIATE SOURCE:(B) CLONE: 246(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 3:ATGAACCCTGTTCACAAAAAGATCCCTATTTTGATTCACAATAGTAAAGCCATTTGTGAG60TCTCTAAACATTCTTGAGTACATTGATGAAGTCTGGCATGACAAATGTCCATTACTTCCT120TCTGATCCTTACGAAAAGTCACAAGCCAGATTCTGGGCCGACTATATTGACAAGAAGATA180TATAGCACAGGAAGAAGAGTGTGGAGCGGTAAAGGTGAAGATCAAGAAGAAGCAAAGAAG240GAATTCATAGAAATACTCAAGACTTTGGAAGGAGAGCTTGGAAATAAAACTTACTTTGGT300GGTGATAATCTGGGTTTTGTGGATGTGGCTTTGGTTCCCTTTACTAGTTGGTTTTATTCT360TATGAGACTTGTGCAAACTTTAGTATAGAAGCAGAGTGTCCAAAGCTGGTGGTATGGGCA420AAAACATGTATGGAGAGCGAG441(2) INFORMATION FOR SEQ ID NO: 4:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 1096 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 4:TCAAATGAAATACACATAAGAAGCACATAAATTTAAATGCCGTATTAAACTTACAGTATA60CTATAGCGGAAGTTGGCTTGATAAAGGAACGCTGAGGAGAGTAGCCGATGGTGAAACACT120AACATCAAGTGCAAAAGAAAGAAAAACTGAAAACAGAAGATGAATGTTTGAAGTGGGTAA180AAGATTACTTAAAAGATAGGTTTGGTTAACAAATGATTGTGACTGTTACGAAGCAGTGTG240AACCGTTGGGACTTTTAATATTCTTCGGCAGAAGAACATTGCTCTTTCCACGTATGTAGT300CTTTGTCTACTTGTAGTTTTTTTTAATTTAAATTAAATAAGTTAATTAGAGAAATAATAA360GAAGGATATTTTAGTAATTCAACTTTTAACTTTTAGGTTTCCCACTTATAATATAATATA420GATATAGTTTTTTTTAATTTAAATTAAATAAGTTAATTAGAGAAATAATAAGAAGGATAT480TTTAGTAATTCAACTTTTAACTTTTAGGGTTTCCACTTATAATATAATATAGATATAGAT540ATAGATATAGATATAGATAAAGATATATAGATATAGATAGATAATATAGATGGATGAGTC600ATTGGCGATAAAGTGAGGATTGTTTCATTTTTGTTATTAAAAACTTACTACTCCTTAAAT660ATAAAATATGATTCCTTTTAAAAAAGAAATAGAATAAAAATAAAGATAAAACACTAAAAA720TAAATTAATTGTCTAGACAAAATCTACCGTTCACCTCAATTAATACACATCCCCGTCCAC780ATCATGAAGTAGCTAGCACAAGCGTACAGATCAGTTGAAAGAAGAAAAGGGTCCAGTCCT840AAATATCCAAATGTTCATGAAAGGAGGACAACTTAGTTTTTTCTACTAGAAAGAATATTT900TGACGAATTTCGTTCACATTGGCATGCTTTAATTATATTAAGTAGTCTTTCTTGGAAAAG960AAGTATTTGCAATATCAAACCAAATCTTCCCATTACGCAAGCAATGACATCTAAGCAAAT1020ATATATCACTATAAATAGTACTACTAATGTTCAATGACTTTTATAAGCACTACATATATA1080TACTCAAACAAAAAGA1096(2) INFORMATION FOR SEQ ID NO: 5:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 236 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 5:CCTTTTTCGATTCTAATCCAATCAATTCAACAGTGTAAGGTGAAGCAGTCAATTTAAAGG60AAGGCCTTTAAATTCTAAAATATTGTACTTTTCCTGCGCTTCTAAAAGTGAACGACAAAG120AAAAAATAGTTATTCTTGAACTTAATATTGTACAATAGGATAAATTTTAACTATCTATAA180AAAGAGAACAAAACCTTAATCTCTTCAAAATAATATTATAAGAAGTAACATAATTG236(2) INFORMATION FOR SEQ ID NO: 6:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 813 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 6:GAGCTCGGCAAGGCTGACCAAAGTCACAGAAGCGATTGGAATTCGCAGGACAGACCATGC60ACCTGCGCACAAAATGTCGTAGGTGCGACACACCAGAACCAGCACTGGGCAGCAGGTTTC120AATTGCTCTGTGGCTCGTTTGAAACTCATCCGAGCCACTCATGACCTCGTCCGAATATTT180CAACAAGTCCATAAACATAATACGGACATACTCGGGGTTTCACTTCACGTCAAACAACAT240CAAAATTACAAATCACACCCCGATTCGAACCTTGAGTTTTAAACTTTTCAATTTGCAAAT300CTCGTGCCAAAACATATTAAATGAATCCGGAATGACTTCAAATTTATAAATGACATAACG360GAGTTGTTCAAATTTCCAGAATCAGATTCTGCCTTTGATATCAAAAAGTCAACCCCGTGA420TCAAACTTGGAATTCTTTAGCCTTTAAATTGCTAGTTTTCGTTAAATGGTCATAACTTGA480GCTATGGACCTCCAAATTAAATTTCGGGCATACGCTCAAATCCCAATTACGAATACGGAG540CTACCGGACTGTCAAAATACTGATCCGGGTCCGTTTGCTAAAAACGTTGACCAAAGTCCA600CTAAGTTGAGTTTTAAAACTTTATTTCACATTTTAATCCATTTTTTACATGAAAACTTTC660CGGAAAATACGGAGTATGCACGCAAGTCGAGGAATGATAAATGGTACGTTTCGAAGTTTT720AGAACTCAAAATTACTTATTAAATTTAAAGATGACATTTTGGGTCATCACATTGATGAAA780ATTTTGACATTAATATCTGAGAACTTTCTTTGA813(2) INFORMATION FOR SEQ ID NO: 7:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 3046 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: cDNA(iii) HYPOTHETICAL: NO(vii) IMMEDIATE SOURCE:(B) CLONE: 246C(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 7:GAGCTCGGCAAGGCTGACCAAAGTCACAGAAGCGATTGGAATTCGCAGGACAGACCATGC60ACCTGCGCACAAAATGTCGTAGGTGCGACACACCAGAACCAGCACTGGGCAGCAGGTTTC120AATTGCTCTGTGGCTCGTTTGAAACTCATCCGAGCCACTCATGACCTCGTCCGAATATTT180CAACAAGTCCATAAACATAATACGGACATACTCGGGGTTTCACTTCACGTCAAACAACAT240CAAAATTACAAATCACACCCCGATTCGAACCTTGAGTTTTAAACTTTTCAATTTGCAAAT300CTCGTGCCAAAACATATTAAATGAATCCGGAATGACTTCAAATTTATAAATGACATAACG360GAGTTGTTCAAATTTCCAGAATCAGATTCTGCCTTTGATATCAAAAAGTCAACCCCGTGA420TCAAACTTGGAATTCTTTAGCCTTTAAATTGCTAGTTTTCGTTAAATGGTCATAACTTGA480GCTATGGACCTCCAAATTAAATTTCGGGCATACGCTCAAATCCCAATTACGAATACGGAG540CTACCGGACTGTCAAAATACTGATCCGGGTCCGTTTGCTAAAAACGTTGACCAAAGTCCA600CTAAGTTGAGTTTTAAAACTTTATTTCACATTTTAATCCATTTTTTACATGAAAACTTTC660CGGAAAATACGGAGTATGCACGCAAGTCGAGGAATGATAAATGGTACGTTTCGAAGTTTT720AGAACTCAAAATTACTTATTAAATTTAAAGATGACATTTTGGGTCATCACATTGATGAAA780ATTTTGACATTAATATCTGAGAACTTTCTTTGACCTTTTTCGATTCTAATCCAATCAATT840CAACAGTGTAAGGTGAAGCAGTCAATTTAAAGGAAGGCCTTTAAATTCTAAAATATTGTA900CTTTTCCTGCGCTTCTAAAAGTGAACGACAAAGAAAAAATAGTTATTCTTGAACTTAATA960TTGTACAATAGGATAAATTTTAACTATCTATAAAAAGAGAACAAAACCTTAATCTCTTCA1020AAATAATATTATAAGAAGTAACATAATTGTCAAATGAAATACACATAAGAAGCACATAAA1080TTTAAATGCCGTATTAAACTTACAGTATACTATAGCGGAAGTTGGCTTGATAAAGGAACG1140CTGAGGAGAGTAGCCGATGGTGAAACACTAACATCAAGTGCAAAAGAAAGAAAAACTGAA1200AACAGAAGATGAATGTTTGAAGTGGGTAAAAGATTACTTAAAAGATAGGTTTGGTTAACA1260AATGATTGTGACTGTTACGAAGCAGTGTGAACCGTTGGGACTTTTAATATTCTTCGGCAG1320AAGAACATTGCTCTTTCCACGTATGTAGTCTTTGTCTACTTGTAGTTTTTTTTAATTTAA1380ATTAAATAAGTTAATTAGAGAAATAATAAGAAGGATATTTTAGTAATTCAACTTTTAACT1440TTTAGGTTTCCCACTTATAATATAATATAGATATAGTTTTTTTTAATTTAAATTAAATAA1500GTTAATTAGAGAAATAATAAGAAGGATATTTTAGTAATTCAACTTTTAACTTTTAGGGTT1560TCCACTTATAATATAATATAGATATAGATATAGATATAGATATAGATAAAGATATATAGA1620TATAGATAGATAATATAGATGGATGAGTCATTGGCGATAAAGTGAGGATTGTTTCATTTT1680TGTTATTAAAAACTTACTACTCCTTAAATATAAAATATGATTCCTTTTAAAAAAGAAATA1740GAATAAAAATAAAGATAAAACACTAAAAATAAATTAATTGTCTAGACAAAATCTACCGTT1800CACCTCAATTAATACACATCCCCGTCCACATCATGAAGTAGCTAGCACAAGCGTACAGAT1860CAGTTGAAAGAAGAAAAGGGTCCAGTCCTAAATATCCAAATGTTCATGAAAGGAGGACAA1920CTTAGTTTTTTCTACTAGAAAGAATATTTTGACGAATTTCGTTCACATTGGCATGCTTTA1980ATTATATTAAGTAGTCTTTCTTGGAAAAGAAGTATTTGCAATATCAAACCAAATCTTCCC2040ATTACGCAAGCAATGACATCTAAGCAAATATATATCACTATAAATAGTACTACTAATGTT2100CAATGACTTTTATAAGCACTACATATATATACTCAAACAAAAAGAATGGAGAGCAACAAC2160GTGGTTCTGCTAGATTTCTGGCCAAGCTCTTTTGGTATGAGGCTAAGAATTGCATTGGCC2220TTAAAGGGAATCAAATATGAAGCAAAGGAGGAAAACTTATCTGATAAAAGCCCTTTGCTT2280CTGGAGATGAACCCTGTTCACAAAAAGATCCCTATTTTGATTCACAATAGTAAAGCCATT2340TGTGAGTCTCTAAACATTCTTGAGTACATTGATGAAGTCTGGCATGACAAATGTCCATTA2400CTTCCTTCTGATCCTTACGAAAAGTCACAAGCCAGATTCTGGGCCGACTATATTGACAAG2460AAGGTAATAAACATCTCACAAAGACTTAACAGTCAATGTAACATGACCTTTACTAAGTTC2520ATCTTGTGTAGTTTCACCGAGCTGTTTAAGGTCGTCGTACATTTGAATATTAGGTGTTTC2580ACATTTGAATTTTTTTATCCCCTTGTTAGAATTCCTGATTCTGTCAATACTTATGGACGT2640TGGTTTAATGCAGATATATAGCACAGGAAGAAGAGTGTGGAGCGGTAAAGGTGAAGATCA2700AGAAGAAGCAAAGAAGGAATTCATAGAAATACTCAAGACTTTGGAAGGAGAGCTTGGAAA2760TAAAACTTACTTTGGTGGTGATAATCTGGGTTTTGTGGATGTGGCTTTGGTTCCCTTTAC2820TAGTTGGTTTTATTCTTATGAGACTTGTGCAAACTTTAGTATAGAAGCAGAGTGTCCAAA2880GCTGGTGGTATGGGCAAAAACATGTATGGAGAGCGAGAGTGTCTCAAAGTCCCTTCCTCA2940TCCTCACAAGATCTATGGTTTTGTCTTGGAACTCAAGCACAAGCTTGGTCTTGCTTGAAC3000AAGAAACACTTCTTACCTACTGCAGAAACCAATCATGTCCTTCGTC3046(2) INFORMATION FOR SEQ ID NO: 8:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 809 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 8:ACGTATGTAGTCTTTGTCTACTTGTAGTTTTTTTTAATTTAAATTAAATAAGTTAATTAG60AGAAATAATAAGAAGGATATTTTAGTAATTCAACTTTTAACTTTTAGGTTTCCCACTTAT120AATATAATATAGATATAGTTTTTTTTAATTTAAATTAAATAAGTTAATTAGAGAAATAAT180AAGAAGGATATTTTAGTAATTCAACTTTTAACTTTTAGGGTTTCCACTTATAATATAATA240TAGATATAGATATAGATATAGATATAGATAAAAGATATATAGATATAGATAGATAATATA300GATGGATGAGTCATTGGCGATAAAGTGAGGATGTTTCATTTTTGTTATTAAAAACTTACT360ACTCCTTAAATATAAAATATGATTCCTTTTAAAAAAGAAATAGAATAAAAATAAAGATAA420AACACTAAAAATAAATTAATTGTCTAGACAAAATCTACCGTTCACCTCAATTAATACACA480TCCCCGTCCACATCATGAAGTAGCTAGCACAAGCGTACAGATCAGTTGAAAGAAGAAAAG540GGTCCAGTCCTAAATATCCAAATGTTCATGAAAGGAGGACAACTTAGTTTTTTCTACTAG600AAAGAATATTTTGACGAATTTCGTTCACATTGGCATGCTTTAATTTATTAAGTAGTCTTT660CTTGGAAAAGAAGTATTTGCAATATCAAACCAAATCTTCCCATTACGCAAGCAATGACAT720CTAAGCAAATATATATCACTATAAATAGTACTACTAATGTTCAATGACTTTTATAAGCAC780TACATATATATTCTCAAACAAAAAGAATG809(2) INFORMATION FOR SEQ ID NO: 9:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 331 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:ACGTATGTAGTCTTTGTCTACTTGTAGTTTTTTTTAATTTAAATTAAATAAGTTAATTAG60AGAAATAATAAGAAGGATATTTTAGTAATTCAACTTTTAACTTTTAGGTTTCCCACTTAT120AATATAATATAGATATAGTTTTTTTTAATTTAAATTAAATAAGTTAATTAGAGAAATAAT180AAGAAGGATATTTTAGTAATTCAACTTTTAACTTTTAGGGTTTCCACTTATAATATAATA240TAGATATAGATATAGATATAGATATAGATAAAAGATATATAGATATAGATAGATAATATA300GATGGATGAGTCATTGGCGATAAAGTGAGGA331(2) INFORMATION FOR SEQ ID NO: 10:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 314 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 10:TGTTTCATTTTTGTTATTAAAAACTTACTACTCCTTAAATATAAAATATGATTCCTTTTA60AAAAAGAAATAGAATAAAAATAAAGATAAAACACTAAAAATAAATTAATTGTCTAGACAA120AATCTACCGTTCACCTCAATTAATACACATCCCCGTCCACATCATGAAGTAGCTAGCACA180AGCGTACAGATCAGTTGAAAGAAGAAAAGGGTCCAGTCCTAAATATCCAAATGTTCATGA240AAGGAGGACAACTTAGTTTTTTCTACTAGAAAGAATATTTTGACGAATTTCGTTCACATT300GGCATGCTTTAATT314(2) INFORMATION FOR SEQ ID NO: 11:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 161 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: 11:TATTAAGTAGTCTTTCTTGGAAAAGAAGTATTTGCAATATCAAACCAAATCTTCCCATTA60CGCAAGCAATGACATCTAAGCAAATATATATCACTATAAATAGTACTACTAATGTTCAAT120GACTTTTATAAGCACTACATATATATTCTCAAACAAAAAGA161(2) INFORMATION FOR SEQ ID NO: 12:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 307 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: 12:CTTTTAATATTCTTCGGCAGAAGAACATTGCTCTTTCCACGTATGTAGTCTTTGTCTACT60TGTAGTTTTTTTTAATTTAAATTAAATAAGTTAATTAGAGAAATAATAAGAAGGATATTT120TAGTAATTCAACTTTTAACTTTTAGGTTTCCCACTTATAATATAATATAGATATAGTTTT180TTTTAATTTAAATTAAATAAGTTAATTAGAGAAATAATAAGAAGGATATTTTAGTAATTC240AACTTTTAACTTTTAGGGTTTCCACTTATAATATAATATAGATATAGATATAGATATAGA300TATAGAT307(2) INFORMATION FOR SEQ ID NO: 13:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 538 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: 13:AAAGATATATAGATATAGATAGATAATATAGATGGATGAGTCATTGGCGATAAAGTGAGG60ATTGTTTCATTTTTGTTATTAAAAACTTACTACTCCTTAAATATAAAATATGATTCCTTT120TAAAAAAGAAATAGAATAAAAATAAAGATAAAACACTAAAAATAAATTAATTGTCTAGAC180AAAATCTACCGTTCACCTCAATTAATACACATCCCCGTCCACATCATGAAGTAGCTAGCA240CAAGCGTACAGATCAGTTGAAAGAAGAAAAGGGTCCAGTCCTAAATATCCAAATGTTCAT300GAAAGGAGGACAACTTAGTTTTTTCTACTAGAAAGAATATTTTGACGAATTTCGTTCACA360TTGGCATGCTTTAATTATATTAAGTAGTCTTTCTTGGAAAAGAAGTATTTGCAATATCAA420ACCAAATCTTCCCATTACGCAAGCAATGACATCTAAGCAAATATATATCACTATAAATAG480TACTACTAATGTTCAATGACTTTTATAAGCACTACATATATATACTCAAACAAAAAGA538(2) INFORMATION FOR SEQ ID NO: 14:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 4284 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 14:AAGCTTGGCAAGGCTGACCAAAGTCACAGAAGCGATTGGAATTCGCAGGACAGACCATGC60ACCTGCGCACAAAATGTCGTAGGTGCGACACACCAGAACCAGCACTGGGCAGCAGGTTTC120AATTGCTCTGTGGCTCGTTTGAAACTCATCCGAGCCACTCATGACCTCGTCCGAATATTT180CAACAAGTCCATAAACATAATACGGACATACTCGGGGTTTCACTTCACGTCAAACAACAT240CAAAATTACAAATCACACCCCGATTCGAACCTTGAGTTTTAAACTTTTCAATTTGCAAAT300CTCGTGCCAAAACATATTAAATGAATCCGGAATGACTTCAAATTTATAAATGACATAACG360GAGTTGTTCAAATTTCCAGAATCAGATTCTGCCTTTGATATCAAAAAGTCAACCCCGTGA420TCAAACTTGGAATTCTTTAGCCTTTAAATTGCTAGTTTTCGTTAAATGGTCATAACTTGA480GCTATGGACCTCCAAATTAAATTTCGGGCATACGCTCAAATCCCAATTACGAATACGGAG540CTACCGGACTGTCAAAATACTGATCCGGGTCCGTTTGCTAAAAACGTTGACCAAAGTCCA600CTAAGTTGAGTTTTAAAACTTTATTTCACATTTTAATCCATTTTTTACATGAAAACTTTC660CGGAAAATACGGAGTATGCACGCAAGTCGAGGAATGATAAATGGTACGTTTCGAAGTTTT720AGAACTCAAAATTACTTATTAAATTTAAAGATGACATTTTGGGTCATCACATTGATGAAA780ATTTTGACATTAATATCTGAGAACTTTCTTTGACCTTTTTCGATTCTAATCCAATCAATT840CAACAGTGTAAGGTGAAGCAGTCAATTTAAAGGAAGGCCTTTAAATTCTAAAATATTGTA900CTTTTCCTGCGCTTCTAAAAGTGAACGACAAAGAAAAAATAGTTATTCTTGAACTTAATA960TTGTACAATAGGATAAATTTTAACTATCTATAAAAAGAGAACAAAACCTTAATCTCTTCA1020AAATAATATTATAAGAAGTAACATAATTGTCAAATGAAATACACATAAGAAGCACATAAA1080TTTAAATGCCGTATTAAACTTACAGTATACTATAGCGGAAGTTGGCTTGATAAAGGAACG1140CTGAGGAGAGTAGCCGATGGTGAAACACTAACATCAAGTGCAAAAGAAAGAAAAACTGAA1200AACAGAAGATGAATGTTTGAAGTGGGTAAAAGATTACTTAAAAGATAGGTTTGGTTAACA1260AATGATTGTGACTGTTACGAAGCAGTGTGAACCGTTGGGACTTTTAATATTCTTCGGCAG1320AAGAACATTGCTCTTTCCACGTATGTAGTCTTTGTCTACTTGTAGTTTTTTTTAATTTAA1380ATTAAATAAGTTAATTAGAGAAATAATAAGAAGGATATTTTAGTAATTCAACTTTTAACT1440TTTAGGTTTCCCACTTATAATATAATATAGATATAGTTTTTTTTAATTTAAATTAAATAA1500GTTAATTAGAGAAATAATAAGAAGGATATTTTAGTAATTCAACTTTTAACTTTTAGGGTT1560TCCACTTATAATATAATATAGATATAGATATAGATATAGATATAGATAAAGATATATAGA1620TATAGATAGATAATATAGATGGATGAGTCATTGGCGATAAAGTGAGGATTGTTTCATTTT1680TGTTATTAAAAACTTACTACTCCTTAAATATAAAATATGATTCCTTTTAAAAAAGAAATA1740GAATAAAAATAAAGATAAAACACTAAAAATAAATTAATTGTCTAGACAAAATCTACCGTT1800CACCTCAATTAATACACATCCCCGTCCACATCATGAAGTAGCTAGCACAAGCGTACAGAT1860CAGTTGAAAGAAGAAAAGGGTCCAGTCCTAAATATCCAAATGTTCATGAAAGGAGGACAA1920CTTAGTTTTTTCTACTAGAAAGAATATTTTGACGAATTTCGTTCACATTGGCATGCTTTA1980ATTATATTAAGTAGTCTTTCTTGGAAAAGAAGTATTTGCAATATCAAACCAAATCTTCCC2040ATTACGCAAGCAATGACATCTAAGCAAATATATATCACTATAAATAGTACTACTAATGTT2100CAATGACTTTTATAAGCACTACATATATATACTCAAACAAAAAGAATGGAGAGCAACAAC2160GTGGTTCTGCTAGATTTCTGGGGGTACGGTCAGTCCCTTATGTTACGTCCTGTAGAAACC2220CCAACCCGTGAAATCAAAAAACTCGACGGCCTGTGGGCATTCAGTCTGGATCGCGAAAAC2280TGTGGAATTGATCAGCGTTGGTGGGAAAGCGCGTTACAAGAAAGCCGGGCAATTGCTGTG2340CCAGGCAGTTTTAACGATCAGTTCGCCGATGCAGATATTCGTAATTATGCGGGCAACGTC2400TGGTATCAGCGCGAAGTCTTTATACCGAAAGGTTGGGCAGGCCAGCGTATCGTGCTGCGT2460TTCGATGCGGTCACTCATTACGGCAAAGTGTGGGTCAATAATCAGGAAGTGATGGAGCAT2520CAGGGCGGCTATACGCCATTTGAAGCCGATGTCACGCCGTATGTTATTGCCGGGAAAAGT2580GTACGTATCACCGTTTGTGTGAACAACGAACTGAACTGGCAGACTATCCCGCCGGGAATG2640GTGATTACCGACGAAAACGGCAAGAAAAAGCAGTCTTACTTCCATGATTTCTTTAACTAT2700GCCGGAATCCATCGCAGCGTAATGCTCTACACCACGCCGAACACCTGGGTGGACGATATC2760ACCGTGGTGACGCATGTCGCGCAAGACTGTAACCACGCGTCTGTTGACTGGCAGGTGGTG2820GCCAATGGTGATGTCAGCGTTGAACTGCGTGATGCGGATCAACAGGTGGTTGCAACTGGA2880CAAGGCACTAGCGGCACTTTGCAAGTGGTGAATCCGCACCTCTGGCAACCGGGTGAAGGT2940TATCTCTATGAACTGTGCGTCACAGCCAAAAGCCAGACAGAGTGTGATATCTACCCGCTT3000CGCGTCGGCATCCGGTCAGTGGCAGTGAAGGGCGAACAGTTCCTGATTAACCACAAACCG3060TTCTACTTTACTGGCTTTGGTCGTCATGAAGATGCGGACTTACGTGGCAAAGGATTCGAT3120AACGTGCTGATGGTGCACGACCACGCATTAATGGACTGGATTGGGGCCAACTCCTACCGT3180ACCTCGCATTACCCTTACGCTGAAGAGATGCTCGACTGGGCAGATGAACATGGCATCGTG3240GTGATTGATGAAACTGCTGCTGTCGGCTTTAACCTCTCTTTAGGCATTGGTTTCGAAGCG3300GGCAACAAGCCGAAAGAACTGTACAGCGAAGAGGCAGTCAACGGCGAAACTCAGCAAGCG3360CACTTACAGGCGATTAAAGAGCTGATAGCGCGTGACAAAAACCACCCAAGCGTGGTGATG3420TGGAGTATTGCCAACGAACCGGATACCCGTCCGCAAGTGCACGGGAATATTTCGCCACTG3480GCGGAAGCAACGCGTAAACTCGACCCGACGCGTCCGATCACCTGCGTCAATGTAATGTTC3540TGCGACGCTCACACCGATACCATCAGCGATCTCTTTGATGTGCTGTGCCTGAACCGTTAT3600TACGGATGGTATGTCCAAAGCGGCGATTTGGAAACGGCAGAGAAGGTACTGGAAAAAGAA3660CTTCTGGCCTGGCAGGAGAAACTGCATCAGCCGATTATCATCACCGAATACGGCGTGGAT3720ACGTTAGCCGGGCTGCACTCAATGTACACCGACATGTGGAGTGAAGAGTATCAGTGTGCA3780TGGCTGGATATGTATCACCGCGTCTTTGATCGCGTCAGCGCCGTCGTCGGTGAACAGGTA3840TGGAATTTCGCCGATTTTGCGACCTCGCAAGGCATATTGCGCGTTGGCGGTAACAAGAAA3900GGGATCTTCACTCAGCGACCGCAAACCGAAGTCGGCGGCTTTTCTGCTGCAAAAACGCTG3960GACTGGCATGAACTTCGGTGAAAAACCGCAGCAGGGAGGCAAACAATGAGAGCTCGAATT4020TCCCCGATCGTTCAAACATTTGGCAATAAAGTTTCTTAAGATTGAATCCTGTTGCCGGTC4080TTGCGATGATTATCATATAATTTCTGTTGAATTACGTTAAGCATGTAATAATTAACATGT4140AATGCATGACGTTATTTATGAGATGGGTTTTTATGATTAGAGTCCCGCAATTATACATTT4200AATACGCGATAGAAAACAAAATATAGCGCGCAAACTAGGATAAATTATCGCGCGCGGTGT4260CATCTATGTTACTAGATCGAATTC4284(2) INFORMATION FOR SEQ ID NO: 15:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 58 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 15:ACTACTAATGTTCAATGACTTTTATAAGCACTACATATATATACTCAAACAAAAAGAG58(2) INFORMATION FOR SEQ ID NO: 16:(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: 16:AAGCTTGCACGACACACTTGTCTACTCCAAAAATATCAAAGATACAGTCCTCAGAAGACC60AAAGGGCCAATTGAGACTTTTCAACAAAGGGTAATATCCGGAAACCTCCTCGGATTCCAT120TGCCCAGCTATCTGTCACTTTATTGTGAAGATAGTGGAAAAGGAAGGTGGCTCCTACAAA180TGCCATCATTGCGATAAAGGAAAGGCCATCGTTGAAGATGCCTCTGCCGACAGTGGTCCC240AAAGATGGACCCCCACCCACGAGGAGCATCGTGGAAAAAGAAGACGTTCCAACCACGTCT300TCAAAGCAAGTGGATTGATGTGATATCTCCACTGACGTAAGGGATGACGCACAATCCCAC360TATCCTTCGCAAGACCCTTCCTCTATATAAGGAAGTTCATTTCATTTGGAGAGAACACGG420GGGACTCTAGAGGATCCATGAGGCGAACTTCTAAATTGACTACTTTTTCTTTGCTGTTTT480CTCTGGTTTTGCTGAGTGCTGCCTTGGCACAGAATTGTGGTTCACAGGGCGGAGGCAAAG540TTTGTGCGTCGGGACAATGTTGCAGCAAATTCGGGTGGTGCGGTAACACTAATGACCATT600GTGGTTCTGGCAATTGTCAAAGTCAGTGTCCAGGTGGCGGCCCTGGTCCTGGTCCTGTTA660CTGGTGGGGACCTCGGAAGCGTCATCTCAAATTCTATGTTTGATCAAATGCTTAAGCATC720GTAACGAAAATTCTTGTCAAGGAAAGAATAATTTCTACAGTTACAATGCCTTTATTACTG780CTGCTAGGTCTTTTCCTGGCTTTGGTACAAGTGGTGATATCAATGCCCGTAAAAGGGAAA840TTGCTGCTTTCTTTGCCCAAACCTCCCATGAAACTACTGGTATGTGTATAACCATTCACA900TCGAACCATTAAAATATAATTTCATTTTATTTTATTTAGTAATTGATTATATATGTAGGA960GGATGGCCTTCCGCACCTGATGGACCATTCGCATGGGGTTACTGTTTCCTTAGAGAACGA1020GGTAACCCCGGTGACTACTGTTCACCAAGTAGTCAATGGCCTTGTGCACCTGGAAGGAAA1080TATTTCGGACGAGGCCCAATCCAAATTTCACAGTAAGCTACATAAATCTATATATGGTAA1140AATTTGATGAACTTGTAGTGTCTAATTACGTGTATTTTGACATTTCAAAACAGCAACTAC1200AACTATGGGCCATGTGGAAGAGCCATCGGAGTGGACCTTTTAAACAATCCTGATTTAGTA1260GCCACAGACCCAGTCATCTCATTCAAGACTGCTATCTGGTTCTGGATGACCCCTCAATCA1320CCAAAGCCTTCTTGCCACGATGTCATCATTGGAAGATGGAACCCATCTGCCGGTGACCGA1380TCAGCCAATCGTCTTCCTGGATTTGGTGTCATCACAAACATCATCAATGGGGGCCTGGAA1440TGTGGTCGTGGCAATGACAATAGGGTCCAGGATCGCATTGGGTTTTACAGGAGGTATTGC1500GGTATTCTTGGTGTTAGTCCTGGTGACAATCTTGATTGCGGAAACCAGAGATCTTTTGGA1560AACGGACTTTTAGTCGATACTATGTAATGAGCTCGAATTTCCCCGATCGTTCAAACATTT1620GGCAATAAAGTTTCTTAAGATTGAATCCTGTTGCCGGTCTTGCGATGATTATCATATAAT1680TTCTGTTGAATTACGTTAAGCATGTAATAATTAACATGTAATGCATGACGTTATTTATGA1740GATGGGTTTTTATGATTAGAGTCCCGCAATTATACATTTAATACGCGATAGAAAACAAAA1800TATAGCGCGCAAACTAGGATAAATTATCGCGCGCGGTGTCATCTATGTTACTAGATCGAA1860TTC1863(2) INFORMATION FOR SEQ ID NO: 17:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 18 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 17:GAANNGAANNTTCNNTTC18(2) INFORMATION FOR SEQ ID NO: 18:(i) SEQUENCE CHARACTERISTICS:(A) LENGTH: 18 base pairs(B) TYPE: nucleic acid(C) STRANDEDNESS: single(D) TOPOLOGY: linear(ii) MOLECULE TYPE: DNA (genomic)(iii) HYPOTHETICAL: NO(xi) SEQUENCE DESCRIPTION: SEQ ID NO: 18:TTCNNTTCNNGAANNGAA18__________________________________________________________________________