CN1858207A - Plant multifunction activity and broad spectrum resistance cell signal factor encoding hrpZ gene and its expression product and use - Google Patents
Plant multifunction activity and broad spectrum resistance cell signal factor encoding hrpZ gene and its expression product and use Download PDFInfo
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- CN1858207A CN1858207A CN 200510020814 CN200510020814A CN1858207A CN 1858207 A CN1858207 A CN 1858207A CN 200510020814 CN200510020814 CN 200510020814 CN 200510020814 A CN200510020814 A CN 200510020814A CN 1858207 A CN1858207 A CN 1858207A
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- Peptides Or Proteins (AREA)
Abstract
The present invention discloses a kind of hrpZ gene of cell signal factor encoding multifunctional activity and broad spectrum resistance and its expression product and application. The gene of the present invention is originated from Pseudomonas syringae pv.tomota strain, has 1113 nucleotides and the nucleotide sequence of SEQ ID No.1. The gene has wide application in agricultural breeding and transgenic plant related to regulating plant's growth and development and preventing and controlling diseases and pests. The gene coded protein has the amino acid sequence of SEQ ID No.2, and possesses several functional activities of inducing plant to generate broad spectrum disease resistance, pest expelling resistance and stress tolerance, promoting plant growth and development and raising yield.
Description
Technical field
The invention belongs to the biological gene engineering field, more particularly, relate to the hrpZ gene and the expression product thereof of a kind of multifunctional activity of coded plant and broad spectrum resistante cell singal gene, and this gene and its expression product are in the application of aspects such as improvement plant quality.
Background technology
The microbial proteinous agricultural chemicals is that multiple kinds of crops is had the very class protein medicine of strong biological activity, can be divided into traditional microbial proteinous agricultural chemicals and novel microorganism albumen agricultural chemicals again according to the difference of the mechanism of action.Tradition microbial proteinous agricultural chemicals mainly is the insecticidal crystal protein (ICP) from bacillus thuringiensis (Bt), novel microorganism albumen agricultural chemicals mainly is an albumen exciton class material, the difference of it and traditional microbial proteinous agricultural chemicals maximum is its directly kill pests and pathogen, but excite the disease-resistant, insect-prevention expression of gene of plant self, and promote growth and development of plant.At present the representative novel microorganism albumen agricultural chemicals of research report mainly contains allergen protein (Harpin), latent ground albumen (Cryptogein) and activator (Activator) etc., and is wherein of greatest concern, what application prospect was arranged most is Harpin proteinoid exciton.
Harpin albumen mainly is can excite the anaphylactoid protein of plant (30-40kda) by the bacteriogenic class of Erwinia (Erwinia), but the expression of series of genes in its inducing plant body, the growing system of activated plant self and defence system, thereby make plant can resist infecting of multiple diseases and coercing of adverse circumstance, and obtain to promote to grow and improve the effect of volume increase.1992, the Wei Zhongmin of U.S. Cornell University etc. at first clone this class allergen protein gene from pears fire epidemic disease Erwinias (E.amylovora), and the anaphylaxis that proposes the protein induced plant of Harpin first may be relevant with its disease resistance effect, promoted the rise of novel microorganism albumen pesticide research thus.Through about 10 years effort; U.S. Eden biotechnology company as background successfully develops and develops the novel microorganism albumen agricultural chemicals Messenger with broad-spectrum disease resistance insect protected function; this product to the good effect in field crop and cash crop disease-resistant yield-increasing aspect and to the remarkable contribution of green non-pollution agricultural, once obtained the presidential Green Chemistry challenge prize that the U.S. environment protection council issues with it twice.
Modern molecule plant pathology discloses, plant pathogenetic bacteria is existing, and it is pathogenic, the ability that also has inducing plant to produce disease resistance and promote to grow, and determine that the gene of this ability is hrp (the hypersensitive response and pathogenicity) gene cluster of plant pathogenetic bacteria.The hrp gene is determining plant pathogenetic bacteria to excite anaphylaxis (hypersensitive response on non-host plants, ability HR) and the basic parasitics on host plant or pathogenic (parasitism or pathogenicity onhost plants) on non-host plant.HR is a kind of partial, cell dead form of programming fast of plant, be the initiatively result of resistance of plant, its resistance effect not only shows the restriction of pathogenetic bacteria being infected expansion, and the further interior systemic acquired resistance reaction that produces similar immunologic mechanism of inducing plant body.
Continue (Wei ZM, et al.Science, 1992,257 (5066): 85-88) successfully clone and express hrpN such as Wei Zhongmin
EaAfter the gene, people are cloned into the gene of coding Harpin proteinoid again in succession from E.carotovora subspcarotovora, E.chrysanthemi, P.s.syringae, P.s.pv.glycinea, P.s.tomato, R.solanacearum during the nearly last ten years, and successful expression these albumen, as Harpin
Ecc, 36kda (Mukherjee A., Mol.Plant-Microbe Interact.1997,10:462-471); Harpin
Ech, 36kda (Bauer D.W., Mol.Plant Microbe Interact, 1995,8:484 491); Harpin
Pss, 34.7kda; Harpin
Psg, 35.3kda; Harpin
Pst, 36.5kda (Preston G, Mol Plant-Microbe Interact., 1995,8:717); Harpin
Xoo, 15.3kda, Harpin
Xooc, 15.6kda (Wen Weigang, plant pathology, 2001,31 (4): 295-300) etc.
Up to now, all these Harpin proteinoids almost all have following characterization of molecules: (1) wetting ability; (2) to thermally-stabilised, 100 ℃ handle 10 minutes can inactivation; (3) to Proteinase K and ultraviolet-sensitive; (4) be rich in glycine and lack halfcystine; (5) water-soluble acid albumen; (6) no quaternary structure.
Nearest studies show that the Harpin proteinoid may play an important role in the signal path of plant.The researchist handles Arabidopis thaliana with Harpin, find that Cl, Ca, K, H, Cu, Zn ionic channel and various oxydase are activated in the Arabidopis thaliana, these oxydase comprise ACC synthetic enzyme, Vitamin C oxidase, Cu/Zn superoxide-dismutase, Cu molecular chaperones precursor or the like.It has been generally acknowledged that now, extensively there is the proteic acceptor of Harpin in the plant cell wall, be that conjugated protein (Harpin-binding proteins, HrBP), Harpin can be by combining the many signal paths in the activated plant with these receptor proteins HrBP for Harpin.These signal paths roughly can be divided into following three classes: the activation of the signal path that (1) is relevant with plant disease-resistant and expelling parasite comprises the approach of anaphylaxis and necrocytosis, ion-exchange passage, salicylate pathway, jasmonic approach, phenylalanine ammonia lyase mediation and the approach of some other resistant gene mediation; (2), comprise that general growth regulator, plumular axis extend transcription factor, growth transcription factor, ethylene reaction element conjugated protein system and sucrose synthase and other embryos form enzyme etc. with the activation that promotes the signal path that plant-growth is relevant; (3) activation of the signal path relevant with plant stress-resistance comprises heat shock protein(HSP), COR gene and salt tolerant zinc albumen etc.May also there be the signal path of a more special plant that does not rely on the NPR1 mediation in addition to bacterial resistance.
Though Harpin albumen derives from pathogenic bacteria, as the nonspecific elicitor protein factor of a class, but can cause non-host plant generation anaphylaxis, and induce the increase of its disease resistance, insect-repellent and resistance, and promote to grow, improve output etc.Changeing hrpN
EaOn the pears of gene, Harpin
EaThe host bacterial parasite E.amylovora that produces fire blight of pear is also shown very strong resistance.
Summary of the invention
The hrpZ gene and the expression product thereof that the purpose of this invention is to provide a kind of multifunctional activity of coded plant and broad spectrum resistante cell singal gene, and the application of this gene and its expression product.
The hrpZ gene of a kind of multifunctional activity of coded plant provided by the present invention and broad spectrum resistante cell singal gene, name is called hrpZ
CSCS008Its gene coding region has 1113 Nucleotide altogether, SEQ ID No.1 in its nucleotide sequence such as the sequence table, this gene source is in the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) CSCS008 bacterial strain, tomato is the host plant of this bacillus, and this gene is present on the chromosomal DNA of CSSY002 bacterial strain with hrpZ gene cluster form.This gene can be used for promoting growth and development of plants; Strengthen the broad spectrum resistance of plant, comprise resistance various bacteria, fungi and virus; Strengthen the insect-repellent of plant; Strengthen the resistance (plant is to the tolerance of arid, severe cold, poor environment such as saline and alkaline) of plant; Prolong the storage time of crop product; Plastotype effect to potted flower, nursery stock.This gene can also be as genetic resources in addition, grows the Agricultural biotechnologies breeding relevant with prevention and elimination of disease and pests, transgenic plant and is widely used with aspects such as genetic recombination body that other desirable genes recombination to construct has a commercial value in coordinate plant growth.The genetic recombination body that contains this gene also can be applicable to coordinate plant growth and grows aspects such as the Agricultural biotechnologies breeding relevant with prevention and elimination of disease and pests, transgenic plant.
The present invention also provides this expression of gene product Harpin
CSCS008Protein, SEQ ID No.2 in its aminoacid sequence such as the sequence table, this protein has 370 amino-acid residues, molecular weight is 36.52kda, iso-electric point pI:4.01, be rich in glycine Gly and lack halfcystine Cys, and have the basic molecule attribute and the biologic activity of Harpin proteinoid.This protein (comprises the resistance to various bacteria, fungi and virus in the broad spectrum resistance that promotes growth and development of plants, enhancing plant; ) strengthen the insect-repellent of plant, the resistance (plant is to the tolerance of arid, severe cold, poor environment such as saline and alkaline) that strengthens plant, prolongation crop product storage time, the plastotype effect aspect of potted flower, nursery stock is had wide application prospects.Therefore, this protein can be mixed with biological products, is applied to above aspect.
Gene hrpZ about a kind of multifunctional activity of coded plant and broad spectrum resistante cell singal gene provided by the invention
CSCS008And expression product Harpin
CSCS008Protein, specifically explain by following content:
1, hrpZ
CSCS008The source hrpZ of gene
CSCS008Gene is from the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) CSCS008 bacterial strain, and tomato is its host plant.This gene is present on the chromosomal DNA of CSSY002 bacterial strain with hrpZ gene cluster form.
2, hrpZ
CSCS008The clone of gene and order-checking (1) are at first screened the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) CSCS008 bacterial strain on the LB flat board, this bacterial strain can be secreted xanthein, and under UV-light fluorescence takes place.(2) with the mono-clonal bacterium colony of choosing, under 28 ℃ in the LB liquid nutrient medium shaking culture 12 hours, centrifugal collection thalline, with the genomic dna separating kit separate, the purification of bacterial chromosomal DNA.(3) bacterial chromosomal dna partly digests through Sau3A, makes up the genomic library of the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) CSCS008 bacterial strain with plasmid vector pLARF5.(4) make molecular probe with the hrpZ gene of the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) DC3000 bacterial strain, screen from the CSCS008 genomic library by clone hybridization and differentiate hrpZ
+Plasmid obtains to comprise the 2.0kb DNAs fragment of the whole coding region of hrpZ gene, and further this fragment subclone is advanced in the pBluescript carrier.(5) carry out nucleotide sequencing with general T7 primer, wherein have the reading frame (reading frame) of a 1113bp to be hrpZ
CSCS008The coding region of gene, sequence such as SEQ ID No.1.
3, hrpZ
CSCS008The pcr amplification of gene and purifying are according to hrpZ
CSCS008The nucleotide sequence of gene, design one couple of PCR amplimer, i.e. P1:5 '-TGT
GGATCCATGCAAGCACTTAACAGCATCAG-3 ' and P2:5 '-TGT
AAGCTTTCAGGCCACAGCCTGGTTAGTCTG-3 '.Wherein G/GATCC is the restriction enzyme site of the restriction enzyme BamH I of introducing, and A/AGCTT is the restriction enzyme site of the restriction enzyme HindIII of introducing.Chromosomal DNA with the CSCS008 bacterial strain of purifying is made template, carries out the PCR reaction by following amplification parameter: 95 ℃ of pre-sex change 5min earlier, 1 circulation of 94 ℃/2min then; 94 ℃/15sec+55 ℃/30sec+72 ℃/24 circulations of 15sec; 94 ℃/1min+55 ℃/2min+72 ℃/a 3min1 circulation.Amplified production carries out purifying with PCR product purification test kit.
4, hrpZ
CSCS008The structure hrpZ of engineering strain
CSCS008The pcr amplification product of gene is after restriction enzyme BamH I and HindIII digestion, and the clone enters the BamH I-HindIII site of high-expression vector pET28a (+).With pET28a (+)-hrpZ
CSCS008Plasmid transformation receptor bacterium E.coli JM109 (DE3) contains pET28a (+)-hrpZ by selecting to press to filter out
CSCS008The positive expression engineering strain of plasmid.
5, hrpZ
CSCS008Expression of gene product and detection hrpZ thereof
CSCS008The expression of gene product is Harpin
CSCS008Protein.To contain hrpZ
CSCS008Gene overexpression plasmid pET28a (+)-hrpZ
CSCS008Colibacillus engineering strain E.coli JM109 (DE3) 37 ℃ of incubation growth in being added with the LB liquid nutrient medium of 50ml/L Km, treat OD
600After reaching 0.7 (being that bacterium enters logarithmic phase), add inductor IPTG again, continue to cultivate after 6 hours centrifugal collection bacterial cell to final concentration 1mM.Bacterial cell on the bacteria samples swimming lane of electrophoresis offset plate, can present a remarkable wide and dense 36.52kda band through ultrasonic disruption, centrifugal, 12%SDS-PAGE gel electrophoresis, and it is exactly hrpZ
CSCS008Expression of gene product Harpin
CSCS008Protein accounts for about 50% of bacterioprotein total amount.With Harpin
CSCS008The further separation and purification of protein, and to Harpin
CSCS008Protein carries out Western blot analysis and HR detects.
According to hrpZ
CSCS008The nucleotide sequence of gene is inferred, Harpin
CSCS008Proteinic aminoacid sequence such as SEQ ID No.2.This protein has following attribute: (1) is made up of 370 amino-acid residues; (2) molecular weight 36.52kda; (3) iso-electric point pI:4.01; (4) be rich in glycine Gly, lack halfcystine Cys; (5) special stable to temperature, tolerance still had activity in 10-15 minute in 100 ℃ of boiling water; (6) there is not quaternary structure.
6, Harpin
CSCS008The biological activity assay method of the Harpin proteinoid that proteinic biologic activity and application thereof are generally acknowledged at present mainly contains: (1) anaphylaxis (hypersensitive response, HR), usually do tested plant with tobacco, this also is quick, the easiest method of Harpin proteinoid biological activity assay; (2) serological reaction, promptly make serum antibody with the pure product of Harpin albumen of standard, with this antiserum(antisera) unknown sample is carried out Western blot then and analyze,, can accurately detect the Harpin proteinoid in the unknown sample by antibody-antigen recognition reaction.
Through detecting Harpin
CSCS008Protein has following main biological function: (1) promotes growth and development of plants, improves output; (2) broad spectrum resistance of enhancing plant comprises the resistance to various bacteria, fungi and virus; (3) make the insect-repellent of plant acquisition to some harmful insect; (4) resistance of enhancing plant; (5) storage time of prolongation plant prod; (6) potted flower, nursery stock also had good plastotype effect.
Because Harpin
CSCS008Protein is strengthening plant disease-resistant, expelling parasite, degeneration-resistant and promote growth and improve good result aspect the output, it is environmentally friendly in addition, to people and animals bird fish nontoxicity, and can not cause the resistance of pathogen, also change that can inducing plant genetic construction (genomic dna), in environment, decompose, do not have residual public hazards easily, be expected to become the following first-selection that progressively substitutes the good environment protection biological product of high poison, high residue chemical pesticide and chemical regulator.At present various crops, vegetables, fruit, flowers and various economic plants are comprised that the disease-resistant expelling parasite of tens of kind of plant such as tobacco, tealeaves and short long effect of increasing production test and the product ratio widely with regard to it.Existing test-results shows Harpin
CSCS008Albumen is obvious to disease-resistant expelling parasite and the short long effect of increasing production of cucumber, tomato, potato, capsicum, tobacco, corn, strawberry etc., simultaneously to improve certain plants such as tobacco, quality of tea leaves also has good effect, and contrast effect is also very remarkable in similar Harpin product.Harpin
CSCS008Albumen can directly apply to growth and development of plant and regulate and the prevention and control of plant diseases, pest control, comprises the maintenance on food crop, economic plants, vegetables, fruit, flowers and gardens and grassland etc.; Using method has seed soaking, dresses seed, dips in root, seed pelleting, plant injection, foliage-spray, flowers and fruits spraying etc.; Using dosage is different because of using method and kind, and general 5 μ g/ml-80 μ g/ml are effective concentration; Use the back and promptly have an effect in 2-12 hour, sustainable about 20 days of drug effect, but season of growth medication 2-3 time.
Employed engineering bacteria E.coli JM109 (DE3) bacterial strain and hrpZ among the present invention
CSCS008The widespread use in molecular biology research and the medicine industry at home and abroad of efficient expression vector pET28a (+) plasmid of gene, environmentally safe reliable.
The shortenings that uses among the present invention: LB (bacteria culture medium, yeast powder 5g/L+ peptone 10g/L+NaCl10g/L, pH7.0); Km (kantlex); IPTG (isopropylthio-beta galactose glycosides); PMSF (phenylmethylsulfonyl fluoride); Tris (Tutofusin tris).
Embodiment
Embodiment 1 hrpZ
CSCS008The clone of gene and order-checking
(1) hrpZ
CSCS008Gene is from the bacillary tikka pseudomonas of tomato (Pseudomonas syringaepv.tomota) CSCS008 bacterial strain, and this gene is present on the chromosomal DNA of CSSY002 bacterial strain with hrpZ gene cluster form.The bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) CSCS008 bacterial strain is at first screened on the LB flat board, and this bacterial strain can be secreted xanthein, and under UV-light fluorescence takes place.(2) with the mono-clonal bacterium colony of choosing, under 28 ℃ in the LB liquid nutrient medium shaking culture 12 hours, centrifugal collection thalline, with the genomic dna separating kit separate, the purification of bacterial chromosomal DNA.(3) bacterial chromosomal dna partly digests through Sau3A, makes up the genomic library of the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) CSCS008 bacterial strain with plasmid vector pLARF5.(4) make molecular probe with the hrpZ gene of the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota) DC3000 bacterial strain, screen from the CSCS008 genomic library by clone hybridization and differentiate hrpZ
+Plasmid obtains to comprise the 2.0kb DNAs fragment of the whole coding region of hrpZ gene, and further this fragment subclone is advanced in the pBluescript carrier.(5) carry out nucleotide sequencing with general T7 primer, wherein have the reading frame (reading frame) of a 1113bp to be hrpZ
CSCS008The coding region of gene, sequence such as SEQ ID No.1.
Embodiment 2 Harpin
CSCS008Proteinic preparation and purifying
Strain preparation and large scale fermentation (1) preparation original seed: will have hrpZ
CSCS008Engineering bacteria E.coli JM109 (DE3) bacterial strain of gene efficient expression plasmid pET28a (+) is rule 37 ℃ of overnight incubation on the inclined-plane of glycerine-LB+Km20 μ g/ml.(2) preparation is female plants: well-grown mono-clonal colony inoculation on the original seed inclined-plane is shaken in the bottle in the 250ml that is added with 100ml glycerine-LB+Km20 μ g/ml, in 37 ℃ of 110rpm shaking culture 12h.(3) preparation is produced kind: mother is planted bacterium liquid be inoculated in by 1% volume ratio in the 5L fermentor tank that is added with 3L glycerine-LB+Km25 μ g/ml, cultivate 12h under 37 ℃ of 110rpm and the 0.5L/min air flow condition.(4) large scale fermentation: after the fermentor tank more than the 50L being added the Km of the glycerine-LB of 70% volume and final concentration 40 μ g/ml, in-situ sterilization 30min (120 ℃, 1.1MPa); Insert the seeding bacterium by 1% volume ratio then, 37 ℃ of 200rpm and 1L/min air flow condition bottom fermentation are cultivated; After treating that bacterium enters logarithmic phase (OD600=0.7), regulate rotating speed and air flow, to guarantee yeasting competent oxygen supply (DO>30%) is arranged, and carry out logarithm feed supplement by stages by specific program; Before the bacterium logarithmic phase finishes 1-2 hour, by millipore filtration adding inductor IPTG to final concentration 1mM; Continue to induce fermentation 4-6 hour, can play jar.This method can realize the high-density or the high-efficient culture of engineering bacteria.
Harpin
CSCS008Proteinic preparation and purifying Harpin
CSCS008Protein mainly exists with inclusion body (inclusion body) form in Bacillus coli cells.Industrial scale operation Harpin
CSCS008During albumen, adopt the broken preparation of 8M urea.In the laboratory in order to obtain further Harpin
CSCS008The pure product of protein matter, can operate by follow procedure: centrifugal (5,000rpm, 10min) 4-6 hour Bacillus coli cells is induced in collection through IPTG, after the abundant suspension of 20mMTris damping fluid (pH9.0), add the N,O-Diacetylmuramidase (100mg/ml) of 10 μ l/25ml, ice bath 10min, add 0.5ml/25mlPMSF (20mg/ml), the broken 10min of ultrasonic wave (20KHz) adds the PMSF of 0.5ml/25ml again, ultrasonic disruption 10min again behind the mixing, 10, the centrifugal 10min of 000rpm gets supernatant liquor in 100 ℃ of water-bath 10min, cooling back 12, the centrifugal 10min of 000rpm collects supernatant liquor.The Harpin that promptly contains higher degree in this supernatant liquor
CSCS008Protein, concentration reach 3600 μ g/ml.
Embodiment 3 Harpin
CSCS008Proteinic using method
Harpin
CSCS008Protein method in the use is various, can be because of handling the different differences to some extent of material, into treatment sites, treatment time and processing intent.Specifically can use by the method for following introduction:
(1) seed soaking: at first water is with Harpin
CSCS008Protein is made into the concentration of 30-60 μ g/ml, then seed is dipped in wherein 8-12 hour.Suitable crop or the vegetable seed of doing vernalization of this method.After seed soaking finishes, with seed from Harpin
CSCS008Take out in the protein seed-soaking liquid, can vernalization or sowing.Emerge after a week, the height of seedling comparison is according to increasing more than 10%, and increment also improves more than 10%, and seedling stage anti-samping off ability also obviously strengthen.
(2) seed dressing: seed is moistening a little, the Harpin of adding grain weight 0.1%
CSCS008Protein formulation is fully mixed the back sowing thoroughly.The neat seedling of back seedling of emerging is strong, strengthens the ability of anti-samping off in seedling stage.
(3) dip in root: be suitable for transplanting the crop that grows surely, as melon and fruit, vegetables, cotton, corn etc.At first with Harpin
CSCS008Protein formulation is made into the aqueous solution of 30 μ g/ml, and the root that will be transplanted crop seedling then was immersed in this solution 1-2 hour.After the transplanting, plant recovers growth soon, and transplanting seedling time shortens, and the plant growing way is powerful.
(4) foliar spray: the whole growth of crop all can spray season.With Harpin
CSCS008Protein formulation is made into the aqueous solution of 15-20 μ g/ml, in seedling stage of crop, tillering phase, initial bloom stage, fruit phase or the filling stage use of spraying just.General sprayable 2-3 time of crop growing season.After the spraying, can improve crop alimentary bulk-growth amount 15-30%, improve output 10-20%, and whole growth can save the chemical pesticide more than 80% season.Some crop such as cucumber can be kept out 60% gray mold, the mosaic virus that tobacco can be kept out 60-80%.Also have certain degeneration-resistant (drought resisting, cold-resistant, salt tolerant alkali etc.) and anthelminthic effect in addition.
Embodiment 4 hrpZ
CSCS008The related application of gene
(1) with gene recombination technology with hrpZ
CSCS008Gene clone is advanced in the Ti-plasmids carrier of anti-kantlex, forms hrpZ
CSCS008-Ti-plasmids; (2) use hrpZ
CSCS008-Ti-plasmids transforms agrobatcerium cell, and screening contains hrpZ
CSCS008The positive expression Agrobacterium of-Ti-plasmids; (3) the Radix Dauci Sativae protoplastis that will be in regeneration wall period with contain hrpZ
CSCS008The Agrobacterium of-Ti-plasmids was cultivated 36-48 hour together altogether, and centrifuge washing goes containing the carrot cell clone that screening transforms on the selection substratum of kantlex behind the bacterium; (4) carrot cell that transforms is cloned in cultivates into regeneration plant on the division culture medium, promptly obtain Radix Dauci Sativae hrpZ
CSCS008The gene transgenic plant, this transfer-gen plant with do not change hrpZ
CSCS008The Radix Dauci Sativae regeneration plant of gene is compared, and has obvious growth advantage and anti-soft rot characteristic.
Embodiment 5 hrpZ
CSCS008The application of gene-correlation genetic recombination body
(1) with gene recombination technology with hrpZ
CSCS008Gene and hrpN
EaGene fusion forms hrpZ
CSCS008-hrpN
EaFusion gene; (2) with hrpZ
CSCS008-hrpN
EaFusion gene cloning advances among the efficient expression plasmid carrier pETa (+) of anti-kantlex, forms hrpZ
CSCS008-hrpN
Ea-pETa (+) plasmid; (3) use hrpZ
CSCS008-hrpN
Ea-pETa (+) plasmid transforms engineering bacteria JM 109 (DE3), selects to depress screening and contains hrpZ adding kantlex
CSCS008-hrpN
EaThe positive expression bacterial strain of-pETa (+) plasmid; (4) the fusion rotein Harpin that expresses with this fusion gene of fermentative Production
CSCS008-Harpin
Ea, and by SDS PAGE detection Expression of Fusion Protein situation, thereby obtain the stronger and wider Harpin of sphere of action of biologic activity
CSCS008Class fusion rotein exciton.
Embodiment 6 Harpin
CSCS008Proteinic applicating example
Tens of kinds of crops, vegetables, fruit, flowers have been made Harpin at present
CSCS008Proteinic application effect test, though the performance degree is different on the Different Crop kind, Harpin
CSCS008The effect of aspects such as proteinic short long volume increase, disease-resistant expelling parasite, raising resistance and potted flower, nursery stock plastotype is significant.Lifting several examples below is illustrated:
(1) corn: choose 4 leaf phase maize seedling fields of two 5 fens ground sizes, be used separately as contrast and treatment samples piece.Treating piece is the Harpin with 15-20 μ g/ml in 4 leaf phases and 6 leaf phases respectively
CSCS008Protein soln has been made foliar spray, does not use any agricultural chemicals in addition, and the management of others is the same with the contrast piece.Find that in process of the test in a week after the medication, the average plant height comparison for the treatment of piece exceeds 10-15cm according to piece, the corn northern and southern leaf blight sickness rate is also compared according to the low 20-30% of piece; Treating piece is bloomed to compare according to piece and is shifted to an earlier date 5-10 days simultaneously, and the filling stage, two luxuriant rates were apparently higher than contrast.The results back is output relatively, and the treating piece comparison is shone the piece volume increase more than 12%.
(2) cucumber: choose 3 leaf phase cucumber seedling fields of two 5 fens ground sizes, be used separately as contrast and Harpin
CSCS008Protein treatment samples piece, the Harpin of processing seedling canopy
CSCS008The concentration of albumen treatment solution is 20 μ g/ml.Treating piece carried out foliar spray in 3 leaf phases, 5 leaf phases and 7 leaf phases, and other management is with contrast.Test-results shows: Haprin
CSCS008The protein treating piece is bloomed comparison according to having shifted to an earlier date 8 days; The mosaic disease comparison is according to having reduced 65%; The comparison of grey mold handle is according to having reduced 30%; Yield increased has increased more than 23%.
(3) strawberry: choose 3 leaf phase of the wing-rooms on either side of a one-story house strawberry seedling canopy of about 2 minutes ground sizes, compare respectively and Harpin
CSCS008Protein treatment samples piece.Handle the Harpin of seedling canopy
CSCS008The concentration of albumen treatment solution is 20 μ g/ml.3 leaf phases began foliar spray, and later every interval sprayed once in 15 days, amounted to 5 times.The result shows that the comparison of processing canopy is done sth. in advance about 10 according to canopy and bloomed; Individual plant flower, the contrast of fruit rate average specific increase 2-3; The gray mold incidence obviously is less than contrast; The fresh fruit colour generation is good, the fruit type is excellent, the malformed fruit rate is low, and yield increased is increased production more than 25%.In addition, weigh, find that the dry-matter accumulation of processing canopy is also compared according to increasing 1-2% by the equivalent fresh fruit is dried.
(4) Cyclamen persicum: Cyclamen persicum is the potted flower kind that liked by masses, but the mortality ratio that caused by bacterial soft rot is very high, dormancy during high temperature, and also due to illness the abnormal leaf, the flower that cause of viral disease had a strong impact on its ornamental value and commercial value.We have chosen 400 basin 3-4 monthly age Cyclamen persicums and have done to be divided into two groups at random for the examination material, compare respectively and Harpin
CSCS008Protein is handled.Harpin
CSCS008The working concentration of albumen treatment solution is 20 μ g/ml.Treatment process is a foliar spray, sprays once in every interval 10-15 days.The result shows, after one week of medication, the leaf look of treatment group deepens, glossy, and that plant type also obviously becomes is tall and straight, compact, live and take off, and can break the high temperature dormancy; After the medication one month, viral disease and spire that deformity is curled begins to be extended into gradually normal morphology due to illness in the past, the spire of the control group more and more deformity that then becomes, the petal of leaving also is deformity and twists.In addition, Harpin
CSCS008Protein also has certain effect of driveing to the trialeurodes vaporariorum on the Cyclamen persicum blade.
(5) tobacco: Harpin
CSCS008Albumen is to the property killed of plant harmful insect.Tobacco is the aphid susceptible plants.Harpin with 25 μ g/ml concentration
CSCS008Protein formulation was soaked seed 24-48 hour to tobacco seed under the 250C condition, and compare seed soaking with the 5mM potassium phosphate buffer of pH6.5 and handle, be sowed at respectively then in three culture plates and sprout, grouping is transplanted in same big Tanaka after waiting to emerge, subsequently the number of observed and recorded infection every day aphid.Found that the mean number of control treatment group individual plant infection in the 1st, 2,3,6,7,8,9,10 days aphid is respectively: 0,3,3,6,7,9,13,17; Harpin
CSCS008The mean number of albumen treatment group individual plant infection in the 1st, 2,3,6,7,8,9,10 days aphid is respectively: 0,0,0,1,0,0,2,2.
(6) African Flower of Garden Balsam: Harpin
CSCS008Albumen improves the resistance of plant.The Africa Flower of Garden Balsam is a kind of common showy flowers of herbaceous plants of viewing and admiring.Get the African Flower of Garden Balsam of 10 basin growth potential basically identicals, divide to deal with and contrast 2 groups, every group 5 basin, treatment group and control group are used the Harpin of 25 μ g/ml concentration respectively
CSCS008Protein formulation and water carry out foliar spray, spray altogether 2 times, and each 7 days at interval, other management condition unanimity.After treating 15 days, 2 groups of materials are stopped water and fertilizer management (promptly stopping to water and applying fertilizer), found that after 15 days, the control group plant begins to occur withered and yellow withered, the mosaic virus outburst, and mosaic virus does not take place in treatment group plant growing way health.
(7) Harpin
CSCS008The storage time that albumen prolongs the crop product is got 100 of the fresh strawberries of firm collection, becomes to handle and contrasts 2 groups by 50 1 components, and treatment group is with 30 μ g/ml Harpin
CSCS008Protein solution soaked 10 minutes, and control group is contained in respectively in 2 ventilative corbeils then with pure water logging 10 minutes, above coated with gauze, placed for 1 week under the room temperature, the result shows that the control group strawberry is softening more than 90%, color is dun, wherein 10% seriously goes rotten, and treatment group strawberry 90% above color is vivid, and the fruit grain is tender and crisp, have only several grains to darken, the deliquescing of fruit grain.
Sequence table
<110〉Pairun Biological Science and Technology Co., Ltd., Chengdu
<120〉the hrpZ gene of a kind of multifunctional activity of coded plant and broad spectrum resistante cell singal gene and expression product and application
<160>2
<170>PatentIn?Version?2.1
<210>1
<211>1113
<212>DNA
<213〉the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota)
<221>1-1113
<400>1
1 atgcaagcac?ttaacagcat?cagttcgttg?caaacctctg?catcattgtt?ccccgtgtcg
61 ctcaacagcg?atgtgagcgc?caacaccagc?acttccagca?aagagctcaa?ggctgtgatc
121 gatcagctgg?ttcaggcgct?gacccaaagt?gggcagctcg?atgaaacctc?accgctcggc
181 aaaatgctcg?ccaaggccat?ggctgcggat?ggcaagtcgg?ctaacagcat?cgatgacatc
241 actgcatcgc?tcgacaagct?gatccacgaa?aagctcggcg?acaatttcgg?tgcctctgcc
301 ggcatcggcg?cgggtggcgg?tggcggtggc?attggcgggg?cgggttctgg?ttcgggtgtc
361 ggtggcggtc?tgagcagcga?cgcgggtgcc?gggcaatccg?atctgatgag?ccaggtcctg
421 aacggcctcg?gcaaagccgt?gctggacgat?ctgctgacac?cgagtggtga?aggcggaaca
481 accttttcca?gtgatgacat?gccgaccctg?gaaaaagtcg?cccagttcat?ggacgacaac
541 aaggcccagt?tccctactcg?ggacggcggc?tcgtggatga?acgagctgaa?ggaagacaat
601 ggcctggatg?cacaggaaac?cgctcagttt?cgttcggctc?tcgacgtcat?tggtcaacag
661 ctcggccagc?aacaaggtga?tgccagtggc?gttaccagtg?gcggcggtct?gggttcgccc
721 gtgagtgaca?gctccctggg?taatcctgca?atcgatgcca?acacaggtcc?cgcggccaat
781 ggcaatgcca?gcgtcgacgt?aggtcaactg?atcggtcaac?tcatcgaccg?tggtttgcag
841 tcggtttcgt?cgggtggcgg?tctgggtaca?ccggtcgaca?attccacgca?gccgacaggt
901 ggcacgccag?cggctaaccc?gacgggcaac?gtgtccaatc?aggacctggg?tcaactgctg
961 agcggcttgc?tgcaacgcgg?gctggaagcg?acgcttcagg?atgctggcaa?caccggcgcc
1021?gacctgcaat?cgagcgctgc?gcaagtggca?gctcagctga?tcaatgcgct?gttgcaaggc
1081?accaataacc?agactaacca?ggctgtggcc?tga
<210>2
<211>370
<212>PRT
<213〉the bacillary tikka pseudomonas of tomato (Pseudomonas syringae pv.tomota)
<400>2
Met?Gln?Ala?Leu?Asn?Ser?Ile?Ser?Ser?Leu?Gln?Thr?Ser?Ala?Ser?Leu
1 5 10 15
Phe?Pro?Val?Ser?Leu?Asn?Ser?Asp?Val?Ser?Ala?Asn?Thr?Ser?Thr?Ser
20 25 30
Ser?Lys?Glu?Leu?Lys?Ala?Val?Ile?Asp?Gln?Leu?Val?Gln?Ala?Leu?Thr
35 40 45
Gln?Ser?Gly?Gln?Leu?Asp?Glu?Thr?Ser?Pro?Leu?Gly?Lys?Met?Leu?Ala
50 55 60
Lys?Ala?Met?Ala?Ala?Asp?Gly?Lys?Ser?Ala?Asn?Ser?Ile?Asp?Asp?Ile
65 70 75 80
Thr?Ala?Ser?Leu?Asp?Lys?Leu?Ile?His?Glu?Lys?Leu?Gly?Asp?Asn?Phe
85 90 95
Gly?Ala?Ser?Ala?Gly?Ile?Gly?Ala?Gly?Gly?Gly?Gly?Gly?Gly?Ile?Gly
100 105 110
Gly?Ala?Gly?Ser?Gly?Ser?Gly?Val?Gly?Gly?Gly?Leu?Ser?Ser?Asp?Ala
115 120 125
Gly?Ala?Gly?Gln?Ser?Asp?Leu?Met?Ser?Gln?Val?Leu?Asn?Gly?Leu?Gly
130 135 140
Lys?Ala?Val?Leu?Asp?Asp?Leu?Leu?Thr?Pro?Ser?Gly?Glu?Gly?Gly?Thr
145 150 155 160
Thr?Phe?Ser?Ser?Asp?Asp?Met?Pro?Thr?Leu?Glu?Lys?Val?Ala?Gln?Phe
165 170 175
Met?Asp?Asp?Asn?Lys?Ala?Gln?Phe?Pro?Thr?Arg?Asp?Gly?Gly?Ser?Trp
180 185 190
Met?Asn?Glu?Leu?Lys?Glu?Asp?Asn?Gly?Leu?Asp?Ala?Gln?Glu?Thr?Ala
195 200 205
Gln?Phe?Arg?Ser?Ala?Leu?Asp?Val?Ile?Gly?Gln?Gln?Leu?Gly?Gln?Gln
210 215 220
Gln?Gly?Asp?Ala?Ser?Gly?Val?Thr?Ser?Gly?Gly?Gly?Leu?Gly?Ser?Pro
225 230 235 240
Val?Ser?Asp?Ser?Ser?Leu?Gly?Asn?Pro?Ala?Ile?Asp?Ala?Asn?Thr?Gly
245 250 255
Pro?Ala?Ala?Asn?Gly?Asn?Ala?Ser?Val?Asp?Val?Gly?Gln?Leu?Ile?Gly
260 265 270
Gln?Leu?Ile?Asp?Arg?Gly?Leu?Gln?Ser?Val?Ser?Ser?Gly?Gly?Gly?Leu
275 280 285
Gly?Thr?Pro?Val?Asp?Asn?Ser?Thr?Gln?Pro?Thr?Gly?Gly?Thr?Pro?Ala
290 295 300
Ala?Asn?Pro?Thr?Gly?Asn?Val?Ser?Asn?Gln?Asp?Leu?Gly?Gln?Leu?Leu
305 310 315 320
Ser?Gly?Leu?Leu?Gln?Arg?Gly?Leu?Glu?Ala?Thr?Leu?Gln?Asp?Ala?Gly
325 330 335
Asn?Thr?Gly?Ala?Asp?Leu?Gln?Ser?Ser?Ala?Ala?Gln?Val?Ala?Ala?Gln
340 345 350
Leu?Ile?Asn?Ala?Leu?Leu?Gln?Gly?Thr?Asn?Asn?Gln?Thr?Asn?Gln?Ala
355 360 365
Val?Ala *
370
Claims (10)
1. the hrpZ gene of multifunctional activity of coded plant and broad spectrum resistante cell singal gene, it is characterized in that: the nucleotide sequence of this gene is the SEQ ID No.1 in the sequence table.
2. the hrpZ gene of multifunctional activity of coded plant as claimed in claim 1 and broad spectrum resistante cell singal gene is characterized in that: this gene is from the bacillary tikka pseudomonas of tomato (Pseudomonassyringae pv.tomota) bacterial strain.
3. the genetic recombination body that contains claim 1 or 2 described hrpZ genes.
4. hrpZ gene as claimed in claim 1 or 2 is grown the Agricultural biotechnologies breeding relevant with prevention and elimination of disease and pests, the application aspect the transgenic plant in coordinate plant growth.
5. hrpZ gene as claimed in claim 1 or 2 is in the application of following either side: (1) promotes growth and development of plants; (2) broad spectrum resistance of plant comprises the resistance to various bacteria, fungi and virus; (3) insect-repellent of plant; (4) resistance of plant improves plant to comprising the tolerance of arid, severe cold, poor environment such as saline and alkaline; (5) storage time of prolongation crop product; (6) to the plastotype effect of potted flower, nursery stock.
6. genetic recombination body as claimed in claim 3 is grown the Agricultural biotechnologies breeding relevant with prevention and elimination of disease and pests, the application aspect the transgenic plant in coordinate plant growth.
7. the Harpin protein of the hrpZ genes encoding of multifunctional activity of coded plant and broad spectrum resistante cell singal gene, it is characterized in that: this protein has the aminoacid sequence of SEQ ID No.2 in the sequence table, has following attribute: (1) has 370 amino-acid residues; (2) molecular weight 36.52kda; (3) iso-electric point pI:4.01; (4) glycine Gly lacks halfcystine Cys; (5) tolerance still had activity in 10-15 minute in 100 ℃ of boiling water; (6) there is not quaternary structure.
8. contain the proteinic biological products of the described Harpin of claim 7.
9. Harpin protein as claimed in claim 7, in the application of following either side: (1) promotes growth and development of plants; (2) broad spectrum resistance of plant comprises the resistance to various bacteria, fungi and virus; (3) insect-repellent of plant; (4) resistance of plant improves plant to comprising the tolerance of arid, severe cold, poor environment such as saline and alkaline; (5) storage time of prolongation crop product; (6) to the plastotype effect of potted flower, nursery stock.
10. the proteinic biological products of Harpin as claimed in claim 8, in the application of following either side: (1) promotes growth and development of plants; (2) broad spectrum resistance of plant comprises the resistance to various bacteria, fungi and virus; (3) insect-repellent of plant; (4) resistance of plant improves plant to comprising the tolerance of arid, severe cold, poor environment such as saline and alkaline; (5) storage time of prolongation crop product; (6) to the plastotype effect of potted flower, nursery stock.
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Cited By (3)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
CN108264565A (en) * | 2016-12-30 | 2018-07-10 | 四川本原作物科技有限公司 | Chitosan-modified Hrps electrostatic self-assembled trimeric polypeptides and preparation method thereof |
CN108264564A (en) * | 2016-12-30 | 2018-07-10 | 四川本原作物科技有限公司 | Zn++Covalent trimeric polypeptides of Hrps modified with maltodextrin pair and preparation method thereof |
CN114681591A (en) * | 2020-12-31 | 2022-07-01 | 吴伯骥 | Application of HrpZpss protein in identifying and activating multiple types of receptors and/or membrane proteins and signal pathways thereof in pharmacy |
-
2005
- 2005-04-29 CN CN 200510020814 patent/CN1858207A/en active Pending
Cited By (3)
Publication number | Priority date | Publication date | Assignee | Title |
---|---|---|---|---|
CN108264565A (en) * | 2016-12-30 | 2018-07-10 | 四川本原作物科技有限公司 | Chitosan-modified Hrps electrostatic self-assembled trimeric polypeptides and preparation method thereof |
CN108264564A (en) * | 2016-12-30 | 2018-07-10 | 四川本原作物科技有限公司 | Zn++Covalent trimeric polypeptides of Hrps modified with maltodextrin pair and preparation method thereof |
CN114681591A (en) * | 2020-12-31 | 2022-07-01 | 吴伯骥 | Application of HrpZpss protein in identifying and activating multiple types of receptors and/or membrane proteins and signal pathways thereof in pharmacy |
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