CN113604477B - Lilium regale defensin antibacterial peptide gene LrDEF1 and application thereof - Google Patents

Lilium regale defensin antibacterial peptide gene LrDEF1 and application thereof Download PDF

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CN113604477B
CN113604477B CN202110957485.3A CN202110957485A CN113604477B CN 113604477 B CN113604477 B CN 113604477B CN 202110957485 A CN202110957485 A CN 202110957485A CN 113604477 B CN113604477 B CN 113604477B
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刘迪秋
王自娥
梁婷婷
邓婕
苏琳琳
陈虹均
葛锋
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Kunming University of Science and Technology
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    • C12N15/8282Phenotypically and genetically modified plants via recombinant DNA technology with agronomic (input) traits, e.g. crop yield for stress resistance, e.g. heavy metal resistance for biotic stress resistance, pathogen resistance, disease resistance for fungal resistance

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Abstract

The invention discloses a Lilium regale defensin antibacterial peptide geneLrDef1The nucleotide sequence is shown as SEQ ID NO. 1, and the protein with the amino acid sequence shown as SEQ ID NO. 2 is coded, and the invention is proved by related technical research of functional genomicsLrDef1The gene has the function of improving the antifungal effect of plants, and the invention is antifungalLrDef1The gene is constructed on a plant expression vector and is transferred into tobacco for over-expression, a transgenic tobacco plant has strong capability of resisting fungal infection, and the experimental result shows that the over-expression is realizedLrDef1The transgenic tobacco has high-level resistance to infection by fusarium oxysporum, phoma herbarum and fusarium equiseti.

Description

Lilium regale defensin antibacterial peptide gene LrDEF1 and application thereof
Technical Field
The invention relates to the technical field related to molecular biology and genetic engineering, in particular to a Lilium regale defensin antibacterial peptide gene with antifungal infection capacityLrDef1And application thereof.
Background
Pathogenic bacteria are important influencing factors causing loss of plant yield and quality, and plant diseases caused by the pathogenic bacteria can reduce the yield of crops by 20-40%; wherein the fungal diseases are the largest number of plant diseases, and account for about 70-80% of the total number of the diseases. The traditional method for controlling plant diseases mainly uses chemical pesticides, improves cultivation management measures and cultivates new resistant varieties. Although the methods have certain effect, the traditional breeding period is long, the effect of cultivation measures is poor, and pesticides are easy to cause the problems of environmental safety, food safety and the like. With the rapid development of biotechnology, the new disease-resistant variety cultivated by using a genetic engineering method can overcome the defects of the prevention and treatment method, reduce the damage to beneficial microorganisms in soil to the maximum extent and realize the sustainable development of agriculture.
Plant Antimicrobial peptides (AMPs) are small, cysteine-rich, basic cationic peptides that are part of the plant immune system, have inhibitory or killing effects on pathogenic microorganisms such as bacteria, fungi, and viruses, and play a crucial role in plant defense reactions (Zasloff Michael, antimicrobial peptides of multicell organisms. Nature, 2002, 415 (6870): 389-395). Plant defensins are important AMPs, and when plants are subjected to biotic stress, the plant defensins can be combined with specific characteristic membrane components of fungi to cause the cell membranes of pathogenic bacteria to be sunken, embedded into the cell membranes or transported into the cell membranes, so that a series of biochemical changes are generated.
Various defensin genes have been introduced into plants for enhancing plant resistance. Tobacco (A)Nicotiana megalosiphon) Defensins (A)NmDef02) Is a common plant defensin with antibacterial activity, and expressesNmDef02Turn of (2)Gene soybean (A)Glycine max) Plant rust of soybean: (Phakopsora pachyrhizi) And anthrax bacteria (B)Colletotrichum truncatum) Show a higher resistance (Soto N, Y Hern ndz, delgado C, et al. Field resistance toPhakopsora pachyrhizi and Colletotrichum truncatumof transgenic soybean expressing the NmDef02Plant defenses gene, frontiers in Plant Science, 2020, 11: 562). In tobacco (A), (B)N. alata) Separating to obtain a flower budNaD1The content of the defensin is as follows,NaD1can be specifically combined with fungal Cell walls and enter fungal cytoplasm to trigger The rapid increase of intracellular active oxygen concentration, so that The cytoplasmic membrane of The fungi is permeabilized, and finally The fungal Cell Death is caused (Baxter AA, poon IK, hulett MD. The plant defensen NaD1 indens Cell Death, cellular processing, cell Death Discovery, 2017, 3 (1): 402-410). In addition, the NaD1 protein is specific to Fusarium oxysporum (F.), (II.), (III.) the proteinFusarium oxysporum) A Botrytis cinerea (A. Cinerea: (B.))Botrytis cinerea) Candida, andCandida albicans) The like has good antibacterial activity (Luo Xianlin, zhao Degang, zhao Yichen. Floral tobacco)NaD1Prokaryotic expression and purification of gene molecular plant breeding 2020, 18 (11): 3502-3508).
The Bulbus Lilii is Liliaceae (Liliaceae) Lilium (Lilium)Lilium) The plant is a general term of perennial root flowers. During the processes of seed ball propagation and fresh cut flower production, lily is vulnerable to various pathogenic bacteria such as fungi, viruses and bacteria. The lily diseases found at present are more than dozens, wherein the sickle belongs toFusarium spp.) blight caused by fungi (also known as basal rot, stem rot) is the most serious disease in lily production. After the fusarium infects the lily bulbs, the basal disc is necrotic, and the scales are rotted and fall off, so that the quality of the bulbs is reduced; after the plants are infected with fusarium, the leaves turn yellow and droop wilting, and the plants die in advance, so that the yield and the quality of cut lily flowers are seriously influenced; wherein, the fusarium oxysporum has the strongest pathogenicity and the highest separation frequency and is the main pathogenic bacterium of the lily wilt. Lilium regale (Lilium regale)L. regale Wilson) is peculiar to ChinaThe seeds are only distributed in rock cracks from valleys with the altitude of 800-2700 m in Minjiang river basin to the mountains, have strong blight resistance and are important germplasm resources for modern lily breeding. The antibacterial peptide is an important component of a plant defense system, so that the antibacterial peptide has important research and application values on the discovery and functional analysis of the antibacterial peptide gene in Lilium regale.
Disclosure of Invention
The invention aims to provide a Lilium regale defensin antibacterial peptide geneLrDef1And application thereof, namely, the application of the composition in improving the resistance of tobacco to fusarium oxysporum (F)F. oxysporum) Phoma graminearum (A) and (B)Phoma herbarum) Fusarium equiseti (F.) hand. -Mazz: (F.), (F. equiseti) Use in resistance.
The defensin antibacterial peptide gene with antifungal activity, which is cloned from Lilium regaleLrDef1LrDef1The nucleotide sequence is shown as SEQ ID NO. 1, the gene cDNA full length sequence is 501bp, comprises a 225bp open reading frame, a 5 'untranslated region of 37 bp and a 3' untranslated region of 239 bp, and codes protein of the amino acid sequence shown as SEQ ID NO. 2.
In the inventionLrDef1The coding region of the gene is a nucleotide sequence shown in 38 th to 262 th sites in a sequence table SEQ ID NO. 1.
The invention separates and clones a complete cDNA segment of an antifungal related gene of Lilium regale, and utilizes agrobacterium tumefaciens (A), (B) and (C)Agrobacterium tumefaciens) The target gene is transferred into a receptor plant by mediation and is over-expressed, whether the gene has antifungal activity is verified by further experiments, a foundation is laid for the capability of improving tobacco and other plants to resist fungal diseases by utilizing the gene in the later period, and the inventor names the gene asLrDef1
As described aboveLrDef1The gene can be applied to improving the antifungal property of tobacco, and the specific operation is as follows:
(1) Using amplificationLrDef1The specific primer of (2) is used for extracting total RNA from Lilium regale roots inoculated with fusarium oxysporum and amplifying the total RNA by reverse transcription-polymerase chain reaction (RT-PCR)LrDef1Full length braidConnecting the code region to pGEM-T carrier, and obtaining clone with target gene through sequencing;
(2) Using restriction endonucleasesEcoRI andBamh I enzyme digestion pGEM-T-LrDef1Vector, obtaining target gene fragment by glue recovery, using same endonuclease to enzyme-cut plant expression vector pCAMBIA2300s, obtaining required vector large fragment by glue recovery, and obtaining the obtained vector large fragmentLrDef1Connecting the gene fragment with the pCAMBIA2300s fragment to construct a plant overexpression vector, and then transferring the constructed recombinant vector into tobacco to express through the mediation of agrobacterium tumefaciens;
(3) Screening transformants by using a resistance marker on the recombinant vector T-DNA, obtaining a real transgenic plant through PCR and RT-PCR detection, analyzing the inhibition capability of total protein of a transgenic plant leaf on the growth of pathogenic fungi, and finally screening the transgenic plant with obviously enhanced resistance to the fungi.
The invention provides a new method for improving the resistance of plants to fungal diseases, the defects of traditional breeding can be overcome by cultivating disease-resistant plants by means of genetic engineering, the breeding period is shortened, the operation is simple, and high-resistance materials are easy to obtain. The invention is derived from Lilium regaleLrDef1The gene can enhance the resistance of plants to fungi, and the gene is introduced into tobacco, so that new varieties and new materials with fungal resistance can be generated; the method has obvious advantages and irreplaceable importance when the genetic engineering technology is utilized to culture resistant plant varieties and materials; the invention not only can provide convenience for large-scale production of crops, medicinal materials, horticultural plants and the like, greatly reduces the use of chemical pesticides, but also can save the cost for agricultural production and reduce the environmental pollution, thereby having wide market application prospect.
Drawings
FIG. 1 is a drawing of the present inventionLrDef1A PCR detection result graph of transgenic tobacco genome DNA, wherein: the Marker is DL2000 DNA Marker (Dalibao biology); the positive control is plasmid pGEM-T-LrDef1PCR product as template; WT is the product of PCR using total DNA of non-transgenic tobacco (wild type) as template;
FIG. 2 shows the positivity of the present inventionLrDef1In transgenic tobaccoLrDef1A graph of the results of expression analysis at the transcriptional level; in the figure: marker is DL2000 DNA Marker (Dalibao biology); WT is a PCR product with non-transgenic tobacco total RNA reverse transcription cDNA as a template; the positive control was plasmid pGEM-T-LrDef1PCR product as template;
FIG. 3 is a drawing of the present inventionLrDef1A bacteriostatic effect graph of the transgenic tobacco on the growth of pathogenic fungi in vitro; the fungi shown in panels a, b, c are Phoma herbarum: (P. herbarum) Fusarium equiseti (F.) hieron (F.)F. equiseti) Fusarium oxysporum (F.), (F. oxysporum) (ii) a WT was the wild type tobacco total protein and Buffer was the blank, i.e., no protein control (Buffer used to extract protein).
Detailed Description
The present invention is further illustrated by the following figures and examples, but the scope of the present invention is not limited to the above description, and the examples are conventional methods unless otherwise specified, and reagents used are conventional commercially available reagents or reagents formulated according to conventional methods unless otherwise specified.
Example 1:LrDef1gene cloning and sequence analysis
Inoculating Lilium regale with Fusarium oxysporum, extracting total RNA from roots inoculated with 24 h, grinding the inoculated Lilium regale roots into powder with liquid nitrogen, transferring into a centrifuge tube, extracting the total RNA by a guanidine isothiocyanate method, synthesizing a first cDNA chain by using reverse transcriptase M-MLV (promega) and using the total RNA as a template, wherein a reaction system and an operation process are as follows: mu.g of total RNA was taken and added with 50ng oligo (dT), 2. Mu.L dNTP (2.5 mM) and DEPC water in sequence to a reaction volume of 14.5. Mu.L; after uniformly mixing, heating and denaturing at 70 ℃ for 5min, rapidly cooling on ice for 5min, then sequentially adding 4 mu L of 5 XFirst-stand buffer, 0.5 mu L of RNase (200U) and 1 mu L M-MLV (200U), uniformly mixing and centrifuging for a short time, carrying out warm bath at 42 ℃ for 1.5h, taking out, heating at 70 ℃ for 10min, and stopping reaction; the first strand cDNA is synthesized and stored at-20 deg.C for further use.
Amplifying target gene using synthesized first strand cDNA as templateLrDef1The sequences of the used upstream and downstream primers are 5' TCGTCGTCCCCATCTCAG ' and 5' AAATACAAGAGAACTTACTCCA 3' is provided. Advantage is taken TM 2 PCR Enzyme (Clontech) to amplify the target gene; and (3) PCR reaction conditions: 5min at 94 ℃; 30s at 94 ℃, 30s at 54 ℃, 30s at 72 ℃ and 32 cycles; 7min at 72 ℃; the reaction system (20. Mu.L) was 0.5. Mu.L of cDNA, 2. Mu.L of 10 × Advantage 2 PCR Buffer, 0.4. Mu.L of 50 × dNTP Mix (10 mM each), 0.4. Mu.L of forward primer (10. Mu.M), 0.4. Mu.L of reverse primer (10. Mu.M), 0.4. Mu.L of Advantage 2 PCR Polymerase Mix, 15.9. Mu.L of PCR-Grade water; after the PCR was completed, 5. Mu.L of the resulting mixture was subjected to agarose gel electrophoresis to examine the specificity and size of the amplified product.
The PCR product was TA cloned using pGEM-T Vector System I (Promega, USA) as a kit, and the reaction System and procedure were as follows: mu.L of the PCR product was taken, and 1. Mu.L of pGEM-T Vector (50 ng/. Mu.L) and 2.5. Mu.L of 2 × Ligation solution I were sequentially added thereto, mixed well and then left to react at 16 ℃ overnight. The ligation product was transformed into E.coli DH 5. Alpha. Using a heat shock transformation method. Screening positive clones with LB solid medium containing ampicillin (Ampicillin, amp), selecting several single colonies, shaking, and amplifyingLrDef1Identifying the multiple cloning site insertLrDef1The clones identified are sequenced and finally obtainedLrDef1The full-length cDNA was 501bp, which was found to contain a 225bp open reading frame by NCBI ORF finder (http:// www.ncbi.nlm.nih.gov/gorf. Html) analysis (see sequence listing),LrDef1encodes a 74 amino acid protein with a molecular weight of about 8.06kDa and an isoelectric point of about 8.22. Analysis by means of bioinformatics software SignalP 5.0LrDef1The encoded protein sequence, and detecting whether the protein sequence has an N-terminal signal peptide. The results showed that a signal peptide was present at the N-terminus of LrDef1, and thus the protein was presumed to be a secreted protein.
Example 2: construction of plant overexpression vectors
The insertion is extracted by adopting a SanPrep column type plasmid DNA small extraction kit (Shanghai worker)LrDef1The E.coli plasmid pGEM-T-LrDef1And the plasmid of the plant expression vector pCAMBIA2300s, taking 1 mu L of the plasmid for agarose gel electrophoresis to detect the integrity and the concentration of the extracted plasmid; by restrictionEndonucleaseEcoRI (TaKaRa) andBamHI (TaKaRa) against plasmid pGEM-T-LrDef1And pCAMBIA2300s (100 mu L system), wherein the reaction system and the operation process are as follows: taking 20. Mu.L of pGEM-T-LrDef1And pCAMBIA2300s plasmid, 10. Mu.L of 10 XK buffer, 4. Mu.LEcoRI、6μL BamHI、60μL ddH 2 O, mixing uniformly, centrifuging for a short time, and reacting at 37 ℃ overnight; all the products of the digestion are spotted in agarose gel for electrophoresis, and thenLrDef1The fragments and the pCAMBIA2300s vector large fragment are respectively subjected to gel recovery, and a SanPrep column type DNA gel recovery kit (Shanghai Biotechnology) is used in the whole process; taking 1 microliter of the recovered product, detecting the size and concentration of the recovered fragment by agarose gel electrophoresis, and storing at-20 ℃ for later use.
Using T4 DNA Ligase (TaKaRa), recoveringLrDef1 The DNA fragment and the pCAMBIA2300s vector fragment were ligated, and the reaction system (20. Mu.L) and the procedure were as follows: taking 10 μ LLrDef1 The DNA fragment was sequentially added with 2. Mu.L of pCAMBIA2300s vector DNA, 2. Mu.L of 10 XT 4 DNA Ligase Buffer, 1. Mu. L T4 DNA Ligase, and 5. Mu.L of ddH 2 And O, mixing uniformly, centrifuging for a short time, and then carrying out water bath at 16 ℃ for overnight reaction. Then transferring the ligation product into Escherichia coli DH5 alpha by heat shock transformation, screening positive clone with solid culture medium containing 50mg/L kanamycin (Km), selecting single colony shake bacteria, and amplifying with bacteria liquid as templateLrDef1The specific primers of (1) are subjected to PCR, and selectedLrDef1And (3) if the detected bacterial strain is positive, adding glycerol and storing at-80 ℃ for later use.
Extracting and purifying pCAMBIA2300s-LrDef1Plasmid, then the plant expression vector pCAMBIA2300s-LrDef1Transferred into Agrobacterium tumefaciens LBA4404 competent cells. The operation steps are as follows: taking 2 μ g of pCAMBIA2300s-LrDef1Adding the plasmid into a centrifuge tube containing 200 μ L competent cells, gently mixing, performing ice bath for 5min, transferring into liquid nitrogen, freezing for 1min, rapidly placing in 37 deg.C water bath for 5min, immediately performing ice bath for 2min, adding 800 μ L LB liquid culture medium, performing shake culture at 28 deg.C for 4h; coating the activated agrobacterium with the coating solutionPerforming static culture at 28 ℃ on an LB solid culture medium containing 50mg/L Km; selecting single colony shake bacteria, and amplifyingLrDef1The specific primer of (1) is used for PCR to detect pCAMBIA2300s-LrDef1If the positive clone is transferred into agrobacterium, adding glycerol into the positive clone, and storing the positive clone at-80 ℃ for later use.
Example 3: agrobacterium-mediated genetic transformation of plants and transgenic plant screens
The transgenic recipient in this experiment was tobacco, tobacco seeds were soaked in 75% alcohol for 30s, washed with sterile water and then washed with 0.1% HgCl 2 Soaking for 8min, washing with sterile water for several times, sowing on 1/2 MS culture medium, dark culturing at 28 deg.C for 6d, germinating, transferring to light incubator (25 deg.C, 16 h/d light), and subculturing with 1/2 MS culture medium once a month.
Taking out the preserved materials containing pCAMBIA2300s from a-80 ℃ refrigeratorLrDef1Agrobacterium LBA4404 strain of plasmid was inoculated into 5mL LB liquid medium containing 50mg/L Km and 20mg/L rifampicin, and cultured at 28 ℃ until the medium became turbid. Sucking 1mL of turbid bacterial liquid to an LB solid culture medium containing 50mg/L Km, and culturing at 28 ℃ for 48 h; then, appropriate amount of the agrobacteria on LB solid medium was scraped and inoculated into MGL liquid medium supplemented with 20mg/L acetosyringone, and shake-cultured at 28 ℃ for 2-3h to activate the agrobacteria.
Cutting sterile tobacco seedling leaf into 1 cm 2 And completely soaking the left and right leaf discs in the MGL liquid culture medium containing the activated agrobacterium for 15min, sucking bacterial liquid on the surfaces of the leaves by using sterile filter paper, placing the leaf discs on a co-culture medium for room temperature culture, wherein the co-culture medium for tobacco transformation is MS +0.02 mg/L6-BA +2.1mg/L NAA +30g/L sucrose +6g/L agar, and co-culturing for 2 days at 22 ℃ in the absence of light.
Transferring the co-cultured leaf disc to an MS screening culture medium added with antibiotics to be divided into seedlings, and screening transgenic plants; the tobacco screening culture medium is MS +0.5 mg/L6-BA +0.1mg/L NAA +30g/L sucrose +6g/L agar +50mg/L Km +200 mg/L cephamycin (cefixime sodium salt, cef); during screening culture, the culture bottle is transferred to an illumination culture box for culture (25 ℃,16 h/d illumination, 8 h/d darkness), after the tobacco grows out of buds, the tobacco is subcultured by using an MS culture medium containing 50mg/L Km and 200mg/L Cef, and due to the fact that the callus differentiation rate of the tobacco is high, the regenerated plants need to be further screened, the tobacco regenerated seedlings are transferred to the MS culture medium containing 50mg/L Km to enable the tobacco regenerated seedlings to root, and finally the regenerated seedlings with good rooting are selected for further detection.
Extracting genome DNA of transgenic tobacco plant leaf by CTAB method, collecting 1 μ L of the extracted genome DNA, detecting its integrity and concentration by agarose gel electrophoresis, and amplifying with the genome DNA of transgenic plant as templateLrDef1After the PCR is finished, 8 mu L of the product is used for agarose gel electrophoresis to detect positive transgenic plants, the amplification result of part of transgenic tobacco is shown in figure 1, and 30 positive transgenic tobacco plants are screened out altogether.
Example 4: in transgenic tobaccoLrDef1Expression analysis of (3) and functional analysis of transgenic plants against fungal infection
Taking positive transgenic single plant and tender leaf of non-transgenic tobacco (wild type) to extract total RNA, reverse transcribing to generate cDNA first chain, and using it as template to make amplificationLrDef1The specific primers are used for carrying out PCR, and each transgenic individual is analyzed according to the PCR resultLrDef1The expression of transcription level, total RNA extraction and RT-PCR were performed as in example 1, after PCR was completed, 8. Mu.L of the DNA was applied to agarose gel electrophoresis, and the results of detection of some individuals were shown in FIG. 2, and 20 transgenic individuals were detectedLrDef1The expression was expressed in a large amount at the transcriptional level, and the numbers of these individuals were L1 to L20.
Several kinds of pathogenic fungi stored in a laboratory are inoculated on a PDA solid culture medium (200 g/L of potato, 15g/L of agar and 20g/L of glucose), dark culture is carried out at 28 ℃, plant protein is added when bacterial colonies grow to be about 2-3cm in diameter, and the in-vitro antifungal activity of transgenic plants is analyzed. In order to prevent other bacteria from polluting the extracted protein, the whole process of extracting the vegetable protein is aseptic operation. Firstly, 1g of single transgenic tobacco plant (numbered L-8, L-9 and L-16 respectively) and wild type leaves are put into a mortar, 1mL of protein extract (1M NaCL, 0.1M sodium acetate and 1% PVP, pH6.0) is added, and the mixture is fully ground. Transferred into a 1.5mL centrifuge tubeAfter mixing, the mixture was left to stand at 4 ℃ overnight. Centrifuge at 4 deg.C for 30min (12,000g/min), take the supernatant in a new 1.5mL centrifuge tube, and take an appropriate amount to measure the total protein concentration with an ultraviolet spectrophotometer. The total protein concentration of the transgenic and wild type plants was adjusted to 0.2. Mu.g/. Mu.L, and then 20. Mu.L of each was dropped onto sterile filter paper of each fungal culture. In addition to the total protein of the different transgenic tobacco plants, the total protein of the wild type tobacco and a blank (protein extract) were added in parallel to each fungal plate. The growth of the fungus was observed after several days of cultivation at 28 ℃ and evaluated therefromLrDef1The results of the in vitro antifungal activity of the transgenic tobacco are shown in FIG. 3,LrDef1the transgenic tobacco protein has obvious inhibition effect on the growth of fusarium oxysporum, phoma herbarum and fusarium equiseti.
Sequence listing
<110> university of Kunming science
<120> Lilium regale defensin antibacterial peptide gene LrDEF1 and application
<160> 4
<170> SIPOSequenceListing 1.0
<210> 1
<211> 501
<212> DNA
<213> Lilium regale Wilson
<400> 1
tcgtcgtccc catctcagtg gccgactatc tcttgcaatg gcgaagcttc ccaccatcct 60
gctgctcttg ttccttgtca tggccactga gatggggacg acgacggtgg aggcgaggac 120
atgcctgtcg cagagccaca agttcaaggg gacctgtttg agggcggcca actgtgctag 180
tgtctgccag acggagggat tcaaaggagg ggtttgcgag ggcatccgcc gccgttgctt 240
ctgcgaagcc gactgtcact gatgcctgag ttcttggctt taataagtaa tgtcggacta 300
tccgagaaga ataagatgga cctggtgttg ttggttttac agtctcttct tcggtgtggg 360
gactcggtac tttcatctag gtttctgata tgtagttgtt catgtctggg ttgagctgta 420
gggctgtgtg ctgtagttgg atttgtagtg gagtaagttc tcttgtattt gatttgtagt 480
ggagtaagtt ctcttgtatt t 501
<210> 2
<211> 74
<212> PRT
<213> Lilium regale Wilson
<400> 2
Met Ala Lys Leu Pro Thr Ile Leu Leu Leu Leu Phe Leu Val Met Ala
1 5 10 15
Thr Glu Met Gly Thr Thr Thr Val Glu Ala Arg Thr Cys Leu Ser Gln
20 25 30
Ser His Lys Phe Lys Gly Thr Cys Leu Arg Ala Ala Asn Cys Ala Ser
35 40 45
Val Cys Gln Thr Glu Gly Phe Lys Gly Gly Val Cys Glu Gly Ile Arg
50 55 60
Arg Arg Cys Phe Cys Glu Ala Asp Cys His
65 70
<210> 3
<211> 18
<212> DNA
<213> Artificial sequence (Artificial)
<400> 3
tcgtcgtccc catctcag 18
<210> 4
<211> 22
<212> DNA
<213> Artificial sequence (Artificial)
<400> 4
aaatacaaga gaacttactc ca 22

Claims (2)

1. Lilium regale defensin antibacterial peptide geneLrDef1The nucleotide sequence is shown in SEQ ID NO. 1.
2. Lilium regale defensin antibacterial peptide gene as claimed in claim 1LrDef1In improving the resistance of tobacco to fusarium oxysporum: (Fusarium oxysporum) Phoma graminearum (A) and (B)Phoma herbarum) Fusarium equiseti (F.) hieron (F.)Fusarium equiseti) Use in resistance.
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