CN103468719B - The RNA of a kind of high resistance TuMV and the RNAi carrier of this RNA of coding - Google Patents
The RNA of a kind of high resistance TuMV and the RNAi carrier of this RNA of coding Download PDFInfo
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Abstract
The invention discloses the RNA of a kind of high resistance TuMV and the RNAi carrier of this RNA of coding.The RNA of this high resistance TuMV has one of following nucleotide sequence: the nucleotide sequence shown in SEQ ID № .2 1) in sequence table; 2) with 1) the RNA sequence that limits has more than 90% homology, and has the RNA sequence of identical function; Concrete, described homology is more than 95%; Concrete is more than 96% again; Concrete is more than 97% again; Concrete is more than 98% again; Concrete is more than 99% again.The RNAi carrier of RNA of the present invention and this RNA of coding, can be used to strengthen the resistance of plant to TuMV or careless ammonium phosphine weedicide, simultaneously also for the cultivation of high resistance TuMV transgenic plant is laid a good foundation.
Description
Technical field
The invention belongs to genetic engineering for plant virus resistance field, be specifically related to the RNA of a kind of high resistance TuMV and the RNAi carrier of this RNA of coding.
Background technology
Brassica 2 et 4 (Turnip Mosaic Virus, TuMV) belongs to marmor upsilon section (Potyviridae), Potyvirus (Potyviruse).TuMV host range is very extensive, can infect 43 sections 156 and belong to 318 kind of plant.TuMV endangers crop in cruciferae virus the most serious.Infect the crop after virus and also easily infect oidium and soft rot, cause Combined Infection, directly have influence on output and commodity value.
Rape is the main oil crops of China, and turnip mosaic virus is one of important disease of rape.In China middle and lower reach of Yangtze River, rape generally reaches 20-30% because of the virus disease underproduction, and year of being very popular reaches about 50%.Susceptible rape not only output reduces, and oil yield rate and seed germination rate also obviously reduce.According to another investigation China Chinese cabbage because TuMV endangers the production loss causing 5-10% every year on average, the plot that disease is serious almost has no harvest.
TuMV mainly propagates in the mode of perishability by aphid, has at least 89 kinds of aphids can propagate this virus.And adopt sterilant can not kill whole aphids very soon to stop the propagation of virus, only kill by sterilant the DeGrain that aphid prevents and treats virus disease, also easily cause environmental pollution.Therefore seek new disease-resistant method and become a urgent task.
Summary of the invention
An object of the present invention is to provide the RNA of a kind of high resistance TuMV and the RNAi carrier of this RNA of coding.
A kind of RNA provided by the invention, has one of following nucleotide sequence:
1) nucleotide sequence shown in SEQ ID № .2 in sequence table;
2) with 1) the RNA sequence that limits has more than 90% homology, and has the RNA sequence of identical function; Concrete, described homology is more than 95%; Concrete is more than 96% again; Concrete is more than 97% again; Concrete is more than 98% again; Concrete is more than 99% again.
Described have identical function and specifically refer to have following arbitrary function:
1) plant is strengthened to the resistance of TuMV;
2) plant is strengthened to the resistance of weedicide.
Described plant is specially Arabidopis thaliana or crop in cruciferae; Described crop in cruciferae is specially rape or Chinese cabbage.
Described enhancing plant copies realization to the resistance of TuMV by suppressing TuMV.
Described TuMV is specially TuMV-C4 and/or BJ-R01.
Described weedicide is specially careless ammonium phosphine weedicide.
The encoding gene of described RNA also belongs to protection scope of the present invention.
Recombinant vectors containing described encoding gene, expression cassette, transgenic cell line or Host Strains also belong to protection scope of the present invention.
Described recombinant vectors is specially recombinant expression vector or recombinant cloning vector.
Described recombinant expression vector is inserted in the multiple clone site of the carrier that sets out by DNA fragmentation to obtain; Described DNA fragmentation is that X forward-joining region-X is reverse; X forward is in SEQ ID No.1 shown in the Nucleotide of 15-380 position, and X is reversed the reverse complemental fragment of X forward.
Concrete, described in the carrier that sets out be pBBBast.
In described recombinant expression vector, described X forward-reverse fragment of joining region-X has the 1365-2919 position nucleotide sequence in sequence table described in SEQ ID № .3.
Another object of the present invention is to provide described RNA, the encoding gene of described RNA, the following at least one application of described recombinant vectors, expression cassette, transgenic cell line or Host Strains containing described encoding gene:
1) product of anti-TuMV is prepared;
2) plant is strengthened to the resistance of TuMV;
3) plant is strengthened to the resistance of careless ammonium phosphine weedicide.
In described application, described plant is specially Arabidopis thaliana or crop in cruciferae; Described crop in cruciferae is specially rape or Chinese cabbage.
Described enhancing plant copies realization to the resistance of TuMV by suppressing TuMV.
In described application, described TuMV is specially TuMV-C4 and/or BJ-R01.
In described application, described weedicide is specially careless ammonium phosphine weedicide.
Another object of the present invention is to provide a kind of method of cultivating transgenic plant, is described recombinant expression vector is proceeded to object plant, obtains transgenic plant; Described transgenic plant, compared with described object plant, have following at least one proterties: 1) strengthen the resistance of TuMV; 2) resistance of weedicide is strengthened.
The described resistance to TuMV strengthens by suppressing TuMV to copy realization.
In described method, described TuMV is specially TuMV-C4 and/or BJ-R01.
In described method, described weedicide is specially careless ammonium phosphine weedicide.
In described method, described object plant is specially Arabidopis thaliana or crop in cruciferae; Described crop in cruciferae is specially rape or Chinese cabbage.
Accompanying drawing explanation
Fig. 1 is the digestion verification result of intermediate carrier, and wherein M is molecular weight marker; Swimming lane 1 is that the enzyme of pHannibal-CI carrier cuts result; Swimming lane 2 cuts result for the enzyme being connected into reverse fragment pHannibal-CI (-) carrier; Swimming lane 3 is that the enzyme of pHannibal empty carrier cuts result.
Fig. 2 is the structural representation of carrier pBBBTu-CI.
Fig. 3 is that the MluI enzyme of plant expression vector pBBBTu-CI cuts detected result figure, and wherein M is molecular weight marker; Swimming lane 1 is that the enzyme of pBBBTu-CI carrier cuts result.
Fig. 4 is T
1spray result after careless ammonium phosphine weedicide for seedling, survival be Herbicid resistant strain.
Fig. 5 is partial transgenic T
1for seedling PCR qualification result figure, wherein swimming lane 2 is molecular weight marker; Swimming lane 1 is the result of contrast col-0; Swimming lane 3-9 is the transgenosis T that herbicide screening goes out
1the result of Dai Miao.
Fig. 6 is the picture after different transgenosis high resistance strain inoculation TuMV-C4, and wherein col represents the result of wild-type col-0.
Picture when Fig. 7 is seed harvest after different transgenosis high resistance strain inoculation TuMV-C4, wherein col represents the result of wild-type col-0.
Fig. 8 is the picture after transgenosis high resistance strain #07 and #48 inoculate BJ-R01, and wherein col represents the result of wild-type col-0.
Fig. 9 is the disease index statistics after different transgenosis high resistance strain inoculation TuMV-C4, and wherein col represents the result of wild-type col-0, and #07, #12, #19, #22, #30, #34, #48 represent the result of 7 transgenosis high resistance strains respectively.
Figure 10 is that after TuMV-C4 inoculates Arabidopis thaliana, RT-PCR detects the expression of TuMV coat protein gene in transgenic arabidopsis, and wherein swimming lane 1 is the result of contrast Col-0; Swimming lane 2-6 is followed successively by transgenosis high resistance strain #07, the result of #12, #22, #34, #48.
Figure 11 is that after TuMV-C4 inoculates Arabidopis thaliana, quantitative fluorescent PCR analytical results, wherein col represents the result of wild-type col-0, and #07, #12, #22, #34, #48 represent the result of 5 transgenosis high resistance strains respectively.
Embodiment
The experimental technique used in following embodiment if no special instructions, is ordinary method.
Material used in following embodiment, reagent etc., if no special instructions, all can obtain from commercial channels.
1, material
This tests wildtype Arabidopsis thaliana Col-0 used purchased from Arabidopsis Biological Resource Center.
The Brassica 2 et 4 TuMV main popular strong strain TuMV-C4 that causes a disease in Beijing area is available from vegetable or flower institute of the Chinese Academy of Agricultural Sciences; Reference: Feng Lanxiang, Xu Ling, Liu Jia, button heart lattice, Li Xiusheng, the qualification of Beijing area Turnip Mosaic Virus of Chinese Cabbage strain, China's Vegetable, 1988,4:11-13; The public can obtain this strain from Beijing Agricultural Biological Technology Rsearch Centre.
TuMV radish by force pathogenic strain BJ-R01 gathers from field for contriver and preserves.Reference " Ye Yanying, Zeng Gang, Yan Xiaohong, Ma Rongcai, Wu Caijun, Yao Lei, Agricultural University Of Jiangxi's journal, 2012,34 (2): 264-269 ".The public can obtain from Beijing Agricultural Biological Technology Rsearch Centre.
Intestinal bacteria (Escherichia coli) DH5 α bacterial strain is purchased from Tiangen company, and catalog number is CB101;
Agrobacterium (Agrobacterium tumefacieus) GV3101(pMP90), reference: Koncz, C.andSchell, J. (1986) The promoter of TL-DNA gene5controls the tissue-specificexpression of chimeric genes carried by a novel type of Agrobacterium binaryvector.Mol.Gen.Genet.204,383 – 396.The public can obtain this bacterial strain from Beijing Agricultural Biological Technology Rsearch Centre.
The RNAi carrier pHannibal public can from CSIR O(
http:// www.csiro.au/pi) obtain; Reference: Wesley S V, Helliwell C A, Smith N A.Construct design for efficient, effective and high-throughput gene silencing in plants [J] .The Plant Journal, 2001,27 (6): 581-590.
High-fidelity enzyme Fast pfu DNA Polymerase, Easy Taq enzyme and molecular weight marker are purchased from Quan Shi King Company.The little extraction reagent kit of plasmid, glue reclaim test kit, PCR purification kit is century bio tech ltd purchased from health.M-MLV ThermoScript II, quantitative PCR reagent, restriction enzyme and Klenow Fragment fill enzyme purchased from TaKaRa company.DNTP, dGTP and dCTP are purchased from Promega company.
The preparation of embodiment 1, RNAi carrier
(1) preparation of CI gene conservative fragments
According to the conservative property of listed 118 the TuMV strains of GenBank, the conservative fragments choosing the common 366bp of 882-1247 position nucleotide sequence of CI gene is that RNA disturbs target.
Extract the total serum IgE of TuMV-C4 bacterial strain, and reverse transcription is cDNA, with this cDNA for template, with following CI366F and CI366R(underscore part for restriction enzyme site Xho I, BamH I and EcoR I, Hind III) for primer, carry out pcr amplification with high-fidelity enzyme Fastpfu DNA Polymerase:
CI366 F 5’-cc
ctcgagggatccTGGAACACCTAGCAAGAAGCACT-3’;
CI366 R 5’-cg
gaattcaagcttCGTGCCTGCTTTGCCGTTAC-3'。
Pcr amplification program: 94 DEG C of 5min; 94 DEG C of 30s, 56 DEG C of 30s, 72 DEG C of 1min, 30 circulations; 72 DEG C extend 7min.
PCR primer reclaims after agarose electrophoresis purifying.Through order-checking, gained PCR primer proves that nucleotide sequence is correct, its nucleotide sequence has the nucleotide sequence shown in SEQ ID № .1 in sequence table, and its RNA encoded has the nucleotide sequence shown in SEQ ID № .2 in sequence table.
(2) structure of RNAi carrier
1, the preparation of intermediate carrier pHannibal-CI
1) preparation process
The PCR primer of double digestion pHannibal carrier and above-mentioned preparation is distinguished with Hind III and BamH I.Enzyme reclaims the vector backbone segment of about 5818bp and the PCR primer fragment of about 372bp through purifying after cutting, and 4 DEG C of connections are spent the night.Connect product through thermal shock transformation of E. coli DH5 α.Picked clones, extracts plasmid and by PstI and XhoI digestion verification, obtains the intermediate carrier pHannibal-CI (-) containing reverse fragment.
With XhoI and EcoRI respectively the above-mentioned preparation of double digestion PCR primer and be connected into pHannibal-CI (-) intermediate carrier of reverse fragment.The PCR primer fragment of the purified rear recovery about 6184bp vector backbone segment of digestion products and about 384bp, 4 DEG C of connections are spent the night.Connect product conversion bacillus coli DH 5 alpha, picked clones, extract plasmid also with the checking of PstI and XhoI double digestion, obtain the intermediate carrier pHannibal-CI simultaneously containing reverse and forward fragment.
2) the digestion verification process of constructed carrier
With XhoI and PstI double digestion pHannibal empty carrier, the pHannibal-CI (-) being connected into reverse fragment and pHannibal-CI intermediate carrier respectively, enzyme is cut rear electrophoresis and is detected, and carries out confirmatory experiment.Experimental result is shown in Fig. 1.Fig. 1 result shows: pHannibal empty carrier produces 4276bp and 1548bp two bar segment after double digestion, pHannibal-CI (-) produces 4276bp and 1914bp two bar segment after double digestion, and pHannibal-CI produces 4276bp and 2292bp two bar segment after double digestion.Enzyme is cut and electrophoresis result shows, intermediate carrier pHannibal-CI builds correct.
2, the preparation of plant expression vector pBBBTu-CI
1) preparation process
The RNAi hairpin structure two ends of pHannibal are respectively containing 1 NotI restriction enzyme site.The intermediate carrier pHannibal-CI containing hairpin structure is cut with NotI enzyme, same enzyme is cut in system and is respectively mended two bases G with Klenow enzyme and dGTP at two sticky ends of endonuclease bamhi again, product is in 1% agarose gel electrophoresis purifying, and the fragment that glue reclaims containing the 3708bp of hairpin structure is for subsequent use.Through order-checking, the fragment of the described 3708bp containing hairpin structure has the nucleotide sequence in sequence table described in SEQ ID № .3, and described hairpin structure fragment has the 1365-2919 position nucleotide sequence in sequence table described in SEQ ID № .3.
Plant binary vector pBBBast can be the SspI restriction enzyme site of the double chain DNA molecule insertion vector pBBR1MCS-2 by having nucleotide sequence shown in SEQ ID № .4 in sequence table, the recombinant plasmid that the small segment between the SspI restriction enzyme site of replacement plasmid pBBR1MCS-2 obtains.
The plasmid pBBR1MCS-2 public can obtain from Beijing Agricultural Biological Technology Rsearch Centre; Reference: KovachME; Elzer PH; Hill DS; Robertson GT; Farris MA; Roop RM2nd, Peterson KM.Fournew derivatives of the broad-host-range cloning vector pBBR1MCS, carryingdifferent antibiotic-resistance cassettes.Gene.1995Dec1; 166 (1): 175-6.
With XmaI single endonuclease digestion plant binary vector pBBBast, two base C are respectively mended at two sticky ends again with Klenow enzyme and dCTP, product is in 1% agarose gel electrophoresis, glue reclaims carrier segments 6559bp, be connected with the 3708bp fragment 4 DEG C containing hairpin structure of above-mentioned preparation again and spend the night, obtain expression of plants RNAi plasmid pBBBTu-CI, its structural representation is shown in Fig. 2.
2) the digestion verification process of constructed carrier
The plant expression vector pBBBTu-CI of above-mentioned preparation is carried out MluI enzyme and cuts detection.PBBBast carrier itself has a MluI restriction enzyme site, and connect in the above-mentioned CaMV promotor containing the fragment of hairpin structure and separately have a MluI restriction enzyme site, what enzyme cut rear display 2 band is positive colony.Cut stripe size according to enzyme and can judge that insertion is that clockwise forward connects or counterclockwise Opposite direction connection.Forward ligase enzyme slitting band is 9715bp and 542bp, and Opposite direction connection band is 6494bp and 3773bp band.MluI enzyme is cut detected result and is seen Fig. 3.Fig. 3 result shows to be connected in the XmaI restriction enzyme site of plant binary vector pBBBast for the RNAi structure of CI gene conservative fragments, and is Opposite direction connection.
The functional verification of the RNA of embodiment 2, high resistance TuMV and the RNAi carrier of this RNA that encodes
(1) genetic transformation of Arabidopis thaliana and the screening of positive seedling
Utilize electric shocking method to be proceeded in Agrobacterium GV3101 (pMP90) by pBBBTu-CI carrier, adopt agriculture bacillus mediated inflorescence pickling process to infect Arabidopis thaliana.By the Arabidopis thaliana T of results
0for planting seed in the culture tray filling Nutrition Soil, be placed in 22 DEG C of (daytime)/18 DEG C (night), periodicity of illumination is 16h(light)/8h(is dark) phytotron.Grow sprinkling water after two panels cotyledon until seedling by volume to count dilution 500 times careless ammonium phosphine weedicide (described careless ammonium phosphine weedicide is the commercial weedicide that market is bought, and its medium-height grass ammonium phosphine concentration is 200mg/L) and screen positive seedling.
Through spraying after 2-3 careless ammonium phosphine herbicide screening, non-transgenic seedling can not continued growth, gradually withered and yellow death; And transgenic seedling growing way is healthy and strong, blade keeps green, part seedling the results are shown in Figure 4.Obtain 126 strain T altogether
1for Herbicid resistant plant.Randomly draw the blade of 68 strain resistance seedlings, extract plant genome DNA with a small amount of rapid method.Carry out pcr amplification detection with primer CI366F and CI366R, reaction conditions is: 94 DEG C of 5min; 94 DEG C of 45s, 55 DEG C of 30s, 72 DEG C of 30s, 35 circulations; 72 DEG C of 7min.PCR primer carries out electrophoresis detection on 1% sepharose, and what amplify goal gene fragment 394bp is transgenic positive seedling.Detected result display is all positive seedling.The PCR qualification result of part seedling is shown in Fig. 5.
Choose the transgenosis T1 being accredited as positive seedling to reserve seed for planting for seedling selfing, T
2in generation, randomly draws 32 strain sowings, and seedling sprinkling by volume counts dilution 500 times careless ammonium phosphine weedicide (described careless ammonium phosphine weedicide is the commercial weedicide that market is bought, and its medium-height grass ammonium phosphine concentration is 200mg/L) with water 2-3 time and adds up survival/Mortality Ratio afterwards.Have 18 strain segregation ratio to be about 3:1, tentatively confirm as and singly copy strain, and individual plant selfing sowing is sub.Offspring continues screening and is not separated strain and is homozygous lines.
(2) anti-disease enzyme of transfer-gen plant
Randomly draw 12 homozygous lines and carry out anti-disease enzyme.By homozygous lines, wild-type Col-0 with turn empty carrier Arabidopis thaliana and sow simultaneously, treat that seedling grows to TuMV-C4 or the BJ-R01 strain of 8-10 sheet lotus throne leaf frictional inoculation in period TuMV.Inoculation liquid is by sick leaf weight/phosphoric acid buffer volume (pH=7.0) about 1g/10mL proportions.Each homozygous lines inoculation 8-12 strain, every strain inoculation two panels comparatively big leaf's slice.With non-transgenic wildtype Arabidopsis thaliana Col-0 with turn empty carrier Arabidopis thaliana and inoculate in contrast.Blade is rinsed with clear water immediately after inoculation several minutes.Middle net cover is observed in the controlled environment chamber, carries out anti-disease enzyme and disease index statistics after 20 days.
State of an illness grade classification: 0 grade complete asymptomatic; 1 grade of 1-2 sheet does not inoculate leaf floral leaf or jaundice, energy bolting; 3 grades of 3-4 sheets do not inoculate leaf floral leaf or jaundice energy bolting; 5 grades of 5-6 sheets do not inoculate leaf floral leaf or jaundice, affect bolting; 7 grades of most blade floral leaves or jaundice, can not bolting; 9 grades of most of blades are withered, and plant is at death's door.
Disease index=100 × ∑ (diseased plant number at different levels × typical value at different levels)/(investigating total strain number × highest typical value)
The partial results of disease-resistant inoculation is shown in Fig. 6,7,8, and disease index statistics is shown in Fig. 9.Fig. 6 result shows, after inoculation TuMV-C4 about 20 days, contrast wild-type Col-0 withered death substantially, turn empty vector control result and Col-0 basically identical, and transgenic line shows different resistances, 7 strain (#07, #12, #19, #22, #30, #34, #48) can grow preferably after inoculation, and the later stage can be normally solid, shows the highly resistant to TuMV-C4.Fig. 7 result shows, and the high resistance transgenic line inoculating TuMV-C4 to seed harvest period can normally be set seeds; And the plant contrasting Col-0 is all dead, can gather in the crops without seed.Fig. 9 result shows, and after inoculation TuMV-C4, the disease resistance of disease index statistical result showed high resistance strain improves about 80% than adjoining tree Col-0 resistance, turn empty vector control result and Col-0 basically identical.
After high resistance transgenic line #07 and #48 inoculates BJ-R01, Fig. 8 result shows, the aobvious disease of contrast wild-type Col-0 morbidity, and high resistance transgenic line #07 and #48 shows good growing way, and it has the resistance of height equally to BJ-R01.Illustrate that the resistance of the present invention to the different strain of TuMV has certain broad spectrum.
High resistance transgenic line is reserved seed for planting, and offspring proceeds anti-disease enzyme.Result shows these transgenic lines can genetic stability to the resistance of TuMV.
(3) sxemiquantitative and relative quantification detect the accumulation of virus
5 high resistance strain #07, #12, #22, #34, #48, contrast Col-0 and turn empty vector control inoculation TuMV-C4 after about 20 days, choose each strain and do not inoculate blade TRIzol method and extract total serum IgE respectively, be inverted to cDNA with M-MLV.With the 196bp conservative fragments of TuMV coat protein gene for detected object, be that internal reference carries out sxemiquantitative and quantitative fluorescence analysis with the 298bp fragment of Arabidopis thaliana SAND gene (AT2G28390).
The primer sequence that the 196bp of amplification TuMV-CP gene guards section is as follows:
CP F 5’-AAAGCGTAACCAAGACCGACCAT-3';
CPR 5’-TCCATCCAAGCCGAACAAAT-3'。
The primer sequence of amplification reference gene SAND gene 298bp fragment is as follows:
SAND F 5'-AATGTGGATGGTGACACTGCCTCG-3;
SAND R 5'-ACCTGGTGATTTCCTGCCTTGAC-3'。
RT-PCR response procedures: 94 DEG C of 5min; 94 DEG C of 30s, 57 DEG C of 30s, 72 DEG C of 30s, 30 circulations; 72 DEG C of 7min.PCR primer carries out electrophoresis detection on 1.2% sepharose.
The reaction of quantitative fluorescent PCR is to dilute the cDNA of 40 times for template, and SYBR-green I makees fluorescent indicator, and response procedures adopts two-step approach amplification.Amplification condition is: 95 DEG C of 30s; 95 DEG C of 5s, 57 DEG C of 30s, 72 DEG C of 30s, 40 circulations.Each strain sample carries out repeating experiment for 3 times, averages.
Half-quantitative detection the results are shown in Figure 10.Figure 10 result shows, when reference gene expression amount is almost consistent, a large amount of virus accumulation can be detected in contrast Col-0 plant body, it is basically identical with Col-0 to turn empty vector control result, and micro-virus can only be detected in high resistance transgenic line body.
The detected result of quantitative fluorescent PCR is shown in Figure 11.Figure 11 result shows, consistent with semiquantitative result, in contrast Col-0 body, a large amount of virus detected, turn empty vector control result and Col-0 basically identical, and in 5 high resistance strain plant materialss, almost can't detect viral copying.Illustrate that the RNAi carrier utilizing CI gene fragment to build has played vital role in transgenic plant are antiviral, the disease resistance of transfer-gen plant significantly improves.
Claims (13)
1. a RNA, its nucleotides sequence is classified as shown in the SEQ ID No.2 in sequence table.
2. the encoding gene of RNA according to claim 1.
3. the recombinant vectors containing encoding gene according to claim 2.
4. recombinant vectors according to claim 3, is characterized in that: described recombinant vectors is recombinant expression vector or recombinant cloning vector.
5. recombinant expression vector according to claim 4, is characterized in that: described recombinant expression vector is inserted in the multiple clone site of the carrier that sets out by DNA fragmentation to obtain; Described DNA fragmentation is that X forward-joining region-X is reverse; X forward is in SEQ ID No.1 shown in the Nucleotide of 15-380 position, and X is reversed the reverse complemental fragment of X forward.
6. recombinant expression vector according to claim 5, is characterized in that: described X forward-reverse fragment of joining region-X is SEQ ID No.3 1365-2919 position nucleotide sequence in sequence table.
7. the expression cassette containing encoding gene according to claim 2.
8. the transgenic cell line containing encoding gene according to claim 2.
9. the Host Strains containing encoding gene according to claim 2.
10. the following at least one application of Host Strains described in transgenic cell line described in expression cassette, claim 8 described in RNA according to claim 1, encoding gene according to claim 2, the recombinant vectors described in claim 3 or 4, the recombinant expression vector described in claim 5 or 6, claim 7 or claim 9:
1) product of anti-TuMV is prepared;
2) plant is strengthened to the resistance of TuMV;
3) plant is strengthened to the resistance of careless ammonium phosphine weedicide.
11. 1 kinds of methods of cultivating transgenic plant, are that the recombinant expression vector described in claim 5 or 6 is proceeded to object plant, obtain transgenic plant; Described transgenic plant, compared with described object plant, have following at least one proterties: 1) strengthen the resistance of TuMV; 2) resistance of careless ammonium phosphine weedicide is strengthened.
12. methods according to claim 11, is characterized in that: described object plant is specially Arabidopis thaliana or crop in cruciferae.
13. methods according to claim 12, is characterized in that: described crop in cruciferae is rape or Chinese cabbage.
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