CN103215368A - Method for detecting anti-pyricularia grisea cav. gene pi5 in rice breeding materials by utilizing co-segregation marker pi5-1-2 - Google Patents
Method for detecting anti-pyricularia grisea cav. gene pi5 in rice breeding materials by utilizing co-segregation marker pi5-1-2 Download PDFInfo
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Abstract
The invention belongs to the field of molecular biology and in particular relates to a molecular marker for detecting an anti-pyricularia grisea cav. gene in rice and special primers thereof. The molecular marker is a dominant molecular marker pi5-1-2 of the anti-pyricularia grisea cav. gene pi5. The molecular marker uses a primer pair SEQ ID NO:1 and SEQ ID NO:2 to amplify a nucleotide sequence from the total DNA (deoxyribonucleic acid) of rice, and can be applied to molecular marker-assisted selection of pi5 in rice pyricularia grisea cav. resistance breeding to improve the disease-resistant variety breeding efficiency and reduce the workload of field identification.
Description
Technical field
The invention belongs to biology field, be specifically related to utilize the blast resistant gene pi5 that is divided in mark pi5-1-2 detection rice breed.
Background technology
Rice blast (Pyricularia grisea cav.) is by Pyricularia oryzae (Magnaporthe oryzae; No condition: the rice disease that Pyricularia) causes, its distribution range is very extensive.According to statistics, all there was generation in a country surplus the whole world had 80, and the general popular time can be caused the underproduction of 10%-20%, then reached 40%-50% when seriously taking place.Since the nineties in 20th century, all more than 3,800,000 hm2, annual loss paddy reaches several hundred million kilograms to the year generation area of China's rice blast.Along with simplification, centralization and climatic influences that kind is used, the harm of rice blast is also more and more heavier.Although people have expended huge energy and material input in disease control, be limited to the influence of all many-sided factors, protection effect is unsatisfactory always, especially seriously takes place the time in disease, causes heavy losses usually for production, breeding.With Liaoning Province is example, from the nineties in 20th century, has taken place respectively to take place because of the panicle blast big area that the several main breed disease resistances degenerations of distant round-grained rice 287, distant salt 241, Liaogeng No.454 and Liaoxing No.1 cause, and has had a strong impact on the production of North Japonica Rice.The basic reason that produces this phenomenon is exactly that main breed is narrow to the anti-spectrum of Pyricularia oryzae, and simplification, centralization plantation phenomenon is general, in case the popular microspecies of rice blast fungus change like this, kind is to the just decline rapidly of resistance of rice blast.Therefore, the rice varieties of seed selection polymerization polygene or tool resistance of wide spectrum is particularly necessary.
At present, in the process of blast resisting breed breeding, breeding man is main to adopt pedigree method, or the disease-resistant individuality of binding molecule marker assisted selection.Traditional pedigree method is by two parent's assembly, and seed selection kind according to qualifications from separate the offspring, anti-pest phenotype depend on that identify naturally in the field or the artificial inoculation evaluation, and the discriminating difficulty is big, and accuracy rate is low.Owing to do not understand parent's anti-pest genotype, the breeder in parent's selections very blindly, magnanimity combo normally, magnanimity selection offspring, workload is big, breeding efficiency is low.When utilizing molecular marker assisted selection to carry out breeding for disease resistance, selected be mostly the SSR mark chain with disease-resistant gene, easily cause false-positive judgement, if can design heterogeneic being divided into according to the sequence difference of anti-sense allelotrope itself from mark, not only can at first detect the entrained anti-pest gene of parent, also can when offspring's assisted Selection, improve the accuracy that resistant variety is selected greatly.
Rice blast resistant gene Pi5 (Jeon J S, et al.Genetic and physical mapping of Pi5 (t), a locus associated with broad-spectrum resistance to rice blast.Molecular Genetics and Genomics, 2003,269 (2): 280-289; Wang G L, et al..RFLP Mapping of Genes Conferring Complete and Partial Resistance to Blast in a Durably Resistant Rice Cultivar Genetics, 1994,136 (4): 1421-1434) on paddy rice the 9th karyomit(e) in the 170kb interval between S04G03 and the C1454, the NBS-LRR genoid (Pi5-1 and Pi5-2) that comprises two independent inheritances, and the protein product of two genes all has the CC structure at aminoterminal.Pi5-l and Pi5-2 have 5 and 6 exons respectively, and protein product contains 1025 and 1063 amino acid respectively; Gene expression analysis shows that Pi5-1 is expressed by pathogenic bacterium inducing, and Pi5-2 is the constructive expression, under the greenhouse artificial inoculation conditions, 5 rice blast microspecies such as PO6-6 are showed complete resistances, the original resistance donor of Pi5 gene is RIL260 (Wang G L, et al..RFLP Mapping of Genes Conferring Complete and Partial Resistance to Blast in a Durably Resistant Rice Cultivar Genetics, 1994,136 (4): 1421-1434).
Summary of the invention
For high efficiency selected anti-rice blast rice kind, targetedly, specific selection contains the progeny material of Pi5 gene, the invention provides a kind of molecule marker pi5-1-2 that is used to detect rice blast resistant gene pi5, molecule marker and pi5 gene be divided into from, the assisted Selection that can be used for the Pi5 gene is with the efficient of raising molecular marker assisted selection and the efficient of disease-resistant variety seed selection.
The invention provides following solution:
A kind of and the chain molecule marker pi5-1-2 of rice blast resistant gene pi5, shown in SEQ ID NO:3, described molecule marker pi5-1-2 and rice blast resistant gene pi5 be divided into from.
A kind ofly be used for primer that whether detection molecules mark pi5-1-2 exist to DNA, shown in SEQ ID NO:1 and SEQ ID NO:2.
A kind of method that whether has rice blast resistant gene pi5 in the paddy DNA that detects, with sequence shown in SEQ ID NO:1 and the SEQ ID NO:2 is primer, DNA to be detected increases, and amplicon contains just like sequence (1066bp) shown in the SEQ ID NO:3, is and contains rice blast resistant gene pi5.
A kind of anti-rice blast rice kind molecular marker-assisted selection method, with the rice material that contains blast resistant gene pi5 is the parent, with other rice varieties hybridization, extract filial generation genes of individuals group DNA, with sequence shown in SEQ ID NO:1 and the SEQ ID NO:2 is that primer carries out pcr amplification, and the corresponding individuality that amplicon contains just like sequence shown in the SEQ ID NO:3 promptly contains rice blast resistant gene pi5.
Above-mentioned primer is identified preferably the DNA that rice seedling extracted being carried out mark, detect and whether carry blast resistant gene pi5, because above-mentioned primer designs the difference that is based on genome C DS sequence, therefore easy to detect, accuracy rate height, this molecule marker can be used as the application of pi5 gene molecule marker assisted Selection in the rice blast breeding for disease resistance.
Description of drawings
The gel electrophoresis figure of Fig. 1 amplified production that is molecule marker pi5-1-2 in blast resistant gene Pi5 donor kind RIL260, pi5 single-gene system and 5 high sense rice varieties;
Wherein, M:2000bp molecular weight marker (TIANGEN MD114-02), 200ng; Fragment length is respectively: 100bp, 250bp, 500bp, 750bp, 1000bp, 2000bp.
1:RIL260; 2: Lijiang xintuanheigu; 3: distant salt 241; 4: salt rich 47; 5: Japan is fine; 6: Liaoxing No.1; The 7:pi5 single-gene is that wherein disease-resistant gene donor kind RIL260 and pi5 single-gene are that the amplified production clip size is 1066bp, and susceptible variety does not have amplified production.
The gel electrophoresis figure of Fig. 2 amplified production that is molecule marker pi5-1-2 blast resistant gene Pi5 donor kind RIL260, pi5 single-gene system (introducing) and 16 rice varieties from IRRI.
Wherein, M:2000bp molecular weight marker (TIANGEN MD114-02), 200ng; Fragment length is respectively: 100bp, 250bp, 500bp, 750bp, 1000bp, 2000bp.
1:RIL260; 2: Lijiang xintuanheigu; 3: Japan is fine; 4: distant round-grained rice 371; 5: Shen Nong 606; 6: Liaoxing No.1 7: Shen rice 7; 8: light more; 9: distant salt 241; 10: No. 8, source, port; 11: Shen Nong 265; 12: No. 2, thousandweight wave; 13: the Liao Dynasty's farming 979; 14: distant round-grained rice 294; 15: the Liao Dynasty opens 79; 16: distant star 20; 17: No. 4, iron round-grained rice; 18:pi5 single-gene system.
Wherein No. 13 kind amplified production fragment lengths are consistent with pi5 single-gene system and donor kind, further sequencing result shows that its amplified production sequence is consistent with the described sequence of SEQ ID NO:3, determine to carry blast resistant gene pi5, and all the other kinds all do not have pcr amplification product, illustrate not contain blast resistant gene pi5.
Embodiment
Embodiment 1:DNA extraction, pcr amplification and electrophoretic analysis
One, DNA extraction (CTAB method):
Take by weighing 0.1~0.2g rice leaf and be cut into 1cm length, in liquid nitrogen, grind, treat the intact back of liquid nitrogen vaporization (noting: sample is melted), change the extracting solution (1M Tris pH8.0, the 100mM that contain 65 ℃ of preheatings rapidly over to; 5M NaCl, 1.0M; 0.5M EDTA, 20mM; 10%CTAB, 2.0%) in the centrifuge tube of 400 μ L.Shake up gently.
60~65 ℃ of water-baths 30~60 minutes were shaken evenly in per 10 minutes gently.
Add isopyknic chloroform/primary isoamyl alcohol (24: 1), gentleness is shaken, and makes into milk sap.
Under the room temperature (temperature is not less than 15 ℃), the centrifugal 5min of 12000r/min gets supernatant liquor.
Carefully extract the dehydrated alcohol (or isopyknic primary isoamyl alcohol) that supernatant liquor 200 μ L add 2 times of volumes of precooling with macropore Tip head, place more than 20 minutes centrifugal 5 minutes of 5000r/min, collecting precipitation under-20 ℃ the condition.
70% washing with alcohol precipitation 1~2 time.
Open the pipe lid, put clean place and dry, transparent the getting final product of milky DNA precipitation.
100 μ LTE (Tris-Hcl10mM, PH8.0; EDTA1mM, PH8.0) dissolution precipitation, and be diluted to 100 μ g/mL ,-20 ℃ of preservations are standby.
Two, pcr amplification:
Pcr amplification reaction carries out on the pcr amplification instrument.
1. reaction system is as follows:
2 * Taq PCR Master Mix (Ai Delai PC0902), 10 μ L, each 0.5 μ L of the primer of 10 μ M, the template DNA 1 μ L of 100 μ g/mL, ddH
2O8 μ L.
3.PCR response procedures is: 94 ℃ of pre-sex change 5min, 94 ℃ of sex change 30s, 56 ℃ of annealing 30s, 72 ℃ are extended 70s, 35 circulations, 72 ℃ are extended 10min, 4 ℃ of preservations.
Three, the PCR product detects
Get 4 μ L PCR products, electrophoresis in 1% sepharose through goldview dyeing, is used the gel imaging system log.
The pi5-1-2 marker detection of embodiment 2:pi5 donor kind and single-gene system.
With blast resistant gene Pi5 donor kind RIL260, pi5 single-gene system and 5 high sense rice varieties (Lijiang xintuanheigus; The Liao Dynasty's salt 241; Salt rich 47; Liaoxing No.1; Japan is fine) for trying material, plant in the greenhouse, Liaoning Area popular Pyricularia oryzae ZA9, ZA33, ZB1 and ZB17 are transplanted respectively on the rolled oats tomato juice agar, cultivate 5~7d under 25~27 ℃ of conditions, treat that mycelia covers with, wipe cultivations of preserving moisture behind the aerial hyphae with the cotton swab of sterilization, Pyricularia oryzae is understood big volume production spore.When treating that 7 kind rice seedlings grow to 5 leaves, 1 heart, each bacterial strain conidium of the numerous cultivation of above-mentioned expansion is used the 120ml sterile water wash respectively, filter in the triangular flask of packing into double gauze, preparation spore suspension (concentration is that 20 left and right sides spores are arranged under the 120 power microscope visuals field) is isolated spray inoculation respectively.Inoculation back 24h is overlying on plastic film on the brandreth of vinyl disc top and preserves moisture, and covers the sunshade net and prevent the sunlight direct projection on plastic film.In the 10d investigation of inoculation back, cause a disease response type and microspecies are determined to evaluate by national physiological races of rice blast fungus Combined Trials group (1980) unified standard.
Investigation record standard:
0 grade anosis ... high anti-(HR)
1 grade of brown point that the needle point size is only arranged ... anti-(R)
2 grades big slightly brown point ... anti-(R)
3 grades of little scabs of grey that circle is big slightly, edge brown, scab diameter 1~2mm ... in anti-(MR)
4 grades of typical fusiform scabs, long 1~2cm is confined between two master pulses usually.Cause harm area below 2% ... middle sense (MS)
5 grades of typical scabs, the area 3%~10% of causing harm ... middle sense (MS)
6 grades of typical scabs, the area 11%~25% of causing harm ... sense (S)
7 grades of typical scabs, the area 26%~50% of causing harm ... sense (S)
8 grades of typical scabs, the area 51%~75% of causing harm ... high sense (HS)
9 grades of whole blades are withered ... high sense (HS)
The inoculation qualification result shows, blast resistant gene Pi5 donor kind RIL260 and pi5 single-gene system shows as disease-resistant (R) to 4 physiological races of rice blast fungus of Liaoning Area popular, and Lijiang xintuanheigu, distant salt 241, salt are rich 47, Japan is fine, 5 rice varieties of Liaoxing No.1 all show as susceptible (S) to ZA9, ZA33, ZB1 and ZB17.
Above result shows, with SEQ ID NO:1 and SEQ ID NO:2 be primer carry out the fragment of pcr amplification can be as detecting the mark whether blast resistant gene pi5 exists.Have the kind of specific amplification products can be defined as carrying blast resistant gene pi5, and the kind of not having an amplified production product is not carried this disease-resistant gene.
Conclusion: can detect the existence of blast resistant gene pi5 with this mark reliably.
Embodiment 3: utilize molecule marker pi5-1-2 to detect the breeding parent material and whether contain blast resistant gene pi5
With blast resistant gene Pi5 donor kind RIL260, pi5 single-gene system (introducing from IRRI) and 16 rice varieties are the examination material, normally plant in the field, press embodiment 1 described method seedling stage and extract DNA, with SEQ ID NO:1 and SEQ ID NO:2 is that primer carries out pcr amplification, 18 kind amplifications as shown in Figure 2, except that blast resistant gene Pi5 donor kind RIL260 and pi5 single-gene system (introducing) from IRRI, No. 13 kind the Liao Dynasty farming 979 also amplifies and the consistent specificity product of donor kind and single-gene system, further sequencing result shows sequence unanimity shown in the amplified production sequence SEQ ID NO:3.The inoculation qualification result shows that the Liao Dynasty's 4 physiological races of rice blast fungus of 979 pairs of Liaoning Area popular of farming show as disease-resistant (R).
Result based on molecular markers for identification can determine that these 3 kinds contain blast resistant gene pi5.Gene test shows that the Liao Dynasty's farming 979 contains the pi5 gene.
Conclusion: can be used for the evaluation of the blast resistant gene pi5 of sick breeding parent of anti-rice and progeny material with this mark efficiently.
Claims (2)
1. one kind is detected the method that whether has rice blast resistant gene pi5 in the paddy DNA, with sequence shown in SEQ ID NO:1 and the SEQ ID NO:2 is primer, the DNA to be detected that increases, and amplicon contains just like sequence shown in the SEQ ID NO:3, is and contains rice blast resistant gene pi5.
2. anti-rice blast rice kind molecular marker-assisted selection method, with the rice material that contains blast resistant gene pi5 is the parent, with other rice varieties hybridization, extract filial generation genes of individuals group DNA, with sequence shown in SEQ ID NO:1 and the SEQ ID NO:2 is that primer carries out pcr amplification, and the corresponding individuality that amplicon contains just like sequence shown in the SEQ ID NO:3 promptly contains rice blast resistant gene pi5.
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| CN103497996A (en) * | 2013-09-22 | 2014-01-08 | 江苏里下河地区农业科学研究所 | Molecular marker InDe1587 for detecting rice blast resistant gene Pigm(t) of rice #4 |
| CN104774945A (en) * | 2015-04-10 | 2015-07-15 | 辽宁省农业科学院 | Molecular breeding method for new rice variety carrying gene Pi65(t) with resistance to rice blast |
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Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN103497996A (en) * | 2013-09-22 | 2014-01-08 | 江苏里下河地区农业科学研究所 | Molecular marker InDe1587 for detecting rice blast resistant gene Pigm(t) of rice #4 |
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| CN104774945A (en) * | 2015-04-10 | 2015-07-15 | 辽宁省农业科学院 | Molecular breeding method for new rice variety carrying gene Pi65(t) with resistance to rice blast |
| CN104774945B (en) * | 2015-04-10 | 2017-10-03 | 辽宁省农业科学院 | One kind carries the molecular breeding method of blast resistant gene Pi65 (t) new rice variety |
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