CN108315470B - Indel molecular marker P24 linked with anti-clubroot property of Degao CR117 Chinese cabbage, kit and application thereof - Google Patents

Indel molecular marker P24 linked with anti-clubroot property of Degao CR117 Chinese cabbage, kit and application thereof Download PDF

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CN108315470B
CN108315470B CN201810354431.6A CN201810354431A CN108315470B CN 108315470 B CN108315470 B CN 108315470B CN 201810354431 A CN201810354431 A CN 201810354431A CN 108315470 B CN108315470 B CN 108315470B
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张淑霞
杨晓云
司朝光
张清霞
刘玲
孙吉禄
焦功强
李剑
王殿纯
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QINGDAO ACADEMY OF AGRICULTURAL SCIENCES
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Abstract

The invention provides an Indel molecular marker P24 linked with a German high CR117 Chinese cabbage clubroot disease resistance character, a kit and application thereof, belonging to the technical field of Chinese cabbage breeding. The invention provides an Indel molecular marker P24 closely linked with the anti-clubroot property of Degao CR117 Chinese cabbage and a primer pair for amplification. The Indel molecular marker P24 provided by the invention is applied to screening of Degao CR117 Chinese cabbages with the anti-clubroot property and similar Chinese cabbage varieties. The developed application of the molecular marker solves the problem of effective utilization of clubroot-resistant Chinese cabbage disease-resistant genes such as Degao CR117 and the like. The application of the marker solves the problems of long identification period, germ pollution diffusion and inaccuracy of inoculation identification existing in the type of clubroot disease resistant character inoculation. The screening accuracy is high, and simultaneously, the screening operation is simple and convenient, the cost is low, and the repeatability is good.

Description

Indel molecular marker P24 linked with anti-clubroot property of Degao CR117 Chinese cabbage, kit and application thereof
Technical Field
The invention belongs to the technical field of Chinese cabbage breeding, and particularly relates to an Indel molecular marker P24 linked with a German high CR117 Chinese cabbage anti-clubroot trait, a kit and application thereof.
Background
The cruciferous clubroot is a worldwide disease caused by infection of Plasmodiophora brassica workbench, has a wide host range, and can damage various 100 cultivated and wild cruciferous plants such as Chinese cabbage, radish, cauliflower, rape and the like. Chinese cabbage is one of the most serious cruciferous vegetables with clubroot, and in recent years, clubroot occurs in coastal areas, Yunpuan, northeast areas, western areas and other most areas in China, the area is rapidly increased and is increased year by year, and the Chinese cabbage is the main disease of a main production area of the Chinese cabbage.
Because the dormant spores of plasmodiophora brassicae have strong stress resistance, the plasmodiophora brassicae can survive in soil for more than 10 years, and chemical prevention and treatment are extremely difficult. The breeding and application of disease-resistant varieties are the fundamental way to solve the clubroot disease. Molecular marker assisted breeding is an effective means for breeding clubroot-resistant Chinese cabbage varieties. There are 8 clubroot-resistant genes reported for Chinese cabbage, which are Crr1, Crr2, Crr3, Crr4, CRa, CRb, CRc and CRk (Matsumoto et al, 1998; Piao et al, 2002, 2004; Suwabe et al, 2003, 2006; Hirai et al, 2004; Saito et al, 2006; Sakamoto et al, 2008), wherein Crr1 is located at A8 linkage group, Crr2 is located at A1 linkage group, Crr4 is located at A6 linkage group, CRc is located at A2 linkage group, and Crr3, CRa, CRb, CRk are located at A3 linkage group. The inventor uses 8 molecular marker primers related to the issued clubroot disease-resistant genes to carry out molecular marker screening and utilization on the disease-resistant Chinese cabbage material, and currently, a plurality of markers such as KBrH129J18R and the like can be used for clubroot disease resistance screening, but the existing clubroot disease-resistant molecular markers cannot mark a plurality of disease-resistant varieties with similar disease-resistant types such as Degao CR117, Kanggen No. 51 and the like, so that the transformation and screening utilization of the disease-resistant genes of the varieties are hindered. Therefore, the development and application of the molecular marker for resisting clubroot of the Degao CR117 type variety have important significance for the breeding of resisting clubroot of the Chinese cabbage.
The utilization of the existing De-Gao CR117 type clubroot disease-resistant gene is the selection of the traditional clubroot disease inoculation identification, and the selection of the anti-clubroot disease character of the filial generation separated by hybridization or selfing only depends on manual inoculation identification, so that the identification period is long, the risk of germ diffusion exists, the disease resistance of the disease-resistant variety to the clubroot germ of the Chinese cabbage is shown as partial disease resistance, namely the morbidity and the disease index can not reach 0, and the reliability of the selection result of the inoculation identification can not be ensured.
Disclosure of Invention
In view of the above, the invention aims to provide a molecular marker closely linked with the anti-clubroot property of the degao CR117 Chinese cabbage and an application thereof, wherein the molecular marker can accurately screen the anti-clubroot property of the degao CR117 Chinese cabbage and has the characteristics of simplicity and rapidness.
In order to achieve the above object, the present invention provides the following technical solutions:
the invention provides an Indel molecular marker P24 closely linked with the anti-clubroot character of Degao CR117 Chinese cabbage, and the Indel molecular marker P24 has a nucleotide sequence shown as SEQ ID NO.1 in a sequence table.
The invention provides a primer pair for amplifying an Indel molecular marker P24, which comprises a forward primer and a reverse primer, wherein the forward primer has a nucleotide sequence shown as SEQ ID NO.2 in a sequence table; the reverse primer has a nucleotide sequence shown as SEQ ID NO.3 in the sequence table.
The invention provides a kit for screening the anti-clubroot property of the delta CR117 Chinese cabbage, which comprises a primer pair.
The invention provides an application of the Indel molecular marker P24, the primer pair or the kit in screening the Degao CR117 Chinese cabbage and similar Chinese cabbage varieties with the anti-clubroot property;
the similar Chinese cabbage variety comprises Luxin Jiangen root, Zhenzhi 100 or Kanggen No. 51.
Preferably, the screening method comprises the following steps:
(1) carrying out PCR amplification on samples of the variety of the Chinese cabbage of Degao CR117 and the similar Chinese cabbage to be screened by using the primer pair to obtain a PCR product;
(2) and (3) carrying out SDS-PAGE gel electrophoresis on the PCR product, judging a sample generating a 161bp electrophoresis band as a Degao CR117 Chinese cabbage anti-clubroot character, and judging a sample generating a 154bp electrophoresis band as a Degao CR117 Chinese cabbage material susceptible to the clubroot character.
Preferably, the reaction procedure of the PCR amplification in the step (1) is pre-denaturation at 94 ℃ for 5min, pre-denaturation at 94 ℃ for 45s, annealing at 54 ℃ for 30s, extension at 72 ℃ for 45s, 35 cycles, and extension at 72 ℃ for 10 min.
Preferably, the reaction system for the PCR amplification in step (1) is as follows:
Figure BDA0001634221950000021
Figure BDA0001634221950000031
preferably, the concentration of the SDS-PAGE gel in the step (2) is 6-8%.
Preferably, the delta CR117 Chinese cabbage or the delta CR117 similar disease-resistant Chinese cabbage variety with the anti-clubroot trait also comprises an inbred line.
The invention provides an Indel molecular marker P24 closely linked with the anti-clubroot character of Degao CR117 Chinese cabbage, and the Indel molecular marker P24 has a nucleotide sequence shown as SEQ ID NO.1 in a sequence table. The Indel molecular marker P24 is closely linked with the anti-clubroot property of the German high CR117 Chinese cabbage, and generates a strip which is obviously different from the German high CR117 Chinese cabbage material with the property of being susceptible to the clubroot, and the identification is carried out according to the strip with a specific size. 47 parts of Indel molecular marker P24 provided by the invention represent a high-sensitivity and high-resistance inbred line for verification, and the result shows that the accuracy rate of the anti-clubroot character of the German high CR117 Chinese cabbage screened by adopting the Indel molecular marker P24 provided by the invention is high, and the accuracy rate reaches 100%.
The Indel molecular marker P24 provided by the invention is applied to screening of a similar Chinese cabbage variety of the German high CR117 Chinese cabbage with the anti-clubroot property; the similar Chinese cabbage variety comprises Luxin Jiangen root, Zhenzhi 100 or Kanggen No. 51. The developed application of the molecular marker solves the problem of effective utilization of clubroot-resistant Chinese cabbage disease-resistant genes such as Degao CR117 and the like. The identification period of the marker on the clubroot-resistant character is shortened, the problem of germ pollution diffusion does not exist, and the identification result is accurate. The effect of the embodiment proves that the screening accuracy is up to 100%, and meanwhile, the screening operation is simple and convenient, the cost is low, and the repeatability is good. The identification period of the application is 8-14 d.
Drawings
FIG. 1 is an electropherogram of a small population of samples from example 1 using the Indel molecular marker P24;
FIG. 2 is a graph showing the identification of inbred lines in example 2 using the Indel molecular marker P24.
Detailed Description
The invention provides an Indel molecular marker P24 closely linked with the anti-clubroot character of Degao CR117 Chinese cabbage, and the Indel molecular marker P24 has a nucleotide sequence shown as SEQ ID NO.1 in a sequence table. The Indel molecular marker P24 has difference in expression fragment size in the anti-clubroot and clubroot-susceptible Degao CR117 Chinese cabbage material, the Degao CR117 Chinese cabbage material with the anti-clubroot character generates an electrophoresis band of 161bp, and the Degao CR117 Chinese cabbage material with the clubroot-susceptible character generates an electrophoresis band of 154 bp.
The invention provides a primer pair for amplifying an Indel molecular marker P24, which comprises a forward primer and a reverse primer, wherein the forward primer has a nucleotide sequence shown as SEQ ID NO.2 in a sequence table; the reverse primer has a nucleotide sequence shown as SEQ ID NO.3 in the sequence table. The source of the primer is not particularly limited in the present invention, and a primer pair known in the art may be used. In the embodiment of the invention, the primer pair is synthesized by Competition Biotechnology engineering (Shanghai) corporation.
The invention provides a kit for screening the anti-clubroot property of the delta CR117 Chinese cabbage, which comprises a primer pair. The kit also comprises a conventional reagent for detecting the anti-clubroot property of the delta CR117 Chinese cabbage by adopting PCR.
The invention provides an application of the Indel molecular marker P24, the primer pair or the kit in screening the Degao CR117 Chinese cabbage and similar Chinese cabbage varieties with the anti-clubroot property; the similar Chinese cabbage variety comprises Luxin Jiangen root, Zhenzhi 100 or Kanggen No. 51.
In the present invention, the screening method preferably comprises the following steps:
(1) carrying out PCR amplification on the Degao CR117 Chinese cabbage sample to be screened by using the primer pair to obtain a PCR product;
(2) and (3) carrying out SDS-PAGE gel electrophoresis on the PCR product, judging a sample generating a 161bp electrophoresis band as a material with the anti-clubroot property of the Degao CR117 Chinese cabbage, and judging a sample generating a 154bp electrophoresis band as a material with the susceptibility to the clubroot property of the Degao CR117 Chinese cabbage.
The primer pair is used for carrying out PCR amplification on a Dagao CR117 Chinese cabbage sample to be screened, and the obtained PCR product is the Indel molecular marker P24. In the present invention, the reaction procedure of the PCR amplification is preferably 94 ℃ pre-denaturation for 5min, 94 ℃ pre-denaturation for 45s, 54 ℃ annealing for 30s, 72 ℃ extension for 45s, 35 cycles, and 72 ℃ extension for 10 min. The reaction system for PCR amplification is preferably as follows:
Figure BDA0001634221950000041
Figure BDA0001634221950000051
after obtaining the PCR product, the invention carries out SDS-PAGE gel electrophoresis on the PCR product, a sample generating an electrophoresis band of 161bp is judged to be the material with the anti-clubroot property of the German high CR117 Chinese cabbage, and a sample generating an electrophoresis band of 154bp is judged to be the material of the German high CR117 Chinese cabbage with the susceptibility to the clubroot property.
The concentration of the SDS-PAGE gel is preferably 5% to 8%, more preferably 6%. The method for preparing SDS-PAGE gel according to the present invention is not particularly limited, and a preparation method known to those skilled in the art may be used. The voltage of the SDS-PAGE gel electrophoresis is preferably 1500V to 2200V, more preferably 2000V. The current of the SDS-PAGE gel electrophoresis is preferably 40-80 mA, and more preferably 60 mA. The time of the SDS-PAGE gel electrophoresis is preferably 45-90 min, and more preferably 60 min.
In the present invention, after the SDS-PAGE gel is electrophoresed, it is preferable to stain the SDS-PAGE gel. The staining is preferably silver staining. The silver staining method of the present invention is not particularly limited, and silver staining methods well known in the art may be used. And after obtaining the SDS-PAGE gel after silver staining, observing the size of an amplification band of each sample according to the bands of a Marker in the gel, and judging the result. The sequence of the 161bp electrophoresis strip is specifically shown as a nucleotide sequence shown as SEQ ID NO.1 in a sequence table. The sequence of the 154bp electrophoresis strip is specifically shown as a nucleotide sequence shown as SEQ ID NO.4 in a sequence table.
In the invention, the De-Gao CR117 Chinese cabbage or the De-Gao CR117 similar disease-resistant Chinese cabbage variety with the anti-clubroot disease property preferably further comprises an inbred line.
The Indel molecular marker P24 linked to the anti-clubroot trait of dhodh CR117 chinese cabbage, the kit and the use thereof provided by the present invention will be described in detail with reference to the following examples, but they should not be construed as limiting the scope of the present invention.
Example 1
Preparation of test materials
And performing club root disease inoculation identification on the high CR117 Chinese cabbage F2 population, the high-generation disease-resistant inbred line and the susceptible inbred line in 2016, 9 and 19 days, investigating the onset condition of the club root disease in 10 and 28 days, selecting high-susceptible and high-resistant F2 single plants and the high-susceptible and high-resistant inbred lines to extract genome DNA, and entrusting a gene company to perform genome re-sequencing. And designing a primer according to a sequencing result. The F2 disease-resistant and disease-susceptible single plants are used for carrying out small group (table 1) verification, 11 disease-resistant F2 single plants, 11 disease-susceptible F2 single plants, 1 disease-susceptible high-generation inbred line and 1 disease-resistant high-generation inbred line are selected for small group verification, and the results are shown in figure 1; the results are shown in FIG. 2, which are confirmed by the existing disease-resistant and susceptible inbred lines (Table 2).
TABLE 1 Small population verification
Figure BDA0001634221950000061
Figure BDA0001634221950000071
TABLE 2 inbred line identification
Figure BDA0001634221950000072
Figure BDA0001634221950000081
Figure BDA0001634221950000091
FIG. 1 is an electropherogram of P24 versus a small population. As shown in figure 1, 1-11 are disease-resistant F2 individuals, 12-22 are susceptible F2 individuals, 23 are susceptible high-generation inbred lines, and 24 are disease-resistant high-generation inbred lines.
FIG. 2 is the P24 self-bred line identification map. 47 parts of materials 1,2,3,5,6,7,8,15 and 42 are self-bred materials for diseases; 16 is a hybrid material, and 43 is an anti-clubroot material of other genotypes.
Therefore, the Indel molecular marker P24 and the primer pair provided by the invention can effectively solve the problem of screening the anti-clubroot characteristics of the De-Gao CR117 and similar varieties, and the screening result is accurate and reliable.
The foregoing is only a preferred embodiment of the present invention, and it should be noted that, for those skilled in the art, various modifications and decorations can be made without departing from the principle of the present invention, and these modifications and decorations should also be regarded as the protection scope of the present invention.
Sequence listing
<110> Qingdao city institute of agricultural science
<120> Indel molecular marker P24 linked with anti-clubroot trait of Degao CR117 Chinese cabbage, kit and application thereof
<160> 4
<170> SIPOSequenceListing 1.0
<210> 1
<211> 161
<212> DNA
<213> Artificial Sequence (Artificial Sequence)
<400> 1
gttccagtga ctgtggatga cttcgcagaa cctgatatct gaaaaaaatt aattacaaga 60
cagtttagtc aaagtattag ctcataagca aattagttaa agatcatttc aaacaaagaa 120
cgaataacgt tacctttcca atagcaaccc atctctcatc t 161
<210> 2
<211> 23
<212> DNA
<213> Artificial Sequence (Artificial Sequence)
<400> 2
gttccagtga ctgtggatga ctt 23
<210> 3
<211> 23
<212> DNA
<213> Artificial Sequence (Artificial Sequence)
<400> 3
agatgagaga tgggttgcta ttg 23
<210> 4
<211> 154
<212> DNA
<213> Artificial Sequence (Artificial Sequence)
<400> 4
gttccagtga ctgtggatga cttcgcagaa cctgatatct gaaaaaaata aattacaaaa 60
cagtttagtc aacgtataag ctcatcagca aattagttaa agatcatttc aaacaaaaaa 120
cgttaccttt ccaatagcaa cccatctctc atct 154

Claims (6)

1. The Indel molecular marker P24 closely linked with the anti-clubroot property of the German high CR117 Chinese cabbage is characterized in that the nucleotide sequence is shown as SEQ ID NO.1 in the sequence table.
2. Use of the Indel molecular marker P24 of claim 1, a primer pair for amplifying the Indel molecular marker P24 of claim 1, or a kit comprising the primer pair, for screening dhodra CR117 chinese cabbage with anti-clubroot trait; the primer pair comprises a forward primer and a reverse primer, and the nucleotide sequence of the forward primer is shown as SEQ ID NO.2 in a sequence table; the nucleotide sequence of the reverse primer is shown as SEQ ID NO.3 in the sequence table;
the screening method comprises the following steps:
(1) carrying out PCR amplification on the Degao CR117 Chinese cabbage sample to be screened by using the primer pair to obtain a PCR product;
(2) and (3) carrying out SDS-PAGE gel electrophoresis on the PCR product, judging a sample generating an electrophoresis band of 161bp as the Degao CR117 Chinese cabbage material with the anti-clubroot character, and judging a sample generating an electrophoresis band of 154bp as the Degao CR117 Chinese cabbage material with the susceptibility to the clubroot character.
3. The use of claim 2, wherein the reaction procedure of the PCR amplification in step (1) is as follows: pre-denaturation at 94 ℃ for 5min, pre-denaturation at 94 ℃ for 45s, annealing at 54 ℃ for 30s, extension at 72 ℃ for 45s, 35 cycles, and extension at 72 ℃ for 10 min.
4. The use according to claim 2 or 3, wherein the total volume of the reaction system for PCR amplification in step (1) is 10 μ l, and comprises the following components:
Figure FDA0002885267370000011
Figure FDA0002885267370000021
5. the use according to claim 2, wherein the concentration of the SDS-PAGE gel in step (2) is between 6% and 8%.
6. The use of claim 2, wherein said delta CR117 Chinese cabbage having anti-clubroot trait further comprises a selfed plant.
CN201810354431.6A 2018-04-19 2018-04-19 Indel molecular marker P24 linked with anti-clubroot property of Degao CR117 Chinese cabbage, kit and application thereof Active CN108315470B (en)

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Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2012039445A1 (en) * 2010-09-22 2012-03-29 独立行政法人農業・食品産業技術総合研究機構 Method for producing cruciferous plant resistant to clubroot
CN105543391A (en) * 2016-02-05 2016-05-04 北京市农林科学院 InDel molecular marker for identifying clubroot-resistant QTL (quantitative trait locus) located on Chinese cabbage A03 chromosome and application thereof

Patent Citations (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2012039445A1 (en) * 2010-09-22 2012-03-29 独立行政法人農業・食品産業技術総合研究機構 Method for producing cruciferous plant resistant to clubroot
CN105543391A (en) * 2016-02-05 2016-05-04 北京市农林科学院 InDel molecular marker for identifying clubroot-resistant QTL (quantitative trait locus) located on Chinese cabbage A03 chromosome and application thereof

Non-Patent Citations (4)

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Title
28个大白菜品种对根肿菌不同菌株的抗性反应及抗病基因位点检测;曾令益等;《中国油料作物学报》;20171231;第39卷(第4期);第532-639页 *
Identification and Characterization of Crr1a, a Gene for Resistance to Clubroot Disease (Plasmodiophora brassicae Woronin) in Brassica rapa L.;Katsunori Hatakeyama等;《PLoS One》;20130130;第8卷(第1期);e54745 *
Linkage map construction using InDel and SSR markers and QTL analysis of heading traits in Brassica oleracea var. capitata L.;Hong Hao Lv等;《Molecular Breeding》;20140731;第34卷(第1期);第87-98页 *
大白菜根肿病抗性基因的标记和定位;王彤彤等;《中国蔬菜》;20121231(第14期);第31-35页 *

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