Molecular marker InDeL_33 of main-effect QTL (quantitative trait locus) of soybean hundred-grain weight and application of molecular marker InDeL_33
A molecular marker, 100-grain weight technology, used in recombinant DNA technology, microbial assay/inspection, DNA/RNA fragments, etc.
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Embodiment 1
[0038] Example 1: Acquisition of main effect QTL for 100-grain weight in soybean
[0039] (1) 'NJRINP' group building
[0040]The hybrid F 1 , construct the population through the "single-seed transmission" method, and obtain 284 F 2:8 Generation of recombinant inbred lines ('NJRINP').
[0041] The steps of the "single-seed transmission" method are as follows: a seed harvested from the female plant in the present generation of parental parental hybridization grows into a F1 generation single plant, and its self-crossing (ie self-pollination) yields a F1 plant. 2 generation seeds, the latter is planted to grow into a F2 generation line containing segregation traits, and each individual plant of it is self-fertile and harvests F 3 For generation seeds, the isolated plants of the same traits are harvested and threshed into bags, and each seed is planted separately in the next year. 3 F 4 Generation seeds, ... until the characters of different plants in each family are comple...
Embodiment 2
[0049] Example 2: Acquisition of the main QTL tight marker InDeL_33 for 100-grain weight in soybean
[0050] (1) Molecular marker development
[0051] Using the published soybean physical map information and the sequence information of the sequencing materials of the National Soybean Improvement Center, multiple molecular markers were designed in the Gm11:2261898bp-65p77664bp region of chromosome 11.
[0052] (2) Secondary population molecular marker identification
[0053] Use the kit to extract the genomic DNA of the leaves of NJRINP-derived secondary population soybean material, PCR reaction system (10ul), which contains 3ul DNA template (15ng), upstream and downstream primers (0.2mmol / L) each 1.5ul, 1.2ulMgCl 2 (2.5mmol / L), 0.24uldNTP (10mmol / L, N=A, C, G, T), 0.12ulTaq enzyme (5U / ul) and 1.4ulddH 2 O. PCR reaction program: denaturation at 95°C for 5 min; followed by 35 cycles of denaturation at 94°C for 30 s, annealing at 55°C for 40 s, extension at 72°C for 50 s; exte...
Embodiment 3
[0058] Embodiment 3: the application of InDeL_33 molecular marker on the selection of soybean 100-grain weight
[0059] (1) Genome amplification detection of both parents
[0060] The parents used to verify the QTL of soybean 100-kernel weight were the parent Nannong 86-4 (the InDeL_33 allele band was 100bp, the 100-kernel weight was 18.46g), the parent NP-7 (the InDeL_33 allele band was 120bp, the 100-kernel weight is 8.16g).
[0061] (2) Population amplification detection and marker analysis
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