SSR primers used for analysis of genetic diversity and genetic relationship of curvularia lunata and application
A technique of genetic diversity and kinship, which is applied in the field of SSR primers and application fields for the analysis of genetic diversity and kinship of Curvularia crescens, achieves the effects of easy use, shortened analysis cycle, and improved research efficiency
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Embodiment 1
[0069] Embodiment 1SSR primer development
[0070] (1) Analysis of genomic SSR loci and primer design
[0071] Download the whole genome sequence of Curvularia lunata from the NCBI (National Center for Biotechnology Information) website, use MISA software to search for SSR sites of 2 to 6 nucleotides in the genome sequence, and the search condition is 2 nucleotides The number of repetitions must be ≥6, and the number of repetitions of 3 to 6 nucleotides must be ≥5. Then extract the 200 bp sequence upstream and downstream of the SSR site, and use Primer 5.0 software to design SSR primers, setting parameters: primer length 20-24 bp, annealing temperature 50-65 °C, GC content 40-60%, PCR product length 150-350 bp. Primers were synthesized by Sangon Bioengineering (Shanghai) Co., Ltd.
[0072] (2) DNA extraction and PCR
[0073] 6 strains of Curvularia lunata with different geographical distribution (CL17-27, CL15-27, CL17-30, CL17-35, CL17-64 and CL15-16, see Table 3 for detai...
Embodiment 2
[0088] Example 2 Using SSR primers to analyze the genetic diversity of different populations of Curvularia lunene
[0089] (1) Tested strains and medium
[0090] 24 strains of Curvularia crescens were isolated from diseased plants in the cornfields of Shangqiu City, Zhoukou City and Zhumadian City in Henan Province by tissue separation method (Table 3), then purified by single spore isolation, and transferred to a PDA slope at 4 °C Save it. The medium used was potato dextrose agar (PDA) medium: 200 g of potatoes, 20 g of glucose, 15 g of agar, and 1 L of distilled water.
[0091] Table 3 Information of 24 strains of Curvularia lunene
[0092]
[0093]
[0094] (2) DNA extraction and PCR
[0095] The specific operation is the same as in Example 1, and the amplification primers are CL-SSR2, CL-SSR6, CL-SSR7, CL-SSR19, CL-SSR24, CL-SSR29, CL-SSR35, CL-SSR37, CL-SSR42 and CL-SSR45 ;
[0096] (3) Genetic diversity analysis of different populations of Curvularia lunene
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Embodiment 3
[0101] Example 3 Utilizes SSR primers to analyze the phylogenetic relationship between Curvularia lunata strains
[0102] (1) test bacterial strain and culture medium are with embodiment 2;
[0103] (2) The specific operation of DNA extraction and PCR is the same as in Example 1, and the amplification primers are CL-SSR2, CL-SSR6, CL-SSR7, CL-SSR19, CL-SSR24, CL-SSR29, CL-SSR35, CL-SSR37 , CL-SSR42 and CL-SSR45;
[0104] (3) Genetic relationship analysis between Curvularia lunata strains
[0105] According to 10 pairs of SSR primers (CL-SSR2, CL-SSR6, CL-SSR7, CL-SSR19, CL-SSR24, CL-SSR29, CL-SSR35, CL-SSR37, CL-SSR42 and CL-SSR45), 24 new The results of PCR amplification of Curvularia lunata were calculated using NTSYSpc2.10 software to calculate the genetic similarity coefficient (Table 5) between the strains, and the UPGMA method was used to cluster and build a phylogenetic tree ( image 3 ). According to the genetic similarity coefficient between the strains or the phylo...
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