A kind of detection mtrr gene snp site genotyping pcr primer and method
A genotyping and genotyping technology, applied in biochemical equipment and methods, DNA/RNA fragments, recombinant DNA technology, etc., can solve problems such as incompleteness and low efficiency of PCR products, and achieve high accuracy and ensure accuracy. , the effect of easy operation
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Embodiment 1
[0056] Example 1 Design of primers for detecting genotyping of MTRR gene rs1801394 polymorphism site
[0057] In this embodiment, a pair of primers are designed to obtain the sequence of 1000bp before and after the polymorphic site of MTRR gene rs1801394 (see figure 2 ), wherein the base sequence of the 6121-7260th position of the MTRR gene is shown in SEQ ID NO: 16, and specific typing primers are designed for the SNP site of rs1801394 according to the sequence. Among them, the 3' end of the forward primer is adjacent to the polymorphic site, and the penultimate 3rd base is C, so as to realize the introduction of a recognition sequence through PCR amplification C ATRTG, where C Introduced by a mismatched base, the corresponding sequence of the wild-type allele A is C ATATG, which can be recognized and cleaved by NdeI or isoschizase; the corresponding sequence of the mutant allele G is CATGTG cannot be recognized and cleaved by restriction endonuclease NdeI or isozyzyme, s...
Embodiment 2
[0064] Example 2 A method for detecting the genotype of the rs1801394 polymorphic site of the MTRR gene
[0065] 1) Genomic DNA extraction
[0066] Genomic DNA of human oral epithelial cells was extracted by using Tiangen's buccal swab genomic DNA extraction kit according to the instructions. The DNA source is not limited thereto, and any somatic cell-derived DNA is acceptable.
[0067] 2) PCR amplification of the target fragment
[0068] PCR reaction system:
[0069]
[0070]
[0071] PCR reaction conditions:
[0072]
[0073] PCR products were identified by 1.5% agarose gel electrophoresis.
[0074] 3) Restriction typing of PCR products
[0075] The restriction endonuclease used in this example is Thermo Scientific fast restriction endonuclease NdeI.
[0076] The total volume of the enzyme digestion system is 30 μL, and the specific formula is as follows:
[0077]
[0078] The amount (X μL) of the PCR product can be adjusted depending on the concentration ...
Embodiment 3
[0096] Example 3 A method for detecting the genotype of the rs1801394 polymorphic site of the MTRR gene
[0097] 1) Genomic DNA extraction
[0098] Genomic DNA is extracted from the subject's cells.
[0099] 2) PCR amplification of the target fragment
[0100] The forward primer F and the reverse primer R designed in the present invention are used for PCR amplification to obtain PCR primers.
[0101] 3) Restriction typing of PCR products
[0102] The PCR product was digested with restriction endonuclease NdeI. Agarose gel electrophoresis of PCR amplification products Figure 4 , Lanes 1-10 are PCR products, all of which are 478bp in size, and the size of the target band is consistent.
[0103] One of the electrophoresis patterns of the PCR product digested with restriction endonuclease NdeI Figure 5 , P is the PCR product with a size of 478bp; lanes 1-7 are PCR product digestion bands of 7 different samples, among which 1, 2, 4, and 5 are completely digested, and the ge...
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