Method for detecting methylation level of synuclein intron 1
A synuclein and level detection technology, applied in the field of bioengineering, can solve the problems of decreased quantitative accuracy, time-consuming and laborious, and incapable of quantitative analysis, and achieve the effects of good quantitative characteristics, convenient operation, and high throughput
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[0041] Example: Application of Pyrosequencing in α-Syn Intron 1 Methylation Detection
[0042] 1. Sodium bisulfite treatment
[0043] Genomic DNA is modified using sodium metabisulfite and hydroquinone to convert unmethylated cytosines to uracils, while methylated uracils remain unchanged. The process is briefly described as follows: first, the genomic DNA was denatured with 0.3mol / L NaOH; then, the genomic DNA was treated at 50°C for 16h with a mixed solution of sodium metabisulfite and hydroquinone (pH 5.0). The DNA was purified with a kit, and 0.3 mol / L NaOH was added to incubate at 37°C for 15 min to terminate the reaction, and finally the DNA was precipitated with ethanol.
[0044] 2. PCR amplification
[0045] Perform PCR amplification according to conventional methods, primers and reaction conditions are as follows:
[0046] Forward amplification primers: GAA, ATG, GAA, GTG, TAA, GGA, GGT, T;
[0047] Reverse amplification primers: Biotin-TTC, TAA, TCC, ATC, CAA, CA...
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