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作 者:贾琳娜[1] 王小怡[1] 王博[1] 郭大玮[1] JIA Linna WANG Xiaoyi WANG Bo GUO Dawei.(School of Forensic Medicine, Shanxi Medical University, Taiyuan 030001, Shanxi, China)
出 处:《中国性科学》2017年第1期154-157,共4页Chinese Journal of Human Sexuality
摘 要:目的:研究位于H19转录起始点-3390 bp的HhaI位点是否为差异甲基化位点,为精子DNA识别提供新依据。方法:从51份血样和20份精子样本提取基因组DNA,每个样本分别在同一反应体系中进行甲基化敏感酶HhaI消化和荧光定量PCR反应(MSRE-qPCR),扩增包含上述HhaI位点的114 bp片段。得到每个样本酶切前后的Ct值,用2^(-△△Ct)计算各样本酶切前后模板DNA相对表达量,将其作为DNA甲基化水平。结果:51份血样中该HhaI位点甲基化水平为(44.4±23.8)%,20份精子DNA甲基化水平为(120.5±52.5)%,差异有统计学意义(P<0.001)。结论:甲基化水平高于94%可识别精子DNA,H19差异甲基化区114 bp序列的MSRE-qPCR分析为精子DNA的识别提供了一种新方法。Objectives: To study whether HhaI site,located at the transcription start point- 3390 bp of H19 gene,was differentially methylated site,to provide basis for sperm DNA identification. Methods: These genomic DNA were extracted from 51 blood samples and 20 semen samples,and then every DNA sample was subjected to digestion by a methylationsensitive restriction endonuclease HhaI and qPCR in the same reaction system to amplify the 114 bp target fragment which contained the Hha I site. The Ct of digested group and undigested group were determined from each sample. The DNA methylation level was described by 2^(-△△Ct). Results: DNA methylation level in this HhaI site was 44. 4 % ± 23. 8% in 51 blood samples and 120. 5% ± 52. 5% in 20 semen samples. The difference was of statistical significance( P ﹤ 0. 001). Conclusion: Sperm DNA could be identified if H19 HhaI site methylation level is over 94%. MSRE- qPCR analysis on 114 bp H19 differentially methylated regions is a newmethod to identify sperm DNA.
关 键 词:H19差异甲基化 甲基化敏感性限制性内切酶 实时定量PCR 精子DNA
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