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碱裂解法快速提取口腔拭子DNA对CHRNA3基因多态性的研究
引用本文:朱伟锋,刘卓琦,吴金兰,余乐涵,万福生.碱裂解法快速提取口腔拭子DNA对CHRNA3基因多态性的研究[J].重庆医学,2012,41(8):764-765,768,724.
作者姓名:朱伟锋  刘卓琦  吴金兰  余乐涵  万福生
作者单位:朱伟锋 (南昌大学研究生院医学部,江西南昌,330006) ; 刘卓琦 (南昌大学医学院生物化学与分子生物学教研室,江西南昌,330006) ; 吴金兰 (南昌大学研究生院医学部,江西南昌,330006) ; 余乐涵 (南昌大学医学院生物化学与分子生物学教研室,江西南昌,330006) ; 万福生 (南昌大学研究生院医学部,江西南昌,330006) ;
基金项目:江西省科技支撑计划资助项目
摘    要:目的建立一种快速的从口腔拭子中提取DNA的方法,研究其在尼古丁乙酰胆碱受体α3(CHRNA3)基因多态性分析中的应用。方法以NaOH和乙二胺四乙酸(EDTA)配制碱裂解液,以三羟甲基氨基甲烷-EDTA(TE)为中和液,经加热裂解和中和两步提取口腔拭子DNA。以提取的DNA为模板,用聚合酶链式反应-限制性片段长度多态性(PCR-RFLP)分析对CHRNA3基因的rs6495309进行分型。对不同基因型的样本测序验证。结果 PCR扩增和酶切的靶带清晰,无非特异性条带。酶切结果与测序结果吻合。结论碱裂解法提取口腔拭子DNA具有快速、简便、经济、可靠的特点,可以用于CHRNA3基因多态性的分析。

关 键 词:多态性  限制性片段长度  序列分析  DNA  口腔拭子  尼古丁乙酰胆碱受体α3  碱裂解

Rapid DNA extraction from buccal swabs by alkaline lysis method for study of CHRNA3 gene polymorphism
Zhu Weifeng,Liu Zhuoqi,Wu Jinlan,Yu Lehan,Wan Fusheng.Rapid DNA extraction from buccal swabs by alkaline lysis method for study of CHRNA3 gene polymorphism[J].Chongqing Medical Journal,2012,41(8):764-765,768,724.
Authors:Zhu Weifeng  Liu Zhuoqi  Wu Jinlan  Yu Lehan  Wan Fusheng
Institution:2,3(1.Faculty of Medical Sciences,Graduate School;2.Department of Biochemistry and Molecular Biology,School of Medicine; 3.Department of Laboratory Animal Science,Nanchang University,Nanchang,Jiangxi 330006,China)
Abstract:Objective To establish a rapid method for DNA extraction from buccal swabs and investigate its application in analysis of cholinergic receptor nicotinic alpha3(CHRNA3) gene polymorphism.Methods Lysis solution was made from NaOH and ethylenediaminetetraacetic acid(EDTA),and tris(hydroxymethyl)aminomethane-EDTA(TE) was served as neutralizing solution.DNA was extracted from buccal swabs via two steps:heating and neutralizing.rs6495309 in CHRNA3 gene was genotyped by polymerase chain reaction-restriction fragment length polymorphism(PCR-RFLP) assay using templates of extracted DNA.The samples of different genotypes were confirmed by direct sequencing analysis of PCR products.Results The target DNA bands obtained by PCR amplification and enzyme digestion were clear,and no nonspecific band was detected.The results of PCR-RFLP agreed well with the results of direct sequencing.Conclusion The alkaline lysis method for preparation of DNA from buccal swabs is rapid,simple,economical,reliable,and can be used for analysis of CHRNA3 gene polymorphism.
Keywords:polymorphism  restriction fragment length  sequence analysis  DNA  buccal swab  cholinergic receptor nicotinic alpha3  alkaline lysis
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