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作 者:刘芳[1,2,3,4] 何丽芳[1,2,3,4] 宁寿葆[1,2,3,4] 任建英 黄伟民
机构地区:[1]上海医科大学儿科医院 [2]山东省立医院儿科 [3]卫生部医学分子病毒学实验室 [4]上海市徐汇区中心医院
出 处:《中华儿科杂志》1997年第5期242-245,共4页Chinese Journal of Pediatrics
基 金:国家自然科学基金
摘 要:为比较和探讨家族性载脂蛋白B100缺陷患者apoB-3500位突变的检测方法,对4个高胆固醇血症家族的19名成员,采用聚合酶链反应(PCR)结合酶切法、等位基因特异寡核苷酸(ASO)探针杂交法及PCR产物序列分析法检测此点突变,并通过定点突变法构建一人工突变体作为阳性对照,以确保试验方法可靠。结果:4个家族19名成员通过PCR结合酶切及ASO探针杂交两种方法皆没有检测到apoB-3500位突变,与测序结果一致;测序结果验证人工构建突变体的10658位核苷酸为A。结论:比较而言,PCR结合酶切法是检测apoB-3500位突变的一种简便而可靠方法;通过设计适当引物在PCR产物中引进酶切位点及构建人工阳性对照的方法,是检测点突变疾病的新思路;apoB-3500位突变不是引起此4个家族成员胆固醇升高的原因。To evaluate the methods for detecting apoB 3500 mutation in familial defective apolipoprotein B 100 (FDB), the authors examined 19 members of 4 familial hypercholesterolemic (FH) families by polymerase chain reaction (PCR) combined with endonuclease cleavage, allele specific oligonucleotide (ASO) hybridization and nucleotide sqeuence analysis. In addition, an artificial positive control was constructed by site dirceted mutagenesis to ensure the reliability of the assay. No apoB 3500 mutation was detected in these 19 members by the three methods, and sequencing showed that the 10658 nucleotide in the constructed mutant DNA was A. These results suggested that the method of PCR combined with endonuclease cleavage was easy to perform and reproducible; the idea of introducing an endonuclease cleavage site and constructing artificial mutant into the PCR product proved to be successful, and the hypercholesterolemia of these 4 FH families was not caused by apoB 3500 mutation.
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