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首页> 外文期刊>Japanese heart journal >Molecular Genetic Diagnosis of a Family with Hypercholesterolemia by a Mismatched PCR-RFLP Method for Genotyping Single Base Substitution of the LDL Receptor Gene
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Molecular Genetic Diagnosis of a Family with Hypercholesterolemia by a Mismatched PCR-RFLP Method for Genotyping Single Base Substitution of the LDL Receptor Gene

机译:通过错配PCR-RFLP方法对LDL受体基因的单碱基取代进行基因匹配的高胆固醇血症家庭的分子遗传学诊断。

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摘要

Plasma lipid and lipoprotein levels reflect in part the influence of relevant genetic loci. Defects at some of these loci account for specific types of dyslipoproteinemia occurring with regularity among family members. In the course of familial investigations of coronary artery disease, we identified an family in which several members were affected with elevated low density lipoprotein (LDL) cholesterol levels. To study the genetic defects responsible for plasma lipoprotein abnormality in this pedigree, we developed a simple method for genotyping a single base substitution that does not affect a restriction recognition enzyme site in exon 10 of the LDL receptor gene. Using our mismatched PCR method, this G- >A substitution at nucleotide 1413 could be genotyped in the form of a biallelic restriction fragment length polymorphism (RFLP) after digestion with restriction enzyme Hpa II. Linkage analysis using this molecular method demonstrated that the defect at the LDL receptor locus is responsible for elevated LDL cholesterol phenotype observed in this family by segregation of defective alleles at the LDL receptor locus with the disease (peak decimal logarithm of odds score >3.0).
机译:血浆脂质和脂蛋白水平部分反映了相关遗传基因座的影响。在这些基因座中的一些基因座上的缺陷是导致家族成员中正常发生的特定类型的血脂蛋白异常的原因。在冠状动脉疾病的家族研究过程中,我们确定了一个家庭,其中几个成员的低密度脂蛋白(LDL)胆固醇水平升高。为了研究该谱系中血浆脂蛋白异常的遗传缺陷,我们开发了一种简单的方法,对不影响LDL受体基因第10外显子的限制性酶切位点的单碱基取代进行基因分型。使用我们的错配PCR方法,可以在用限制酶Hpa II消化后以双等位基因限制性片段长度多态性(RFLP)的形式对核苷酸1413处的G-> A取代进行基因分型。使用这种分子方法的连锁分析表明,LDL受体基因座的缺陷是该家族中观察到的LDL胆固醇表型升高的原因,原因是该病在LDL受体基因座处的缺陷等位基因处于隔离状态(赔率得分的峰值十进制对数> 3.0)。

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