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群体规模基因多态性分析的快速方法:以ACE基因为例。

Rapid methods for population-scale analysis for gene polymorphisms: the ACE gene as an example.

作者信息

O'Dell S D, Humphries S E, Day I N

机构信息

Department of Medicine, University College London Medical School, Rayne Institute.

出版信息

Br Heart J. 1995 Apr;73(4):368-71. doi: 10.1136/hrt.73.4.368.

Abstract

OBJECTIVE

To obtain rapid, high throughput genotyping of the angiotensin converting enzyme (ACE) gene intron 16 insertion/deletion polymorphism.

METHODS

DNA was obtained from whole blood samples by a simple liquid phase methanol extraction procedure. The ACE gene was amplified by the polymerase chain reaction (PCR) using two oligonucleotide primers (ACE1 and ACE3) outside the insertion sequence and one primer (ACE2) inside the sequence. Microtitre array diagonal gel electrophoresis (MADGE) was used to determine genotypes.

RESULTS

84 and 65 bp PCR products indicating the presence of deletion (D) and insertion (I) alleles, respectively, were clearly resolved after electrophoresis on a 7.5% polyacrylamide gel. Up to 480 DNA samples on 5 gels could be genotyped in a single electrophoresis run, or up to 1000 samples in a working day.

CONCLUSIONS

A simplified DNA extraction protocol coupled to the high throughput capability of the MADGE electrophoretic system for genotyping enables analysis of large populations for association studies of ACE genotype with cardiac disease events.

摘要

目的

实现血管紧张素转换酶(ACE)基因内含子16插入/缺失多态性的快速、高通量基因分型。

方法

通过简单的液相甲醇提取程序从全血样本中获取DNA。使用位于插入序列外的两条寡核苷酸引物(ACE1和ACE3)以及位于序列内的一条引物(ACE2),通过聚合酶链反应(PCR)扩增ACE基因。采用微量滴定阵列对角线凝胶电泳(MADGE)确定基因型。

结果

分别指示缺失(D)和插入(I)等位基因存在的84 bp和65 bp PCR产物,在7.5%聚丙烯酰胺凝胶上电泳后清晰可辨。一次电泳运行可对5块凝胶上多达480个DNA样本进行基因分型,或在一个工作日内对多达1000个样本进行基因分型。

结论

结合MADGE电泳系统高通量能力的简化DNA提取方案用于基因分型,能够对大量人群进行分析,以研究ACE基因型与心脏疾病事件的关联性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/518e/483832/de1a0487ce91/brheartj00158-0071-a.jpg

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