首页> 外文期刊>Electrophoresis: The Official Journal of the International Electrophoresis Society >FORENSIC APPLICATIONS OF A RAPID, SENSITIVE, AND PRECISE MULTIPLEX ANALYSIS OF THE FOUR SHORT TANDEM REPEAT LOCI HUMVWF31/A, HUMTH01, HUMF13A1, AND HUMFES/FPS
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FORENSIC APPLICATIONS OF A RAPID, SENSITIVE, AND PRECISE MULTIPLEX ANALYSIS OF THE FOUR SHORT TANDEM REPEAT LOCI HUMVWF31/A, HUMTH01, HUMF13A1, AND HUMFES/FPS

机译:四短串联重复序列LOMV HUMVWF31 / A,HUMTH01,HUMF13A1和HUMFES / FPS的快速,灵敏和精确的多重分析法医学应用

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摘要

A system of four short tandem repeat loci (HUMVWF31A, HUMTH01, HUMF13A1, and HUMFES/FPS) has been tested in co-amplification with forensic (post-mortem and post-coital) DNA samples. Semiautomated DNA typing was employed to analyze polymerase chain reaction (PCR) products formed by extension of primers labeled with a fluorescent dye at the 5'-terminus. Most DNA extracts could be typed, although a few required the addition of bovine serum albumin or a pretreatment by ultrafiltration in order to obtain sufficient signal for typing. Balanced signals for the alleles were obtained frequently across the loci, although preferential amplification of HUMTH01 was observed often with the forensic samples. Band splitting due to nontemplate nucleotide addition to the blunt ends of the amplimers was frequently detected for the DNA extracted from the forensic samples. A database was constructed for the African-American population and compared with a Caucasian database. Few differences were observed across the two populations, except at the locus HUMTH01. The fluorescence-based system facilitates large-scale databasing, because the PCR products run off the gel, allowing more than one set of samples to be analyzed per run. Polyacrylamide gel reuse did not diminish genotyping accuracy. [References: 29]
机译:在与法医(验尸和性交后)DNA样本共扩增中,已经测试了四个短串联重复基因座(HUMVWF31A,HUMTH01,HUMF13A1和HUMFES / FPS)的系统。采用半自动DNA分型来分析聚合酶链反应(PCR)产物,该产物是通过在5'端用荧光染料标记的引物延伸而形成的。大多数DNA提取物可以分型,尽管少数需要添加牛血清白蛋白或通过超滤预处理以获得足够的分型信号。尽管经常在法医样本中观察到HUMTH01的优先扩增,但经常在基因座上获得等位基因的平衡信号。对于从法医样品中提取的DNA,经常检测到由于非模板核苷酸添加到扩增子平端而引起的条带分裂。为非裔美国人建立了一个数据库,并与一个白种人数据库进行了比较。除了在基因座HUMTH01以外,在两个种群中几乎没有观察到差异。基于荧光的系统可促进大规模数据库的建立,因为PCR产物从凝胶中流出,每次运行可分析多组样品。聚丙烯酰胺凝胶再利用不会降低基因分型的准确性。 [参考:29]

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