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首页> 外文期刊>International Journal of Legal Medicine >Validation of the PLEX-IDTM mass spectrometry mitochondrial DNA assay
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Validation of the PLEX-IDTM mass spectrometry mitochondrial DNA assay

机译:验证PLEX-IDTM质谱线粒体DNA测定

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摘要

For very challenged biological samples, mitochondrial DNA (mtDNA) analysis can often provide results when the more traditional nuclear DNA markers fail. While reliable, the current method of mtDNA analysis by Sanger sequencing is expensive, labor-intensive, and time-consuming and is limited by its inability to quantify mixed samples. The Abbott PLEX-ID™ instrument, which enables analysis of mtDNA amplicons via electrospray ionization mass spectrometry (ESI-MS), produces comparable accuracy and sensitivity while offering a faster and less expensive alternative to Sanger sequencing. Unlike Sanger sequencing, this system is capable of quantifying DNA species and thus may be exploited for evaluating heteroplasmy and, possibly, mixture deconvolution. Validation studies of the PLEX-ID™ mtDNA assay confirmed that the instrument is highly sensitive and capable of yielding reproducible results. Samples commonly encountered in a forensic setting, as well as population samples, were typed correctly. The PLEX-ID™ mtDNA assay yields reliable results for single-source samples, which are the same sample types currently examined in forensic laboratories via Sanger sequencing, at a level that meets or exceeds that of the current method. While the instrument has the demonstrated capability to quantify mixed samples, the specific assay design for mtDNA analysis can be used only in a limited fashion to analyze mixtures due to the formation of chimeric mtDNA products.
机译:对于具有挑战性的生物样品,当更传统的核DNA标记失效时,线粒体DNA(mtDNA)分析通常可以提供结果。虽然可靠,但目前通过Sanger测序进行mtDNA分析的方法昂贵,费力且费时,并且由于无法定量混合样品而受到限制。雅培PLEX-ID™仪器可通过电喷雾电离质谱(ESI-MS)分析mtDNA扩增子,可提供相当的准确性和灵敏度,同时提供了更快,更便宜的Sanger测序方法。与Sanger测序不同,该系统能够定量DNA种类,因此可用于评估异质性,并可能用于混合物反褶积。对PLEX-ID™mtDNA分析的验证研究证实,该仪器高度灵敏,能够产生可重复的结果。正确键入法医环境中常见的样本以及总体样本。 PLEX-ID™mtDNA分析可为单源样品提供可靠的结果,这些样品与法医实验室目前通过Sanger测序检测的样品类型相同,其水平可达到或超过当前方法的水平。尽管该仪器具有定量混合样品的能力,但由于嵌合mtDNA产物的形成,用于mtDNA分析的特定分析设计只能以有限的方式用于分析混合物。

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