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首页> 外文期刊>Journal of Molecular Diagnostics >Template-Directed Dye-Terminator Incorporation with Fluorescence Polarization Detection for Analysis of Single Nucleotide Polymorphisms Implicated in Sepsis
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Template-Directed Dye-Terminator Incorporation with Fluorescence Polarization Detection for Analysis of Single Nucleotide Polymorphisms Implicated in Sepsis

机译:模板导向的染料终结剂与荧光偏振检测相结合,用于分析脓毒症中涉及的单核苷酸多态性

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Sepsis continues to be a common source of morbidity and mortality in critically ill patients. Single nucleotide polymorphisms (SNPs) present in genes encoding inflammatory mediators have been associated with predisposition and outcome in this syndrome. The use of high throughput SNP analysis in large epidemiological studies is necessary to more fully understand the genetic underpinnings of this disease. We adapted template-directed dye-terminator incorporation with fluorescence polarization detection (TDI-FP) to the analysis of eight SNPs implicated in mediating the sepsis syndrome: TNF- (-308), TNF- (-238), TNF-ß (+250), IL-1ß (+3953), IL-6 (-174), IL-10 (-592), plasminogen activator inhibitor-1 (PAI-1 (-675)), and TLR4 299 (+1032). Optimization of PCR, amplicon purification, and template-directed dye-terminator incorporation reactions were necessary to achieve acceptable performance characteristics for these assays. Sequence validated samples served as controls. Using this method we were able to assign genotype in 99.3% of assays and identified 64 unique genotypes in samples obtained from 90 individuals. TDI-FP is a flexible and robust method of SNP detection that can be optimized in a systematic fashion. This method has potential advantages compared with other high throughput genotyping techniques and appears well suited to clinical situations requiring analysis of large numbers of samples.
机译:脓毒症仍然是重症患者发病率和死亡率的常见来源。存在于编码炎症介质的基因中的单核苷酸多态性(SNP)与该综合征的易感性和预后相关。在大型流行病学研究中使用高通量SNP分析对于更全面地了解这种疾病的遗传基础非常必要。我们将模板导向的染料终止剂与荧光偏振检测(TDI-FP)结合使用,以分析涉及介导败血症综合征的8个SNP:TNF-(-308),TNF-(-238),TNF-ß(+ 250),IL-1ß(+3953),IL-6(-174),IL-10(-592),纤溶酶原激活物抑制剂1(PAI-1(-675))和TLR4 299(+1032)。 PCR,扩增子纯化和模板指导的染料终止剂掺入反应的优化是实现这些测定可接受的性能特征所必需的。经序列验证的样品用作对照。使用这种方法,我们能够在99.3%的测定中分配基因型,并从90个个体中鉴定出64种独特的基因型。 TDI-FP是一种灵活而强大的SNP检测方法,可以系统地对其进行优化。与其他高通量基因分型技术相比,该方法具有潜在优势,并且似乎非常适合需要分析大量样品的临床情况。

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