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首页> 外文期刊>Radiotherapy and oncology: Journal of the European Society for Therapeutic Radiology and Oncology >Optimisation and validation of methods to assess single nucleotide polymorphisms (SNPs) in archival histological material.
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Optimisation and validation of methods to assess single nucleotide polymorphisms (SNPs) in archival histological material.

机译:优化和验证评估档案组织学材料中单核苷酸多态性(SNP)的方法。

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BACKGROUND AND PURPOSE: An increasing amount of evidence indicates that single nucleotide polymorphisms (SNPs) may affect a variety of oncology related phenotypes. Occasionally, it is convenient to base studies addressing genotype-phenotype relationships on historical patient cohorts, from which only archival specimens are available. This study was conducted to validate protocols optimised for assessment of SNPs based on paraffin embedded, formalin fixed tissue samples. PATIENTS AND METHODS: In 137 breast cancer patients, three TGFB1 SNPs were assessed based on archival histological specimens. In 37 of these patients, the SNPs were also assessed using cultured fibroblasts and the assays were validated by direct comparison of the results. From the remaining 100 patients, only archival material was available. In these patients, the existence of a genetic linkage pattern between the assessed TGFB1 SNPs was used to provide an indirect validation of the genotyping results. Furthermore, two different methodsfor DNA extraction were compared (semi-automatic DNA extraction using the ABI Prism trade mark 6100 Nucleic Acid PrepStation versus Proteinase K digestion for 5 days followed by boiling and DNA precipitation). RESULTS: Assessment of SNPs based on archival histological material is encumbered by a number of obstacles and pitfalls. However, these can be widely overcome by careful optimisation of the methods used for sample selection, DNA extraction and PCR. Within 130 samples that fulfil the criteria for analysis a highly reliable SNP assessment was observed. The study demonstrated that different 'down-stream applications' ('single nucleotide primer extension' or 'TaqMan((R))-based' real-time PCR) could be used as genotyping procedure. CONCLUSIONS: Reliable assessment of SNPs in formalin-fixed paraffin-embedded specimens is possible but a number of precautions should be carefully taken.
机译:背景与目的:越来越多的证据表明单核苷酸多态性(SNP)可能会影响多种与肿瘤学有关的表型。有时,在基于历史患者队列的基础上处理基因型与表型关系的研究是很方便的,从中只能获得档案标本。进行这项研究以验证基于石蜡包埋,福尔马林固定组织样品优化的评估SNP的方案。患者和方法:在137例乳腺癌患者中,根据档案组织学标本评估了3个TGFB1 SNP。在这些患者中的37名中,还使用培养的成纤维细胞对SNP进行了评估,并通过直接比较结果验证了测定方法。在其余的100名患者中,只有档案材料可用。在这些患者中,所评估的TGFB1 SNP之间存在遗传连锁模式,用于间接验证基因分型结果。此外,比较了两种不同的DNA提取方法(半自动DNA提取,使用ABI Prism商标6100 Nucleic Acid PrepStation与蛋白酶K消化5天,然后煮沸并沉淀DNA)。结果:基于档案组织学资料的单核苷酸多态性评估受到许多障碍和陷阱的困扰。但是,通过仔细优化用于样品选择,DNA提取和PCR的方法,可以广泛克服这些问题。在满足分析标准的130个样本中,观察到了高度可靠的SNP评估。该研究表明,可以将不同的“下游应用”(“单核苷酸引物延伸”或“基于TaqMan(R))的实时PCR)用作基因分型程序。结论:可以可靠地评估福尔马林固定石蜡包埋的标本中的SNPs,但应谨慎采取许多预防措施。

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