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首页> 外文期刊>Molecular and Cellular Probes: The Location, Diagnosis and Monitoring of Disease by Specific Molecules and Cell Lines >Genomic DNA extraction from whole blood stored from 15- to 30-years at -20 degrees C by rapid phenol-chloroform protocol: a useful tool for genetic epidemiology studies.
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Genomic DNA extraction from whole blood stored from 15- to 30-years at -20 degrees C by rapid phenol-chloroform protocol: a useful tool for genetic epidemiology studies.

机译:通过快速苯酚-氯仿方案从20摄氏度下储存15至30年的全血中提取基因组DNA:用于遗传流行病学研究的有用工具。

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Long-term stored (LTS) whole blood collection can be an important source of DNA without collection costs, but there is a lack of information on methods useful to extract genomic DNA from such type of biological material. Here we report a simple and fast revisited phenol/chloroform extraction method from LTS whole blood. Protocol reliability was assessed by comparison with proteinase K and silica-gel membrane spin column-based DNA extraction methods using LTS -20 degrees C whole blood from 1980, and by testing it on 82 whole blood samples, collected from 1980 to 1995, with high quality (A(260/280) = 1.79 +/- 0.32 O.D., A(260/230) = 1.45 +/- 0.52 O.D.) and quantity results. Genotyping efficiency was also checked by performing RFLP-PCR and ASP-PCR of p53 Pro72Arg (rs1042522) SNP and hTERT MNS16A VNTR, respectively, resulting in 100% of samples successfully typed. In addition to the goodness and the efficiency of method proposed here, this protocol achieves working time reduction combining extraction and purification steps, allowing to work at room temperature. Furthermore, phenol is able to inactivate any potential nuclease and potential infective sources from the first step on. Based on these results we also conclude that LTS -20 degrees C whole blood samples may be considered a reliable and potential resource for future genotyping studies and retrospective analysis in a genetic epidemiological setting.
机译:长期存储(LTS)的全血收集可以成为重要的DNA来源,而无需收取任何费用,但是缺乏有关从此类生物材料中提取基因组DNA的方法的信息。在这里,我们报告从LTS全血中提取的一种简单快速的苯酚/氯仿提取方法。通过与蛋白酶K和硅胶膜旋转柱DNA提取方法(使用1980年以来的LTS -20°C全血)进行比较,并通过对1980年至1995年收集的82份全血样品进行测试,对方案可靠性进行了评估质量(A(260/280)= 1.79 +/- 0.32 OD,A(260/230)= 1.45 +/- 0.52 OD)和数量结果。还分别通过对p53 Pro72Arg(rs1042522)SNP和hTERT MNS16A VNTR进行RFLP-PCR和ASP-PCR检查了基因分型效率,成功地进行了100%的样品分型。除了此处提出的方法的优点和效率外,该协议还减少了提取和纯化步骤,从而缩短了工作时间,从而可以在室温下工作。此外,从第一步开始,苯酚就能使任何潜在的核酸酶和潜在的感染源失活。根据这些结果,我们还得出结论,LTS -20°C全血样本可能被认为是未来在遗传流行病学中进行基因分型研究和回顾性分析的可靠和潜在资源。

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