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快速非酶提取方法从皮肤中分离出可用于 PCR 的羊痘病毒 DNA。

Rapid non-enzymatic extraction method for isolating PCR-quality camelpox virus DNA from skin.

机构信息

Central Biotechnology Laboratory, College of Veterinary Medicine and Animal Resources, Bldg. 999, King Faisal University, Al-Hufof, 31982, Al-Ahsaa, Saudi Arabia.

出版信息

J Virol Methods. 2010 Oct;169(1):138-42. doi: 10.1016/j.jviromet.2010.07.013. Epub 2010 Jul 21.

Abstract

Molecular diagnostic investigations of orthopoxvirus (OPV) infections are performed using a variety of clinical samples including skin lesions, tissues from internal organs, blood and secretions. Skin samples are particularly convenient for rapid diagnosis and molecular epidemiological investigations of camelpox virus (CMLV). Classical extraction procedures and commercial spin-column-based kits are time consuming, relatively expensive, and require multiple extraction and purification steps in addition to proteinase K digestion. A rapid non-enzymatic procedure for extracting CMLV DNA from dried scabs or pox lesions was developed to overcome some of the limitations of the available DNA extraction techniques. The procedure requires as little as 10mg of tissue and produces highly purified DNA [OD(260)/OD(280) ratios between 1.47 and 1.79] with concentrations ranging from 6.5 to 16 microg/ml. The extracted CMLV DNA was proven suitable for virus-specific qualitative and, semi-quantitative PCR applications. Compared to spin-column and conventional viral DNA extraction techniques, the two-step extraction procedure saves money and time, and retains the potential for automation without compromising CMLV PCR sensitivity.

摘要

采用各种临床样本(包括皮肤损伤、内脏组织、血液和分泌物)进行正痘病毒(OPV)感染的分子诊断研究。皮肤样本特别适合用于快速诊断和骆驼痘病毒(CMLV)的分子流行病学研究。经典的提取程序和基于商用离心柱的试剂盒耗时较长,相对昂贵,并且除了蛋白酶 K 消化外,还需要多个提取和纯化步骤。为了克服现有 DNA 提取技术的一些限制,开发了一种从干燥的痂皮或痘疱病变中快速非酶提取 CMLV DNA 的方法。该方法仅需要 10mg 组织,即可产生高度纯化的 DNA [OD(260)/OD(280)比值在 1.47 至 1.79 之间],浓度范围为 6.5 至 16 微克/毫升。提取的 CMLV DNA 适用于病毒特异性定性和半定量 PCR 应用。与离心柱和传统病毒 DNA 提取技术相比,两步提取程序节省了时间和金钱,并且保留了自动化的潜力,而不会影响 CMLV PCR 灵敏度。

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