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首页> 外文期刊>Journal of Virological Methods >Urea-nuclease treatment of concentrated retrovirions preserves viral RNA and removes polymerase chain reaction-amplifiable cellular RNA and DNA
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Urea-nuclease treatment of concentrated retrovirions preserves viral RNA and removes polymerase chain reaction-amplifiable cellular RNA and DNA

机译:浓缩逆转录病毒颗粒的尿素核酸酶处理可保留病毒RNA并去除聚合酶链反应可扩增的细胞RNA和DNA

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摘要

Cellular nucleic acids can interfere with the molecular cloning of retroviruses, a problem that is particularly serious with viruses propagated in lymphoblastoid cells that release large amounts of microvesicles and other cellular components. The approach taken to circumvent such problems involved first suspending viral pellets in water to allow any residual microvesicles to swell and perhaps lyse during overnight or longer incubation periods. Urea was then added to a concentration of 1.5-2.0M to uncoil proteins that may protect nucleic acids from hydrolysis on the further addition of Micrococcal nuclease and ribonuclease A, both of which remain enzymatically active in molar urea solutions. The viral RNA was extracted and residual DNA removed by deoxyribonuclease I treatments. The utility of the method was demonstrated with two different retroviruses, a Moloney murine leukemia virus variant and Rous sarcoma virus, such that viral RNA thus purified was shown to be free of contamination by PCR-amplifiable cellular GAPDH mRNA and ribosomal RNA. This general approach should be applicable to viruses of any type in circumstances where contamination by cellular RNA and DNA poses a problem.
机译:细胞核酸会干扰逆转录病毒的分子克隆,这一问题在释放大量微泡和其他细胞成分的淋巴母细胞中繁殖的病毒尤为严重。避免此类问题的方法包括首先将病毒颗粒悬浮在水中,以使任何残留的微囊肿在过夜或更长时间的孵育过程中溶胀并裂解。然后将尿素添加至1.5-2.0M的浓度以解开蛋白质,该蛋白质可在进一步添加微球菌核酸酶和核糖核酸酶A时保护核酸免于水解,这两种酶在摩尔尿素溶液中均保持酶促活性。提取病毒RNA,并通过脱氧核糖核酸酶I处理除去残留的DNA。用两种不同的逆转录病毒,莫洛尼氏鼠白血病病毒变种和劳斯肉瘤病毒,证明了该方法的实用性,因此,如此纯化的病毒RNA被PCR可扩增的细胞GAPDH mRNA和核糖体RNA所污染。在细胞RNA和DNA污染构成问题的情况下,这种通用方法应适用于任何类型的病毒。

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