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核糖核酸酶保护分析

RNase Protection Assay.

作者信息

Ma YJ, Dissen GA, Rage F, Ojeda SR

机构信息

Division of Neuroscience, Oregon Regional Primate Research Center, 505 N.W. 185th Avenue, Beaverton, Oregon, 97006

出版信息

Methods. 1996 Dec;10(3):273-8. doi: 10.1006/meth.1996.0102.

Abstract

The RNase protection assay is a highly sensitive technique developed to detect and measure the abundance of specific mRNAs in samples of total cellular RNA. The assay utilizes in vitro transcribed 32P-labeled antisense RNA probes that are hybridized in solution to their complementary cellular mRNAs. This is followed by digestion of nonhybridizing (single-stranded) RNA species with RNases, removal of the RNases by treatment with proteinase K, phenol extraction of the cRNA:mRNA complexes, and electrophoretic isolation of the hybridizing cRNA fragments. Since one can synthesize "sense" mRNAs having the same sequence as the target cellular mRNA, appropriate standard curves can be generated and used to quantitate the changes in tissue mRNA levels. Because the assay requires perfect sequence complementarity for full protection, it not only serves as a quantitative tool but also provides conclusive evidence for the existence of a specific mRNA in a given tissue. The procedure described here is a modification of that originally described by M. Gilman [1993, in Current Protocols in Molecular Biology (Ausubel, F. M., Brent, R., Kingston, R. E., Moore, D. D., Seidman, J. G., Smith, J. A., and Struhl, K., Eds.), Vol. 1, pp. 4.7.1-4.7.6, Greene and Wiley-Interscience, New York].

摘要

核糖核酸酶保护分析是一种高度灵敏的技术,用于检测和测量总细胞RNA样品中特定mRNA的丰度。该分析利用体外转录的32P标记反义RNA探针,这些探针在溶液中与它们互补的细胞mRNA杂交。随后用核糖核酸酶消化非杂交(单链)RNA种类,用蛋白酶K处理去除核糖核酸酶,对cRNA:mRNA复合物进行酚抽提,并通过电泳分离杂交的cRNA片段。由于可以合成与靶细胞mRNA具有相同序列的“正义”mRNA,因此可以生成适当的标准曲线并用于定量组织mRNA水平的变化。因为该分析需要完美的序列互补性才能实现完全保护,所以它不仅是一种定量工具,还为给定组织中特定mRNA的存在提供确凿证据。这里描述的方法是对M. Gilman最初描述的方法的改进[1993年,《分子生物学实验指南》(奥苏贝尔,F.M.,布伦特,R.,金斯顿,R.E.,摩尔,D.D.,西德曼,J.G.,史密斯,J.A.和斯特鲁尔,K.编),第1卷,第4.7.1 - 4.7.6页,格林出版社和威利 - 国际科学出版社,纽约]。

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