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RNA测序的直接化学方法。

Direct chemical method for sequencing RNA.

作者信息

Peattie D A

出版信息

Proc Natl Acad Sci U S A. 1979 Apr;76(4):1760-4. doi: 10.1073/pnas.76.4.1760.

Abstract

Four different base-specific chemical reactions generate a means of directly sequencing RNA terminally labeled with 32P. After a partial, specific modification of each kind of RNA base, an amine-catalyzed strand scission generates labeled fragments whose lengths determine the position of each nucleotide in the sequence. Dimethyl sulfate modifies guanosine. Diethyl pyrocarbonate attacks primarily adenosine. Hydrazine attacks uridine and cytidine, but salt suppresses the reaction with uridine. In all cases, aniline induces a subsequent strand scission. The electrophoretic fractionation of the labeled fragments on a polyacrylamide gel, followed by autoradiography, determines the RNA sequence. RNA labeled at the 3' end yields clean cleavage patterns for each purine and pyrimidine and allows a determination of the entire RNA sequence out to 100-200 bases from the labeled terminus.

摘要

四种不同的碱基特异性化学反应产生了一种直接对用³²P末端标记的RNA进行测序的方法。在对每种RNA碱基进行部分特异性修饰后,胺催化的链断裂产生标记片段,其长度决定了序列中每个核苷酸的位置。硫酸二甲酯修饰鸟苷。焦碳酸二乙酯主要攻击腺苷。肼攻击尿苷和胞苷,但盐会抑制与尿苷的反应。在所有情况下,苯胺会引发随后的链断裂。标记片段在聚丙烯酰胺凝胶上进行电泳分离,然后进行放射自显影,从而确定RNA序列。在3'端标记的RNA为每个嘌呤和嘧啶产生清晰的切割模式,并允许从标记末端确定长达100 - 200个碱基的整个RNA序列。

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