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通过链分离琼脂糖凝胶检测噬菌体φ6负链RNA以及在体内和体外合成的新型mRNA异构体。

Detection of bacteriophage phi 6 minus-strand RNA and novel mRNA isoconformers synthesized in vivo and in vitro, by strand-separating agarose gels.

作者信息

Pagratis N, Revel H R

机构信息

Committee on Developmental Biology, University of Chicago, Illinois 60637.

出版信息

Virology. 1990 Jul;177(1):273-80. doi: 10.1016/0042-6822(90)90480-f.

Abstract

Two urea-free agarose gel protocols that resolve the six individual strands of bacteriophage phi 6 dsRNA were developed and used to analyze phage RNA synthesis in vivo and in vitro. Citrate gels separate strands of the large and medium chromosomes while Tris-borate-EDTA (TBE) gels resolve the medium and small dsRNA segments. Minus strands migrate faster than plus strands on citrate gels but are retarded on TBE gels. A study of electrophoretic conditions showed that pH affects strand resolution on citrate gels, and that voltage gradient, agarose concentration, and ethidium bromide significantly alter strand migration on TBE gels. Analysis of native phi 6 RNA synthesized in vivo and in vitro showed that the large and medium message RNAs comigrate with the corresponding plus strands of denatured virion dsRNA. The small messenger RNA is exceptional. Native small mRNA was detected as three isoconformers in vivo and in vitro. The isoconformers were converted by heat denaturation to a single RNA species that comigrates with the virion s+ strand. Minus strands labeled in vivo were detected only after heat denaturation. Minus strand synthesis was detected also in heat-denatured samples from in vitro phi 6 nucleocapsid RNA polymerase reactions at pH values suboptimal for transcription.

摘要

开发了两种无尿素琼脂糖凝胶方法,可分离噬菌体φ6双链RNA的六条单链,并用于分析体内和体外的噬菌体RNA合成。柠檬酸盐凝胶可分离大染色体和中染色体的链,而Tris-硼酸-EDTA(TBE)凝胶可分辨中双链RNA和小双链RNA片段。在柠檬酸盐凝胶上,负链比正链迁移得快,但在TBE凝胶上迁移受阻。电泳条件研究表明,pH值影响柠檬酸盐凝胶上的链分辨率,而电压梯度、琼脂糖浓度和溴化乙锭会显著改变TBE凝胶上的链迁移。对体内和体外合成的天然φ6 RNA的分析表明,大的和中等大小的信使RNA与变性病毒粒子双链RNA的相应正链共迁移。小信使RNA则不同。在体内和体外,天然小mRNA被检测为三种同构体。这些同构体通过热变性转化为与病毒粒子s+链共迁移的单一RNA种类。体内标记的负链仅在热变性后被检测到。在体外φ6核衣壳RNA聚合酶反应的热变性样品中,在转录的最适pH值以下也检测到了负链合成。

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