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T3 RNA聚合酶在T3 DNA上所利用的启动子位点的定位

Mapping of promoter sites utilized by T3 RNA polymerase on T3 DNA.

作者信息

Bailey J N, McAllister W T

出版信息

Nucleic Acids Res. 1980 Nov 11;8(21):5071-88. doi: 10.1093/nar/8.21.5071.

Abstract

Promoter locations for the T3 RNA polymerase on the physical map of T3 DNa have been determined. Through the use of conditions favoring the synthesis of RNA from the class II region, an agarose-formaldehyde gel system which improves the resolution of high molecular weight RNAs, and template DNA that was cut by one of several restriction endonucleases prior to transcription, seventeen promoter locations for the T3 RNA polymerase have been mapped. Ten promoters have been identified in the class II region and one promotor has been identified in the class II region and one promotor has been identified in the early (class I) region. The locations of previously mapped class III promoters and the internal termination signal for the T3 RNA polymerase have been mapped more precisely than in previous reports. The resulting transcription map demonstrates a striking similarity to the transcription map of bacteriophage T7.

摘要

已确定T3 DNA物理图谱上T3 RNA聚合酶的启动子位置。通过使用有利于从II类区域合成RNA的条件、一种可提高高分子量RNA分辨率的琼脂糖-甲醛凝胶系统,以及在转录前用几种限制性内切酶之一切割的模板DNA,已绘制出T3 RNA聚合酶的17个启动子位置。在II类区域已鉴定出10个启动子,在早期(I类)区域已鉴定出1个启动子。与之前的报告相比,已更精确地绘制出了先前定位的III类启动子的位置以及T3 RNA聚合酶的内部终止信号。所得的转录图谱与噬菌体T7的转录图谱显示出惊人的相似性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d37d/324280/5d6096718eb3/nar00438-0240-a.jpg

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