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在诱导的Friend细胞核中准确地进行β-珠蛋白基因转录的体外起始。

Accurate in vitro initiation of beta-globin gene transcription in induced Friend-cell nuclei.

作者信息

Winicov I, Weidner D A, Carlson D P, Ross J

出版信息

Gene. 1986;45(1):1-10. doi: 10.1016/0378-1119(86)90125-3.

Abstract

The initiation of transcription by RNA polymerase II in isolated murine erythroleukemia cell nuclei was investigated by isolating newly synthesized gamma-thio (gamma-S-)-triphosphate-labeled transcripts by Hg-agarose chromatography. The 5' terminus of transcripts initiated in vitro with [gamma-35S]ATP or [gamma-35S]GTP was identified as the thiotetraphosphate in alkaline hydrolysis products from Hg-agarose-selected RNA. Additional control experiments analyzing the nuclear transcription of two well characterized tRNA genes showed that each gene was initiated with the proper triphosphate, either gamma-S-ATP or gamma-S-GTP, indicating little, if any, exchange of the gamma-S-labeled substrate to the other triphosphates. As determined by S1 mapping, newly synthesized beta-globin gene transcripts initiate only with gamma-S-ATP. Their 5'-terminus is located at the cap site, and their synthesis is inhibited by 1 microgram alpha-amanitin/ml. In reactions containing gamma-S-ATP but not gamma-S-GTP, several additional initiation sites are observed that are located in the 5'-flanking region. We conclude that RNA polymerase II can initiate transcription at the cap site in isolated nuclei.

摘要

通过汞琼脂糖层析分离新合成的γ-硫代(γ-S-)三磷酸标记的转录本,研究了RNA聚合酶II在分离的小鼠红白血病细胞核中启动转录的情况。用[γ-35S]ATP或[γ-35S]GTP在体外启动转录的转录本的5'末端,在汞琼脂糖选择的RNA的碱性水解产物中被鉴定为硫代四磷酸。分析两个特征明确的tRNA基因的核转录的其他对照实验表明,每个基因都以适当的三磷酸启动,即γ-S-ATP或γ-S-GTP,这表明γ-S标记的底物与其他三磷酸之间几乎没有(如果有的话)交换。通过S1图谱分析确定,新合成的β-珠蛋白基因转录本仅以γ-S-ATP启动。它们的5'末端位于帽位点,其合成受到1微克/毫升α-鹅膏蕈碱的抑制。在含有γ-S-ATP但不含γ-S-GTP的反应中,观察到几个位于5'侧翼区域中的额外起始位点。我们得出结论,RNA聚合酶II可以在分离的细胞核中的帽位点启动转录。

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