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痘苗病毒粒子转录终止因子的纯化与特性分析

Purification and characterization of a transcription termination factor from vaccinia virions.

作者信息

Shuman S, Broyles S S, Moss B

出版信息

J Biol Chem. 1987 Sep 5;262(25):12372-80.

PMID:3624264
Abstract

A DNA-dependent RNA polymerase that transcribes vaccinia virus early genes was partially purified from virus cores by deoxycholate extraction and DEAE-cellulose column chromatography. Accurately initiated and terminated RNAs were synthesized by this enzyme in the presence of a linear duplex DNA template. Glycerol gradient sedimentation resolved the in vitro transcription system into two components: fraction I, a rapidly sedimenting RNA polymerase that initiated transcription at an early promoter but transcribed beyond the in vivo 3' terminus to yield a run-off transcript, and fraction II, a more slowly sedimenting fraction, itself devoid of RNA polymerase, that restored efficient termination when added back to fraction I. The termination factor was heat-labile, resistant to N-ethylmaleimide, and did not exhibit endonucleolytic activity on run-off transcripts. Factor-dependent termination required specific sequence information upstream of the site of termination. The vaccinia termination factor was purified extensively by column chromatography on DEAE-cellulose, heparin-agarose, phosphocellulose, and DNA-agarose, and by velocity sedimentation in a glycerol gradient. At each step, termination factor copurified with the vaccinia mRNA capping enzyme. The preparation was well over 90% pure with respect to the latter enzyme, suggesting that termination activity was tightly associated with, if not intrinsic to, the capping enzyme. Nonetheless, formation of the 5'-cap structure did not appear to be a prerequisite for termination.

摘要

一种转录痘苗病毒早期基因的依赖DNA的RNA聚合酶通过脱氧胆酸盐提取和DEAE-纤维素柱色谱从病毒核心中部分纯化出来。在双链线性DNA模板存在的情况下,该酶能合成精确起始和终止的RNA。甘油梯度沉降将体外转录系统分离成两个组分:组分I,一种沉降速度快的RNA聚合酶,它在早期启动子处起始转录,但转录超过体内3'末端,产生一个溢流转录本;组分II,一种沉降速度较慢的组分,本身不含RNA聚合酶,当重新加入到组分I中时能恢复有效的终止。终止因子对热不稳定,对N-乙基马来酰胺有抗性,并且对溢流转录本不表现内切核酸酶活性。因子依赖性终止需要终止位点上游的特定序列信息。痘苗终止因子通过在DEAE-纤维素、肝素-琼脂糖、磷酸纤维素和DNA-琼脂糖上的柱色谱以及在甘油梯度中的速度沉降进行了广泛纯化。在每一步中,终止因子都与痘苗mRNA加帽酶共纯化。就后一种酶而言,该制剂的纯度超过90%,这表明终止活性如果不是加帽酶固有的,也是与之紧密相关的。尽管如此,5'-帽结构的形成似乎不是终止的先决条件。

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