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小麦胚芽核糖核酸聚合酶II的体外转录:肝素的影响及模板完整性的作用

In vitro transcription by wheat germ ribonucleic acid polymerase II: effects of heparin and role of template integrity.

作者信息

Dynan W S, Burgess R R

出版信息

Biochemistry. 1979 Oct 16;18(21):4581-8. doi: 10.1021/bi00588a019.

Abstract

Double-stranded deoxyribonucleic acid (DNA) from bacteriophage lambda is a good template for wheat germ DNA-dependent ribonucleic acid (RNA) polymerase II. We delineated conditions for obtaining maximum polymerase activity using as template both the relatively intact DNA extracted from the the lambda phage and DNA into which single-strand nicks have been introduced by deoxyribonuclease (DNase) I digestion. The deliberate introduction of nicks produces a modest increase in transcription. The NaCl and MgCl2 optima are broader with the nicked template, so that higher concentrations of these salts are needed before polymerase activity begins to decline. Heparin inhibits initiation but not elongation by wheat germ polymerase. Polymerase can be protected against heparin inhibition by forming binary complexes with the template. The formation of these complexes is reduced at low temperature. The complexes, once formed, decay in the presence of heparin with a half-life of 10--20 min. The number of complexes is highly dependent on the degree of nicking of the template, suggesting that single-strand nicks are the predominant type of site where these heparin-resistant complexes are formed. Our data do not allow us to decide whether or not the presence of nicks plays as decisive a role in the absence of heparin.

摘要

来自噬菌体λ的双链脱氧核糖核酸(DNA)是小麦胚DNA依赖性核糖核酸(RNA)聚合酶II的良好模板。我们确定了使用从λ噬菌体提取的相对完整的DNA和通过脱氧核糖核酸酶(DNase)I消化引入单链切口的DNA作为模板获得最大聚合酶活性的条件。有意引入切口会使转录适度增加。带切口的模板的NaCl和MgCl2最佳浓度范围更宽,因此在聚合酶活性开始下降之前需要更高浓度的这些盐。肝素抑制小麦胚聚合酶的起始但不抑制延伸。通过与模板形成二元复合物可以保护聚合酶免受肝素抑制。这些复合物的形成在低温下减少。一旦形成,复合物在肝素存在下以10 - 20分钟的半衰期衰变。复合物的数量高度依赖于模板的切口程度,这表明单链切口是形成这些抗肝素复合物的主要位点类型。我们的数据不允许我们确定在没有肝素的情况下切口的存在是否起决定性作用。

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