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首页> 外文期刊>Journal of Biomolecular Structure and Dynamics >Differential scanning calorimetric approach to study the effect of melting region upon transcription initiation by T7 RNA polymerase and role of high affinity GTP binding
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Differential scanning calorimetric approach to study the effect of melting region upon transcription initiation by T7 RNA polymerase and role of high affinity GTP binding

机译:差示扫描量热法研究熔解区对T7 RNA聚合酶转录启动的影响以及高亲和力GTP结合的作用

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摘要

Transcription initiation by T7 RNA polymerase is a multistep process consisting of the transition from closed to open complex. The promoters of bacteriophage T7 share a consensus sequence of 23 base pairs, from -17 to +6, relative to transcription start site (+1). In the present study, we have characterized T7 RNA polymerase-promoter complexes by means of fluorescence spectroscopy and differential scanning calorimetry. We have examined the effect of high affinity GTP binding upon the equilibrium of the transition from closed to open complex. We have employed the promoter containing 23 base pair consensus sequence and two variants containing Adenine-Thymine and Guanine-Cytosine stretches in the melting region of the promoter sequence. Variation in the nucleotide sequence of melting region does not have any effect upon the affinity of promoter-T7 RNAP complex. On the other hand, alteration of the base sequence in the melting region of the promoter affects the isomerization process among the closed and open complexes. When the initiating nucleotide GTP is prebound to T7 RNA Polymerase, the isomerization process is affected only in case of the promoter with consensus sequence.
机译:T7 RNA聚合酶的转录起始是一个多步过程,包括从封闭复合物到开放复合物的转变。相对于转录起始位点(+1),噬菌体T7的启动子共有23个碱基对的共有序列,从-17到+6。在本研究中,我们已经通过荧光光谱和差示扫描量热法对T7 RNA聚合酶-启动子复合体进行了表征。我们已经检查了高亲和力GTP结合对从封闭到开放复合物过渡的平衡的影响。我们采用了含有23个碱基对的共有序列的启动子,以及在启动子序列的熔解区域中含有腺嘌呤-胸腺嘧啶和鸟嘌呤-胞嘧啶序列的两个变体。熔解区核苷酸序列的变化对启动子-T7 RNAP复合物的亲和力没有任何影响。另一方面,启动子解链区中碱基序列的改变影响了封闭和开放配合物之间的异构化过程。当起始核苷酸GTP预结合至T7 RNA聚合酶时,异构化过程仅在启动子具有共有序列的情况下受到影响。

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