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通过配体诱导的构象变化对核酶活性进行变构调节。

Allosteric regulation of a ribozyme activity through ligand-induced conformational change.

作者信息

Araki M, Okuno Y, Hara Y, Sugiura Y

机构信息

Institute for Chemical Research, Kyoto Universitiy, Uji, Kyoto 611-0011, Japan.

出版信息

Nucleic Acids Res. 1998 Jul 15;26(14):3379-84. doi: 10.1093/nar/26.14.3379.

DOI:10.1093/nar/26.14.3379
PMID:9649622
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC147720/
Abstract

An allosteric ribozyme has been designed using the hammerhead ribozyme as the active site and aflavin-specific RNA aptamer as a regulatory site. We constructed six variants with a series of base pairs in the linker region (stem II). Under single turnover conditions, kinetic studies were carried out in the absence and presence of flavin mononucleotide (FMN). Interestingly, FMN addition did not influence the cleavage rate of constructs with a 5-6 bp linker but stimulated the catalytic activity of those bearing a shorter linker. In particular, the apparent k cat of Rz3 increases by approximately 10-fold upon addition of saturating amounts of FMN. To determine the rate constants( K m4and k cat), the ribozyme regulated most effectively by FMN was further investigated. FMN mainly affected the k cat value, reflecting the rate limiting conformational change step of the overall cleavage reaction, depending on helix formation in stem II. Probably, FMN influences the orientation of structures necessary for the cleavage reaction through stem II formation. The result of chemical modification revealed that binding of FMN to the aptamer domain induced the helix formation in stem II required for catalytic activity. Therefore, a specific FMN-mediated allosteric interaction seems to promote a conformational alteration from an open to a closed structure in stem II. The concept of conformational modification in the allosteric effect is consistent with other allosteric enzymes, suggesting that such a conformational change is a fundamental feature of allosteric enzymes in biological systems.

摘要

一种变构核酶已被设计出来,它以锤头状核酶作为活性位点,以黄素特异性RNA适配体作为调节位点。我们构建了六个在连接区(茎II)具有一系列碱基对的变体。在单轮反应条件下,在不存在和存在黄素单核苷酸(FMN)的情况下进行了动力学研究。有趣的是,添加FMN对具有5 - 6个碱基对连接子的构建体的切割速率没有影响,但刺激了那些具有较短连接子的构建体的催化活性。特别是,添加饱和量的FMN后,Rz3的表观催化常数kcat增加了约10倍。为了确定速率常数(Km和kcat),对受FMN调节最有效的核酶进行了进一步研究。FMN主要影响kcat值,这反映了整个切割反应中限速的构象变化步骤,取决于茎II中的螺旋形成。可能,FMN通过茎II的形成影响切割反应所需结构的取向。化学修饰的结果表明,FMN与适配体结构域的结合诱导了催化活性所需的茎II中的螺旋形成。因此,一种特定的FMN介导的变构相互作用似乎促进了茎II中从开放结构到封闭结构的构象改变。变构效应中构象修饰的概念与其他变构酶一致,这表明这种构象变化是生物系统中变构酶的一个基本特征。

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