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抗终止蛋白GlpP与配体及RNA结合的关键残基及构象变化研究。

Exploration of key residues and conformational change of anti-terminator protein GlpP for ligand and RNA binding.

作者信息

Chen Qiaoqing, Cui Wenjing, Zhou Zhemin, Han Laichuang

机构信息

School of Biotechnology, Jiangnan University, Wuxi, Jiangsu, China.

Jiangnan University (Rugao) Food Biotechnology Research Institute, Rugao, Jiangsu, China.

出版信息

Proteins. 2021 Jun;89(6):623-631. doi: 10.1002/prot.26045. Epub 2021 Jan 25.

DOI:10.1002/prot.26045
PMID:33455022
Abstract

Anti-terminator protein GlpP regulates gene expression of glycerol uptake operon at post-transcriptional level in a number of bacteria. By now, the molecular dynamics details of ligand and RNA binding by GlpP are still obscure. In this study, we employed the molecular dynamic (MD) simulation and constructed a functional verification platform of GlpP to resolve these puzzles. By combining molecular docking, MD simulation and alanine scanning mutagenesis, a ligand binding pocket consisting of R14, R104 and R157 was identified. Among these residues with positive charge, R14 was dominant for binding glycerol-3-phosphate (G3P). Moreover, the "parallel to crossed" conformational change of the predicted RNA binding region was observed in MD simulation. In this process, the interaction between R104 and E129 was crucial to trigger the conformational change. To further verify this speculation, three ligand independent mutants were obtained by error-prone PCR. The MD simulation indicated that the conformational change happened in all the three mutants, confirming the "parallel to crossed" conformational change endowed GlpP the activity of binding RNA. In recent years, as a potable biological part, anti-terminator was more and more widely used to regulate gene expression in metabolic engineering and synthetic biology. The work in this study deepened our understanding to the typical anti-terminator GlpP, contributing to the further engineering and application of this type of regulator.

摘要

抗终止蛋白GlpP在许多细菌的转录后水平上调节甘油摄取操纵子的基因表达。到目前为止,GlpP与配体和RNA结合的分子动力学细节仍不清楚。在本研究中,我们采用分子动力学(MD)模拟并构建了GlpP的功能验证平台来解决这些难题。通过结合分子对接、MD模拟和丙氨酸扫描诱变,鉴定出一个由R14、R104和R157组成的配体结合口袋。在这些带正电荷的残基中,R14对结合3-磷酸甘油(G3P)起主导作用。此外,在MD模拟中观察到预测的RNA结合区域发生了“平行到交叉”的构象变化。在此过程中,R104与E129之间的相互作用对于触发构象变化至关重要。为了进一步验证这一推测,通过易错PCR获得了三个不依赖配体的突变体。MD模拟表明所有这三个突变体都发生了构象变化,证实了“平行到交叉”的构象变化赋予了GlpP结合RNA的活性。近年来,作为一种实用的生物元件,抗终止子在代谢工程和合成生物学中越来越广泛地用于调节基因表达。本研究工作加深了我们对典型抗终止子GlpP的理解,有助于这类调节因子的进一步工程化和应用。

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