Literature DB >> 29694856

T7 RNA Polymerase Discriminates Correct and Incorrect Nucleoside Triphosphates by Free Energy.

Shaogui Wu1, Jiayang Wang2, Xuemei Pu3, Laicai Li4, Quan Li5.   

Abstract

RNA polymerase (RNAP) is the primary machine responsible for transcription. Its ability to distinguish between correct (cognate) and incorrect (noncognate) nucleoside triphosphates (NTPs) is important for fidelity control in transcription. In this work, we investigated the substrate selection mechanism of T7 RNAP from the perspective of energetics. The dissociation free energies were determined for matched and unmatched base pairs in the preinsertion complex using the umbrella sampling method. A clear hydrogen-bond-rupture peak is observed in the potential of mean force curve for a matched base pair, whereas no such peaks are present in the position of mean force profiles for unmatched ones. The free-energy barrier could prevent correct substrates from being separated from the active site. Therefore, when NTPs diffuse into the active site, correct ones will stay for chemistry once they establish effective base pairing contacts with the template nucleotide, whereas incorrect ones will be withdrawn from the active site and rejected back to solution. This result provides an important energy evidence for the substrate selection mechanism of RNAP. Then we elucidated energetics and molecular details for correct NTP binding to the active site of the insertion complex. Our observations reveal that strong interactions act on the triphosphate of NTP to constrain its movement, whereas relatively weak interactions serve to position the base in the correct conformation. Triple interactions, hydrophobic contacts from residues M635 and Y639, base stacking from the 3' RNA terminal nucleotide, and base pairing from the template nucleotide act together to position the NTP base in a catalytically competent conformation. At last, we observed that incorrect NTPs cannot be as well-stabilized as the correct one in the active site when they are misincorporated in the insertion site. It is expected that our work can be helpful for comprehensively understanding details of this basic step in genetic transcription.
Copyright © 2018 Biophysical Society. Published by Elsevier Inc. All rights reserved.

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Year:  2018        PMID: 29694856      PMCID: PMC5937113          DOI: 10.1016/j.bpj.2018.02.033

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  25 in total

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4.  Nucleotide Selectivity at a Preinsertion Checkpoint of T7 RNA Polymerase Transcription Elongation.

Authors:  Chao E; Baogen Duan; Jin Yu
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5.  GROMACS 4.5: a high-throughput and highly parallel open source molecular simulation toolkit.

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6.  Exploring transition pathway and free-energy profile of large-scale protein conformational change by combining normal mode analysis and umbrella sampling molecular dynamics.

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7.  Development of polyphosphate parameters for use with the AMBER force field.

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  6 in total

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Review 3.  A Viral T7 RNA Polymerase Ratcheting Along DNA With Fidelity Control.

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Journal:  Comput Struct Biotechnol J       Date:  2019-05-09       Impact factor: 7.271

Review 4.  Mechanism of RNA recognition by a Musashi RNA-binding protein.

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Journal:  Curr Res Struct Biol       Date:  2021-12-14

5.  Dielectricity of a molecularly crowded solution accelerates NTP misincorporation during RNA-dependent RNA polymerization by T7 RNA polymerase.

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Journal:  Sci Rep       Date:  2022-01-21       Impact factor: 4.379

Review 6.  Strategies for Covalent Labeling of Long RNAs.

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  6 in total

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