Literature DB >> 27139643

Walker-A Motif Acts to Coordinate ATP Hydrolysis with Motor Output in Viral DNA Packaging.

Damian delToro1, David Ortiz2, Mariam Ordyan1, Jean Sippy3, Choon-Seok Oh3, Nicholas Keller1, Michael Feiss4, Carlos E Catalano5, Douglas E Smith6.   

Abstract

During the assembly of many viruses, a powerful ATP-driven motor translocates DNA into a preformed procapsid. A Walker-A "P-loop" motif is proposed to coordinate ATP binding and hydrolysis with DNA translocation. We use genetic, biochemical, and biophysical techniques to survey the roles of P-loop residues in bacteriophage lambda motor function. We identify 55 point mutations that reduce virus yield to below detectable levels in a highly sensitive genetic complementation assay and 33 that cause varying reductions in yield. Most changes in the predicted conserved residues K76, R79, G81, and S83 produce no detectable yield. Biochemical analyses show that R79A and S83A mutant proteins fold, assemble, and display genome maturation activity similar to wild-type (WT) but exhibit little ATPase or DNA packaging activity. Kinetic DNA cleavage and ATPase measurements implicate R79 in motor ring assembly on DNA, supporting recent structural models that locate the P-loop at the interface between motor subunits. Single-molecule measurements detect no translocation for K76A and K76R, while G81A and S83A exhibit strong impairments, consistent with their predicted roles in ATP binding. We identify eight residue changes spanning A78-K84 that yield impaired translocation phenotypes and show that Walker-A residues play important roles in determining motor velocity, pausing, and processivity. The efficiency of initiation of packaging correlates strongly with motor velocity. Frequent pausing and slipping caused by changes A78V and R79K suggest that these residues are important for ATP alignment and coupling of ATP binding to DNA gripping. Our findings support recent structural models implicating the P-loop arginine in ATP hydrolysis and mechanochemical coupling.
Copyright © 2016 Elsevier Ltd. All rights reserved.

Entities:  

Keywords:  ATPase; Optical tweezers; mutagenesis of Walker-A motif; terminase; viral DNA packaging motor

Mesh:

Substances:

Year:  2016        PMID: 27139643      PMCID: PMC4905814          DOI: 10.1016/j.jmb.2016.04.029

Source DB:  PubMed          Journal:  J Mol Biol        ISSN: 0022-2836            Impact factor:   5.469


  66 in total

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Authors:  Douglas E Smith
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Authors:  Jean-François Allemand; Berenike Maier; Douglas E Smith
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7.  Biochemical characterization of bacteriophage lambda genome packaging in vitro.

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8.  Repulsive DNA-DNA interactions accelerate viral DNA packaging in phage Phi29.

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  11 in total

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3.  Functional Dissection of a Viral DNA Packaging Machine's Walker B Motif.

Authors:  Damian delToro; David Ortiz; Mariam Ordyan; Joshua Pajak; Jean Sippy; Alexis Catala; Choon-Seok Oh; Amber Vu; Gaurav Arya; Douglas E Smith; Carlos E Catalano; Michael Feiss
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4.  Mechanochemical coupling and bi-phasic force-velocity dependence in the ultra-fast ring ATPase SpoIIIE.

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7.  Evidence that a catalytic glutamate and an 'Arginine Toggle' act in concert to mediate ATP hydrolysis and mechanochemical coupling in a viral DNA packaging motor.

Authors:  David Ortiz; Damian delToro; Mariam Ordyan; Joshua Pajak; Jean Sippy; Alexis Catala; Choon-Seok Oh; Amber Vu; Gaurav Arya; Michael Feiss; Douglas E Smith; Carlos E Catalano
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8.  Structure of the large terminase from a hyperthermophilic virus reveals a unique mechanism for oligomerization and ATP hydrolysis.

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Review 9.  The Impact of the Stringent Response on TRAFAC GTPases and Prokaryotic Ribosome Assembly.

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10.  Function of a viral genome packaging motor from bacteriophage T4 is insensitive to DNA sequence.

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Journal:  Nucleic Acids Res       Date:  2020-11-18       Impact factor: 19.160

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