Structure and mechanism of the RuvB holliday junction branch migration motor

Christopher D. Putnam; Sheila B. Clancy; Hiro Tsuruta; Susana Gonzalez; James G. Wetmur; John A. Tainer

doi:10.1006/jmbi.2001.4852

Structure and mechanism of the RuvB holliday junction branch migration motor

Christopher D. Putnam, Sheila B. Clancy, Hiro Tsuruta, Susana Gonzalez, James G. Wetmur, John A. Tainer

Icahn School of Medicine at Mount Sinai

Research output: Contribution to journal › Article › peer-review

151 Scopus citations

Abstract

The RuvB hexamer is the chemomechanical motor of the RuvAB complex that migrates Holliday junction branch-points in DNA recombination and the rescue of stalled DNA replication forks. The 1.6 Å crystal structure of Thermotoga maritima RuvB together with five mutant structures reveal that RuvB is an ATPase-associated with diverse cellular activities (AAA +-class ATPase) with a winged-helix DNA-binding domain. The RuvB-ADP complex structure and mutagenesis suggest how AAA +class ATPases couple nucleotide binding and hydrolysis to interdomain conformational changes and asymmetry within the RuvB hexamer implied by the crystallographic packing and small-angle X-ray scattering in solution. ATP-driven domain motion is positioned to move double-stranded DNA through the hexamer and drive conformational changes between subunits by altering the complementary hydrophilic protein-protein interfaces. Structural and biochemical analysis of five motifs in the protein suggest that ATP binding is a strained conformation recognized both by sensors and the Walker motifs and that intersubunit activation occurs by an arginine finger motif reminiscent of the GTPase-activating proteins. Taken together, these results provide insights into how RuvB functions as a motor for branch migration of Holliday junctions.

Original language	English
Pages (from-to)	297-310
Number of pages	14
Journal	Journal of Molecular Biology
Volume	311
Issue number	2
DOIs	https://doi.org/10.1006/jmbi.2001.4852
State	Published - 10 Aug 2001

Keywords

AAA+-class ATPases
Arginine finger
Branch migration
Holliday junction
Recombination

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title = "Structure and mechanism of the RuvB holliday junction branch migration motor",

abstract = "The RuvB hexamer is the chemomechanical motor of the RuvAB complex that migrates Holliday junction branch-points in DNA recombination and the rescue of stalled DNA replication forks. The 1.6 {\AA} crystal structure of Thermotoga maritima RuvB together with five mutant structures reveal that RuvB is an ATPase-associated with diverse cellular activities (AAA +-class ATPase) with a winged-helix DNA-binding domain. The RuvB-ADP complex structure and mutagenesis suggest how AAA +class ATPases couple nucleotide binding and hydrolysis to interdomain conformational changes and asymmetry within the RuvB hexamer implied by the crystallographic packing and small-angle X-ray scattering in solution. ATP-driven domain motion is positioned to move double-stranded DNA through the hexamer and drive conformational changes between subunits by altering the complementary hydrophilic protein-protein interfaces. Structural and biochemical analysis of five motifs in the protein suggest that ATP binding is a strained conformation recognized both by sensors and the Walker motifs and that intersubunit activation occurs by an arginine finger motif reminiscent of the GTPase-activating proteins. Taken together, these results provide insights into how RuvB functions as a motor for branch migration of Holliday junctions.",

keywords = "AAA+-class ATPases, Arginine finger, Branch migration, Holliday junction, Recombination",

author = "Putnam, {Christopher D.} and Clancy, {Sheila B.} and Hiro Tsuruta and Susana Gonzalez and Wetmur, {James G.} and Tainer, {John A.}",

note = "Funding Information: We thank Karl-Peter Hopfner and Clifford Mol for helpful discussions; Clifford Mol, David Barondeau, and Andrew Arvai for assisting data collection; and Jie Tong for purifying samples of RuvB that initiated the crystallographic efforts. We are indebted to Tom Macke for the computational generation DNA coordinates for Figure 5 . We thank the staff at the crystallographic beamlines at SSRL, ALS, and APS for excellent data collection facilities. The pEAW112 plasmid was a kind gift from Michael Cox. This work is based upon research conducted at the Stanford Synchrotron Radiation Laboratory (SSRL), which is funded by the Department of Energy (BES, BER) and the National Institutes of Health (NCRR, NIGMS), the Advanced Light Source (ALS) at Lawrence Berkeley National Laboratory (LBNL), and the Advanced Photon Source (APS) at the Argonne National Laboratory. This work has been funded by the NIH grant CA76431 to J.A.T. and a Howard Hughes Predoctoral Fellowship to C.D.P.",

year = "2001",

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doi = "10.1006/jmbi.2001.4852",

language = "English",

volume = "311",

pages = "297--310",

journal = "Journal of Molecular Biology",

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AU - Putnam, Christopher D.

AU - Clancy, Sheila B.

AU - Tsuruta, Hiro

AU - Gonzalez, Susana

AU - Wetmur, James G.

AU - Tainer, John A.

N1 - Funding Information: We thank Karl-Peter Hopfner and Clifford Mol for helpful discussions; Clifford Mol, David Barondeau, and Andrew Arvai for assisting data collection; and Jie Tong for purifying samples of RuvB that initiated the crystallographic efforts. We are indebted to Tom Macke for the computational generation DNA coordinates for Figure 5 . We thank the staff at the crystallographic beamlines at SSRL, ALS, and APS for excellent data collection facilities. The pEAW112 plasmid was a kind gift from Michael Cox. This work is based upon research conducted at the Stanford Synchrotron Radiation Laboratory (SSRL), which is funded by the Department of Energy (BES, BER) and the National Institutes of Health (NCRR, NIGMS), the Advanced Light Source (ALS) at Lawrence Berkeley National Laboratory (LBNL), and the Advanced Photon Source (APS) at the Argonne National Laboratory. This work has been funded by the NIH grant CA76431 to J.A.T. and a Howard Hughes Predoctoral Fellowship to C.D.P.

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Y1 - 2001/8/10

N2 - The RuvB hexamer is the chemomechanical motor of the RuvAB complex that migrates Holliday junction branch-points in DNA recombination and the rescue of stalled DNA replication forks. The 1.6 Å crystal structure of Thermotoga maritima RuvB together with five mutant structures reveal that RuvB is an ATPase-associated with diverse cellular activities (AAA +-class ATPase) with a winged-helix DNA-binding domain. The RuvB-ADP complex structure and mutagenesis suggest how AAA +class ATPases couple nucleotide binding and hydrolysis to interdomain conformational changes and asymmetry within the RuvB hexamer implied by the crystallographic packing and small-angle X-ray scattering in solution. ATP-driven domain motion is positioned to move double-stranded DNA through the hexamer and drive conformational changes between subunits by altering the complementary hydrophilic protein-protein interfaces. Structural and biochemical analysis of five motifs in the protein suggest that ATP binding is a strained conformation recognized both by sensors and the Walker motifs and that intersubunit activation occurs by an arginine finger motif reminiscent of the GTPase-activating proteins. Taken together, these results provide insights into how RuvB functions as a motor for branch migration of Holliday junctions.

AB - The RuvB hexamer is the chemomechanical motor of the RuvAB complex that migrates Holliday junction branch-points in DNA recombination and the rescue of stalled DNA replication forks. The 1.6 Å crystal structure of Thermotoga maritima RuvB together with five mutant structures reveal that RuvB is an ATPase-associated with diverse cellular activities (AAA +-class ATPase) with a winged-helix DNA-binding domain. The RuvB-ADP complex structure and mutagenesis suggest how AAA +class ATPases couple nucleotide binding and hydrolysis to interdomain conformational changes and asymmetry within the RuvB hexamer implied by the crystallographic packing and small-angle X-ray scattering in solution. ATP-driven domain motion is positioned to move double-stranded DNA through the hexamer and drive conformational changes between subunits by altering the complementary hydrophilic protein-protein interfaces. Structural and biochemical analysis of five motifs in the protein suggest that ATP binding is a strained conformation recognized both by sensors and the Walker motifs and that intersubunit activation occurs by an arginine finger motif reminiscent of the GTPase-activating proteins. Taken together, these results provide insights into how RuvB functions as a motor for branch migration of Holliday junctions.

KW - AAA+-class ATPases

KW - Arginine finger

KW - Branch migration

KW - Holliday junction

KW - Recombination

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JO - Journal of Molecular Biology

JF - Journal of Molecular Biology

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ER -

Structure and mechanism of the RuvB holliday junction branch migration motor

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