Interaction between the Rev1 C-Terminal Domain and the PolD3 Subunit of Polζ Suggests a Mechanism of Polymerase Exchange upon Rev1/Polζ-Dependent Translesion Synthesis

Interaction between the Rev1 C-Terminal Domain and the PolD3 Subunit of Polζ Suggests a Mechanism of Polymerase Exchange upon Rev1/Polζ-Dependent Translesion Synthesis

Translesion synthesis (TLS) is a mutagenic branch of cellular DNA damage tolerance that enables bypass replication over DNA lesions carried out by specialized low-fidelity DNA polymerases. The replicative bypass of most types of DNA damage is performed in a two-step process of Rev1/Polζ-dependent TL...

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Main Authors: Pustovalova, Yulia (Author), Magalhães, Mariana T. Q. (Author), Rizzo, Alessandro A. (Author), Korza, George (Author), Korzhnev, Dmitry M. (Author), D'Souza, Sanjay Victor (Contributor), Walker, Graham C (Contributor)
Format: Article
Language:English
Published: American Chemical Society (ACS), 2017-05-01T19:56:54Z.
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LEADER 02619 am a22002413u 4500
001 108560
042 |a dc 
100 1 0 |a Pustovalova, Yulia  |e author 
100 1 0 |a D'Souza, Sanjay Victor  |e contributor 
100 1 0 |a Walker, Graham C  |e contributor 
700 1 0 |a Magalhães, Mariana T. Q.  |e author 
700 1 0 |a Rizzo, Alessandro A.  |e author 
700 1 0 |a Korza, George  |e author 
700 1 0 |a Korzhnev, Dmitry M.  |e author 
700 1 0 |a D'Souza, Sanjay Victor  |e author 
700 1 0 |a Walker, Graham C  |e author 
245 0 0 |a Interaction between the Rev1 C-Terminal Domain and the PolD3 Subunit of Polζ Suggests a Mechanism of Polymerase Exchange upon Rev1/Polζ-Dependent Translesion Synthesis 
260 |b American Chemical Society (ACS),   |c 2017-05-01T19:56:54Z. 
856 |z Get fulltext  |u http://hdl.handle.net/1721.1/108560 
520 |a Translesion synthesis (TLS) is a mutagenic branch of cellular DNA damage tolerance that enables bypass replication over DNA lesions carried out by specialized low-fidelity DNA polymerases. The replicative bypass of most types of DNA damage is performed in a two-step process of Rev1/Polζ-dependent TLS. In the first step, a Y-family TLS enzyme, typically Polη, Polι, or Polκ, inserts a nucleotide across a DNA lesion. In the second step, a four-subunit B-family DNA polymerase Polζ (Rev3/Rev7/PolD2/PolD3 complex) extends the distorted DNA primer-template. The coordinated action of error-prone TLS enzymes is regulated through their interactions with the two scaffold proteins, the sliding clamp PCNA and the TLS polymerase Rev1. Rev1 interactions with all other TLS enzymes are mediated by its C-terminal domain (Rev1-CT), which can simultaneously bind the Rev7 subunit of Polζ and Rev1-interacting regions (RIRs) from Polη, Polι, or Polκ. In this work, we identified a previously unknown RIR motif in the C-terminal part of PolD3 subunit of Polζ whose interaction with the Rev1-CT is among the tightest mediated by RIR motifs. Three-dimensional structure of the Rev1-CT/PolD3-RIR complex determined by NMR spectroscopy revealed a structural basis for the relatively high affinity of this interaction. The unexpected discovery of PolD3-RIR motif suggests a mechanism of "inserter" to "extender" DNA polymerase switch upon Rev1/Polζ-dependent TLS, in which the PolD3-RIR binding to the Rev1-CT (i) helps displace the "inserter" Polη, Polι, or Polκ from its complex with Rev1, and (ii) facilitates assembly of the four-subunit "extender" Polζ through simultaneous interaction of Rev1-CT with Rev7 and PolD3 subunits. 
546 |a en_US 
655 7 |a Article 
773 |t Biochemistry 

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