Purification and Enzymic Properties of Mot1 ATPase, a Regulator of Basal Transcription in the Yeast Saccharomyces Cerevisiae

Overview

Journal J Biol Chem

Specialty Biochemistry

Date 2000 Jul 11

PMID 10887203

Citations 20

Authors

J I Adamkewicz

C G Mueller

K E Hansen

W A Prudhomme

J Thorner

Affiliations

Soon will be listed here.

Abstract

The 1867-residue Mot1 protein is a member of a superfamily of ATPases, some of which are helicases, that interact with protein-nucleic acid assemblies. Mot1 is an essential regulator of RNA polymerase II-dependent transcription in vivo and dissociates TATA box-binding protein (TBP)-DNA complexes in vitro. Mot1-(His)(6) was purified to apparent homogeneity from yeast extracts. The preparation efficiently dissociated TBP.TATA complexes, suggesting that no other protein or cofactor is required. Mot1 behaved as a non-globular monomer in hydrodynamic studies, and no association was detected between differentially tagged co-expressed Mot1 constructs. ATPase activity was stimulated about 10-fold by high ionic strength or alkaline pH, or by deletion of the N-terminal TBP-binding segment, suggesting that the N-terminal domain negatively regulates the C-terminal ATPase domain (Mot1C). Correspondingly, at moderate salt concentration, Mot1 ATPase (but not Mot1C) was stimulated >/=10-fold by yeast TBP, suggesting that interaction with TBP relieves a conformational constraint in Mot1. Double- or single-stranded TATA-containing DNA did not affect ATPase activity of Mot1 or Mot1C, with or without TBP. Mot1 did not exhibit detectable helicase activity in strand displacement assays using substrates with flush ends or 5'- or 3'-overhangs. Mot1-catalyzed dissociation of TBP from DNA was not prevented by a psoralen cross-link positioned immediately preceding the TATA sequence. Thus, Mot1 most likely promotes release of TBP from TATA-containing DNA by causing a structural change in TBP itself, rather than by strand unwinding.

Citing Articles

Conformational changes and catalytic inefficiency associated with Mot1-mediated TBP-DNA dissociation.

Heiss G, Ploetz E, Voith von Voithenberg L, Viswanathan R, Glaser S, Schluesche P Nucleic Acids Res. 2019; 47(6):2793-2806.

PMID: 30649478 PMC: 6451094. DOI: 10.1093/nar/gky1322.

Crystal structure of the full Swi2/Snf2 remodeler Mot1 in the resting state.

Butryn A, Woike S, Shetty S, Auble D, Hopfner K Elife. 2018; 7.

PMID: 30289385 PMC: 6188472. DOI: 10.7554/eLife.37774.

Mechanisms of ATP-Dependent Chromatin Remodeling Motors.

Zhou C, Johnson S, Gamarra N, Narlikar G Annu Rev Biophys. 2016; 45:153-81.

PMID: 27391925 PMC: 9157391. DOI: 10.1146/annurev-biophys-051013-022819.

Molecular Mechanism of Mot1, a TATA-binding Protein (TBP)-DNA Dissociating Enzyme.

Viswanathan R, True J, Auble D J Biol Chem. 2016; 291(30):15714-26.

PMID: 27255709 PMC: 4957054. DOI: 10.1074/jbc.M116.730366.

The Modifier of Transcription 1 (Mot1) ATPase and Spt16 Histone Chaperone Co-regulate Transcription through Preinitiation Complex Assembly and Nucleosome Organization.

True J, Muldoon J, Carver M, Poorey K, Shetty S, Bekiranov S J Biol Chem. 2016; 291(29):15307-19.

PMID: 27226635 PMC: 4946942. DOI: 10.1074/jbc.M116.735134.