Article
- The EMBO Journal (2006) 25, 1492 - 1504
- doi:10.1038/sj.emboj.7601050
Published online: 16 March 2006
Subject Category:
Snf2/Swi2-related ATPase Mot1 drives displacement of TATA-binding protein by gripping DNA
Rebekka O Sprouse1, Michael Brenowitz2 and David T Auble1
- Department of Biochemistry and Molecular Genetics, University of Virginia Health System, Charlottesville, VA, USA
- Department of Biochemistry, The Albert Einstein College of Medicine, Bronx, NY, USA
Correspondence to:
David T Auble, Department of Biochemistry and Molecular Genetics, University of Virginia Health System, 1300 Jefferson Park Avenue, Room 6213, Charlottesville, VA 22908-0733, USA. Tel.: +1 434 243 2629; Fax: +1 434 924 5069; E-mail: dta4n@virginia.edu
Received 6 October 2005; Accepted 20 February 2006
Abstract
Mot1 is a conserved Snf2/Swi2-related transcriptional regulator that uses ATP hydrolysis to displace TATA-binding protein (TBP) from DNA. Several models of the enzymatic mechanism have been proposed, including Mot1-catalyzed distortion of TBP structure, competition between Mot1 and DNA for the TBP DNA-binding surface, and ATP-driven translocation of Mot1 along DNA. Here, DNase I footprinting studies provide strong support for a 'DNA-based' mechanism of Mot1, which we propose involves ATP-driven DNA translocation. Mot1 forms an asymmetric complex with the TBP core domain (TBPc)–DNA complex, contacting DNA both upstream and within the major groove of the TATA Box. Contact with upstream DNA is required for Mot1-mediated displacement of TBPc from DNA. Using the SsoRad54–DNA complex as a model, DNA-binding residues in Mot1 were identified that are critical for Mot1–TBPc–DNA complex formation and catalytic activity, thus placing Mot1 mechanistically within the helicase superfamily. We also report a novel ATP-independent TBPc displacement activity for Mot1 and describe conformational heterogeneity in the Mot1 ATPase, which is likely a general feature of other enzymes in this class.
Keywords:
- ATPase,
- Mot1,
- Snf2,
- Swi2,
- TBP
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