4.8 Article

Structural analysis of the Ras-like G protein MglA and its cognate GAP MglB and implications for bacterial polarity

Journal

EMBO JOURNAL
Volume 30, Issue 20, Pages 4185-4197

Publisher

WILEY
DOI: 10.1038/emboj.2011.291

Keywords

bacterial Ras-like G protein; cell polarity; GTPase-activating protein; intrinsic arginine finger; Roadblock/LC7 domain

Funding

  1. The Max-Planck Society
  2. German Research Foundation
  3. SFB [Nr 642]
  4. LOEWE Research Center for Synthetic Microbiology
  5. graduate programme 'Intra- and intercellular transport and communication'

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The bacterium Myxococcus xanthus uses a G protein cycle to dynamically regulate the leading/lagging pole polarity axis. The G protein MglA is regulated by its GTPase-activating protein (GAP) MglB, thus resembling Ras family proteins. Here, we show structurally and biochemically that MglA undergoes a dramatic, GDP-GTP-dependent conformational change involving a screw-type forward movement of the central beta 2-strand, never observed in any other G protein. This movement and complex formation with MglB repositions the conserved residues Arg53 and Gln82 into the active site. Residues required for catalysis are thus not provided by the GAP MglB, but by MglA itself. MglB is a Roadblock/LC7 protein and functions as a dimer to stimulate GTP hydrolysis in a 2:1 complex with MglA. In vivo analyses demonstrate that hydrolysis mutants abrogate Myxococcus' ability to regulate its polarity axis changing the reversal behaviour from stochastic to oscillatory and that both MglA GTPase activity and MglB GAP catalysis are essential for maintaining a proper polarity axis. The EMBO Journal (2011) 30, 4185-4197. doi: 10.1038/emboj.2011.291; Published online 16 August 2011

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