Database of articles cited by EMDB/PDB/SASBDB data

Keywords
Structure methods	All X-ray diffraction NMR electron microscopy small angle scattering neutron diffraction fiber diffraction powder diffraction infrared spectroscopy EPR fluorescence transfer theoretical model Hybrid
Author
Journal
IF	>30 >20 >10 >5 all

Title	Structural analysis of substrate binding by the TatBC component of the twin-arginine protein transport system.
Journal, issue, pages	Proc Natl Acad Sci U S A, Vol. 106, Issue 32, Page 13284-13289, Year 2009
Publish date	Aug 11, 2009
Authors	Michael J Tarry / Eva Schäfer / Shuyun Chen / Grant Buchanan / Nicholas P Greene / Susan M Lea / Tracy Palmer / Helen R Saibil / Ben C Berks /
PubMed Abstract	The Tat system transports folded proteins across the bacterial cytoplasmic membrane and the thylakoid membrane of plant chloroplasts. In Escherichia coli substrate proteins initially bind to the ...The Tat system transports folded proteins across the bacterial cytoplasmic membrane and the thylakoid membrane of plant chloroplasts. In Escherichia coli substrate proteins initially bind to the integral membrane TatBC complex which then recruits the protein TatA to effect translocation. Overproduction of TatBC and the substrate protein SufI in the absence of TatA led to the accumulation of TatBC-SufI complexes that could be purified using an affinity tag on the substrate. Three-dimensional structures of the TatBC-SufI complexes and unliganded TatBC were obtained by single-particle electron microscopy and random conical tilt reconstruction. Comparison of the structures shows that substrate molecules bind on the periphery of the TatBC complex and that substrate binding causes a significant reduction in diameter of the TatBC part of the complex. Although the TatBC complex contains multiple copies of the signal peptide-binding TatC protomer, purified TatBC-SufI complexes contain only 1 or 2 SufI molecules. Where 2 substrates are present in the TatBC-SufI complex, they are bound at adjacent sites. These observations imply that only certain TatC protomers within the complex interact with substrate or that there is a negative cooperativity of substrate binding. Similar TatBC-substrate complexes can be generated by an alternative in vitro reconstitution method and using a different substrate protein.
External links	Proc Natl Acad Sci U S A / PubMed:19666509 / PubMed Central
Methods	EM (single particle)
Structure data	EMDB-1632: Structural analysis of substrate binding by the TatBC component of the twin-arginine protein transport system. Method: EM (single particle) EMDB-1633: Structural analysis of substrate binding by the TatBC component of the twin-arginine protein transport system. Method: EM (single particle) EMDB-1634: Structural analysis of substrate binding by the TatBC component of the twin-arginine protein transport system. Method: EM (single particle) EMDB-1635: Structural analysis of substrate binding by the TatBC component of the twin-arginine protein transport system. Method: EM (single particle)
Source	Escherichia coli (E. coli)