Structural analysis of a rhomboid family intramembrane protease reveals a gating mechanism for substrate entry

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作者
Zhuoru Wu
Nieng Yan
Liang Feng
Adam Oberstein
Hanchi Yan
Rosanna P Baker
Lichuan Gu
Philip D Jeffrey
Sinisa Urban
Yigong Shi
机构
[1] Lewis Thomas Laboratory,Department of Molecular Biology
[2] Princeton University,Department of Molecular Biology and Genetics
[3] Johns Hopkins University School of Medicine,undefined
[4] State Key Laboratory of Microbial Technology,undefined
[5] Shandong University,undefined
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Intramembrane proteolysis regulates diverse biological processes. Cleavage of substrate peptide bonds within the membrane bilayer is catalyzed by integral membrane proteases. Here we report the crystal structure of the transmembrane core domain of GlpG, a rhomboid-family intramembrane serine protease from Escherichia coli. The protein contains six transmembrane helices, with the catalytic Ser201 located at the N terminus of helix α4 approximately 10 Å below the membrane surface. Access to water molecules is provided by a central cavity that opens to the extracellular region and converges on Ser201. One of the two GlpG molecules in the asymmetric unit has an open conformation at the active site, with the transmembrane helix α5 bent away from the rest of the molecule. Structural analysis suggests that substrate entry to the active site is probably gated by the movement of helix α5.
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页码:1084 / 1091
页数:7
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