| Literature DB >> 26527138 |
Munenori Furuse1, Jun Tamogami2, Toshiaki Hosaka1, Takashi Kikukawa3, Naoko Shinya1, Masakatsu Hato1, Noboru Ohsawa1, So Young Kim4, Kwang Hwan Jung4, Makoto Demura3, Seiji Miyauchi2, Naoki Kamo2, Kazumi Shimono1, Tomomi Kimura-Someya1, Shigeyuki Yokoyama1, Mikako Shirouzu1.
Abstract
Although many crystal structures of microbial rhodopsins have been solved, those with sufficient resolution to identify the functional water molecules are very limited. In this study, the Acetabularia rhodopsin I (ARI) protein derived from the marine alga A. acetabulum was synthesized on a large scale by the Escherichia coli cell-free membrane-protein production method, and crystal structures of ARI were determined at the second highest (1.52-1.80 Å) resolution for a microbial rhodopsin, following bacteriorhodopsin (BR). Examinations of the photochemical properties of ARI revealed that the photocycle of ARI is slower than that of BR and that its proton-transfer reactions are different from those of BR. In the present structures, a large cavity containing numerous water molecules exists on the extracellular side of ARI, explaining the relatively low pKa of Glu206(ARI), which cannot function as an initial proton-releasing residue at any pH. An interhelical hydrogen bond exists between Leu97(ARI) and Tyr221(ARI) on the cytoplasmic side, which facilitates the slow photocycle and regulates the pKa of Asp100(ARI), a potential proton donor to the Schiff base, in the dark state.Entities:
Keywords: X-ray crystal structure; cell-free protein synthesis; light-driven ion pump; membrane protein; microbial rhodopsin
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Year: 2015 PMID: 26527138 DOI: 10.1107/S1399004715015722
Source DB: PubMed Journal: Acta Crystallogr D Biol Crystallogr ISSN: 0907-4449