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Proton Release Reactions in the Inward H+ Pump NsXeR

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JOURNAL OF PHYSICAL CHEMISTRY B
卷 127, 期 39, 页码 8358-8369

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AMER CHEMICAL SOC
DOI: 10.1021/acs.jpcb.3c04100

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Directional ion transport across biological membranes is vital for cellular processes, and understanding the molecular mechanism of vectorial ion transport is crucial. In this study, the protonation steps in the light-driven inward proton pump were tracked, revealing key proton release sites and shedding light on the molecular determinants of proton translocation.
Directional ion transport across biological membranes plays a central role in many cellular processes. Elucidating the molecular determinants for vectorial ion transport is key to understanding the functional mechanism of membrane-bound ion pumps. The extensive investigation of the light-driven proton pump bacteriorhodopsin from Halobacterium salinarum(HsBR) enabled a detailed description of outward proton transport. Although the structure of inward-directed proton pumping rhodopsins is very similar to HsBR, little is known about their protonation pathway, and hence, the molecular reasons for the vectoriality of proton translocation remain unclear. Here, we employ a combined experimental and theoretical approach to tracking protonation steps in the light-driven inward proton pump xenorhodopsin from Nanosalina sp. (NsXeR). Time-resolved infrared spectroscopy reveals the transient deprotonation of D220 concomitantly with deprotonation of the retinal Schiff base. Our molecular dynamics simulations support a proton release pathway from the retinal Schiff base via a hydrogen-bonded water wire leading to D220 that could provide a putative gating point for the proton release and with allosteric interactions to the retinal Schiff base. Our findings support the key role of D220 in mediating proton release to the cytoplasmic side and provide evidence that this residue is not the primary proton acceptor of the proton transiently released by the retinal Schiff base.

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