Article Information
PubMed
Related Articles
- Subsecond Proton-Hole Propagation in BacteriorhodopsinSubsecond Proton-Hole Propagation in Bacteriorhodopsin
Biophysical Journal, Volume 84, Issue 1, 1 January 2003, Pages 671-686
Bettina Schätzler, Norbert A. Dencher, Joerg Tittor, Dieter Oesterhelt, Sharon Yaniv-Checover, Esther Nachliel and Menachem Gutman
AbstractThe dynamics of proton transfer between the surface of purple membrane and the aqueous bulk have recently been investigated by the Laser Induced Proton Pulse Method. Following a Δ-function release of protons to the bulk, the system was seen to regain its state of equilibrium within a few hundreds of microseconds. These measurements set the time frame for the relaxation of any state of acid-base disequilibrium between the bacteriorhodopsin’s surface and the bulk. It was also deduced that the released protons react with the various proton binding within less than 10. In the present study, we monitored the photocycle and the proton-cycle of photo-excited bacteriorhodopsin, in the absence of added buffer, and calculated the proton balance between the Schiff base and the bulk phase in a time-resolved mode. It was noticed that the late phase of the M decay (beyond 1ms) is characterized by a slow (subsecond) relaxation of disequilibrium, where the Schiff base is already reprotonated but the pyranine still retains protons. Thus, it appears that the protonation of D96 is a slow rate-limiting process that generates a “proton hole” in the cytoplasmic section of the protein. The velocity of the hole propagation is modulated by the ionic strength of the solution and by selective replacements of charged residues on the interhelical loops of the protein, at domains that seems to be remote from the intraprotein proton conduction trajectory.
Abstract | Full Text | PDF (679 kb) - Time-Resolved X-Ray Diffraction Reveals Movement of F Helix ...Time-Resolved X-Ray Diffraction Reveals Movement of F Helix of D96N Bacteriorhodopsin during M-MN Transition at Neutral pH
Biophysical Journal, Volume 82, Issue 5, 1 May 2002, Pages 2610-2616
Toshihiko Oka, Naoto Yagi, Fumio Tokunaga and Mikio Kataoka
AbstractD96N bacteriorhodopsin has two photointermediates with the deprotonated Schiff base: the M and MN intermediates. We measure the time-resolved x-ray diffraction of the D96N purple membrane after flash photoexcitation (pH 7.0, 25°C). The data clearly show the M-MN transition during the D96N photocycle. Low-resolution projection maps of these states show that the F helix of the MN intermediate shifts from its original position and this shift is much larger than that of the M intermediate. This indicates that the F helix moves in the M-MN transition of the D96N bacteriorhodopsin photocycle. Moreover, the existence of the MN intermediate in the D96N photocycle under neutral pH indicates that the MN intermediate is not peculiar to the alkaline condition. It is notable that the structural transition of M-MN is independent of the protonation state of the Schiff base. Therefore, the F helix movement precedes reprotonation of the Schiff base in the bacteriorhodopsin photocycle. Our previous study showed that the M-MN transition is hydration-dependent and that the MN intermediate is more hydrated than the M intermediate. Considering this together with the present results, we conclude that the movement of the F helix causes hydration of the cytoplasmic side, which promotes the reprotonation of the Schiff base.
Abstract | Full Text | PDF (145 kb) - Sensory Rhodopsin II from the Haloalkaliphilic Natronobacter...Sensory Rhodopsin II from the Haloalkaliphilic Natronobacterium pharaonis: Light-Activated Proton Transfer Reactions
Biophysical Journal, Volume 78, Issue 2, 1 February 2000, Pages 967-976
G. Schmies, B. Lüttenberg, I. Chizhov, M. Engelhard, A. Becker and E. Bamberg
AbstractIn the present work the light-activated proton transfer reactions of sensory rhodopsin II from (pSRII) and those of the channel-mutants D75N-pSRII and F86D-pSRII are investigated using flash photolysis and black lipid membrane (BLM) techniques. Whereas the photocycle of the F86D-pSRII mutant is quite similar to that of the wild-type protein, the photocycle of D75N-pSRII consists of only two intermediates. The addition of external proton donors such as azide, or in the case of F86D-pSRII, imidazole, accelerates the reprotonation of the Schiff base, but not the turnover. The electrical measurements prove that pSRII and F86D-pSRII can function as outwardly directed proton pumps, whereas the mutation in the extracellular channel (D75N-pSRII) leads to an inwardly directed transient current. The almost negligible size of the photostationary current is explained by the long-lasting photocycle of about a second. Although the M decay, but not the photocycle turnover, of pSRII and F86D-pSRII is accelerated by the addition of azide, the photostationary current is considerably increased. It is discussed that in a two-photon process a late intermediate (N- and/or O-like species) is photoconverted back to the original resting state; thereby the long photocycle is cut short, giving rise to the large increase of the photostationary current. The results presented in this work indicate that the function to generate ion gradients across membranes is a general property of archaeal rhodopsins.
Abstract | Full Text | PDF (193 kb) - …more
Copyright © 1995 The Biophysical Society. All rights reserved.
Biophysical Journal, Volume 69, Issue 5, 2103-2111, 1 November 1995
doi:10.1016/S0006-3495(95)80081-0
Research Article
Functional significance of a protein conformation change at the cytoplasmic end of helix F during the bacteriorhodopsin photocycle
L.S. Brown, G. Váró, R. Needleman and J.K. Lanyi
Department of Physiology and Biophysics, University of California, Irvine 92717, USA.
Abstract
The second half of the photocycle of the light-driven proton pump bacteriorhodopsin includes proton transfers between D96 and the retinal Schiff base (the M to N reaction) and between the cytoplasmic surface and D96 (decay of the N intermediate). The inhibitory effects of decreased water activity and increased hydrostatic pressure have suggested that a conformational change resulting in greater hydration of the cytoplasmic region is required for proton transfer from D96 to the Schiff base, and have raised the possibility that the reversal of this process might be required for the subsequent reprotonation of D96 from the cytoplasmic surface. Tilt of the cytoplasmic end of helix F has been suggested by electron diffraction of the M intermediate. Introduction of bulky groups, such as various maleimide labels, to engineered cysteines at the cytoplasmic ends of helices A, B, C, E, and G produce only minor perturbation of the decays of M and N, but major changes in these reactions when the label is linked to helix F. In these samples the reprotonation of the Schiff base is accelerated and the reprotonation of D96 is strongly retarded. Cross-linking with benzophenone introduced at this location, but not at the others, causes the opposite change: the reprotonation of the Schiff base is greatly slowed while the reprotonation of D96 is accelerated. We conclude that, consistent with the structure from diffraction, the proton transfers in the second half of the photocycle are facilitated by motion of the cytoplasmic end of helix F, first away from the center of the protein and then back.
