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The laser-induced blue state of bacteriorhodopsin: Mechanistic and color regulatory roles of protein-protein interactions, protein-lipid interactions, and metal ions

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JOURNAL OF THE AMERICAN CHEMICAL SOCIETY
卷 124, 期 13, 页码 3418-3430

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AMER CHEMICAL SOC
DOI: 10.1021/ja010116a

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  1. NIGMS NIH HHS [2S06 GM 08066-25] Funding Source: Medline

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In this paper we characterize the mechanistic roles of the crystalline purple membrane (PM) lattice, the earliest bacteriorhodopsin (BR) photocycle intermediates, and divalent cations in the conversion of PM to laser-induced blue membrane (LIBM; lambdamax = 605 nm) upon irradiation with intense 532 nm pulses by contrasting the photoconversion of PM with that of monomeric BR solubilized in reduced Triton X-100 detergent. Monomeric BR forms a previously unreported colorless monomer photoproduct which lacks a chromophore band in the visible region but manifests a new band centered near 360 nm similar to the 360 nm band in LIBM. The 360 nm band in both LIBM and colorless monomer originates from a Schiff base-reduced retinyl chromophore which remains covalently linked to bacterioopsin. Both the PM-LIBM and monomer-->colorless monomer photoconversions are mediated by similar biphotonic mechanisms, indicating that the photochemistry is localized within single BR monomers and is not influenced by BR-BR interactions. The excessively large two-photon absorptivities (greater than or equal to10(6) cm(4) s molecule(-1) photow(-1)) of these photoconversions, the temporal and spectral characteristics of pulses which generate LIBM in high yield, and an action spectrum for the PM-->LIBM photoconversion all indicate that the PM-->LIBM and Mon-->CMon photoconversions are both mediated by a sequential biphotonic mechanism in which I-460(*) is the intermediate which absorbs the second photon. The purple-->blue color change results from subsequent conformational perturbations of the PM lattice which induce the removal of Ca2+ and Mg2+ ions from the PM surface.

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