Kinetic study on the equilibrium between membrane-bound and free photoreceptor G-protein

Schleicher, Andreas; Hofmann, Klaus

doi:10.1007/bf01869489

Cited by 47 publications

(56 citation statements)

References 23 publications

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“…2B, trace a). Accordingly, dissociation of G t mb from the membrane upon activation is seen as decrease of LS ("dissociation signal" (20,36); Fig. 2B, trace b).…”

Section: Quantification Of Membrane-bound Transducin-mentioning

confidence: 95%

“…Notably, binding signals are generally slow as compared with dissociation signals. Previous work resolved this apparent conflict by the finding that, although binding of G t mb to R* is fast, interaction of G t sol with the membrane is slow (36). Consequently, the activation rate of G t sol is limited by its membrane binding, thereby leading to artificially slowed activation rates when total active G t * formation is assayed under conditions where a significant fraction of G t GDP is solubilized.…”

Section: Quantification Of Membrane-bound Transducin-mentioning

confidence: 99%

“…We thus used the kinetic light-scattering technique to obtain initial rates of G t mb activation. Previous work established the dissociation signal as a real time monitor of the fast activation of the membrane-bound fraction of G t GDP (20,36,37). A precise calibration can be obtained from the dependence on [R*] (37, 38) and/or from classical biochemical assays (this work).…”

Section: Steady State Analysis Of G T Activation Rate-mentioning

confidence: 99%

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Maximal Rate and Nucleotide Dependence of Rhodopsin-catalyzed Transducin Activation

Heck

Hofmann

2001

Journal of Biological Chemistry

151

155

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Despite the growing structural information on receptors and G proteins, the information on affinities and kinetics of protein-protein and protein-nucleotide interactions is still not complete. In this study on photoactivated rhodopsin (R*) and the rod G protein, G t , we have used kinetic light scattering, backed by direct biochemical assays, to follow G protein activation. Our protocol includes the following: (i) to measure initial rates on the background of rapid depletion of the G t GDP substrate; (ii) to titrate G t GDP, GTP, and GDP; and (iii) to apply a double displacement reaction scheme to describe the results. All data are simultaneously fitted by one and the same set of parameters. In retinal rod cells, absorption of a photon by the visual pigment rhodopsin initiates a cascade of biochemical reactions that eventually generates an electrical signal (1). Much of the tremendous overall gain (10 5 -10 6 ) of the visual cascade depends on two enzymatic amplification stages, namely the receptor-catalyzed nucleotide exchange in the rod G protein, transducin, and the hydrolysis of the second messenger cGMP by the effector, cGMP phosphodiesterase.Rhodopsin (R) and transducin (G t ) display fundamental similarities to other receptors and G proteins. However, the function of the rod as a single photon sensory cell requires both low basal activities of R and G t and high speed of catalytic nucleotide exchange in the G protein. Any catalytic activity of rhodopsin is effectively blocked in the dark by the covalently bound inverse agonist 11-cis-retinal. Although a mammalian rod cell contains ϳ10 7 rhodopsin molecules, thus providing the necessary target for efficient light absorption, spontaneous single photon-like activity originates only every 100 s from one of the many dormant receptors (2). On absorption of a photon, lightinduced isomerization converts the chromophore to the agonist all-trans-retinal, thereby triggering conformational changes in the receptor protein that result within milliseconds in the formation of the enzymatically active intermediate metarhodopsin II (for review, see Refs. 3 and 4). Once activated, rhodopsin finds by diffusion its substrate G t . In its inactive, GDPbound state (G t GDP), the heterotrimeric G t holoprotein is peripherally bound to the disc membrane by weak hydrophobic and ionic interactions (5-7). The activation of the G protein proceeds through a sequence of two mutual displacements (R* for GDP and GTP for R*; so-called double displacement mechanism). Collisional interaction between light-activated rhodopsin (R*) and G t GDP (Fig. 1A, step 1) triggers a conformational change that opens the G t ␣ nucleotide-binding site. Upon GDP release, a stable R*G t complex with an empty nucleotide-binding site on the G t ␣-subunit is formed (step 2). Binding of GTP to the G t ␣-subunit within the R*G t complex enables a second conformational change (step 3) that eventually induces the dissociation of active G t GTP (G t *) from the receptor (step 4) and the (simultaneous or unmeasurably...

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“…2B, trace a). Accordingly, dissociation of G t mb from the membrane upon activation is seen as decrease of LS ("dissociation signal" (20,36); Fig. 2B, trace b).…”

Section: Quantification Of Membrane-bound Transducin-mentioning

confidence: 95%

Section: Quantification Of Membrane-bound Transducin-mentioning

confidence: 99%

Section: Steady State Analysis Of G T Activation Rate-mentioning

confidence: 99%

See 1 more Smart Citation

Maximal Rate and Nucleotide Dependence of Rhodopsin-catalyzed Transducin Activation

Heck

Hofmann

2001

Journal of Biological Chemistry

151

155

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“…The changes in a dissociation signal were recorded as before (25,26). Measuring conditions were 3 M rhodopsin (WM), 0.4 M Gt, 500 M GTP, 20°C; 0.9% of rhodopsin was flash-activated.…”

Section: Methodsmentioning

confidence: 99%

Signal transfer from rhodopsin to the G-protein: Evidence for a two-site sequential fit mechanism

Kisselev

Meyer

Heck

et al. 1999

Proc. Natl. Acad. Sci. U.S.A.

105

115

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Photoactivation of the retinal photoreceptor rhodopsin proceeds through a cascade of intermediates, resulting in protein-protein interactions catalyzing the activation of the G-protein transducin (Gt). Using stabilization and photoregeneration of the receptor's signaling state and Gt activation assays, we provide evidence for a two-site sequential fit mechanism of Gt activation. We show that the C-terminal peptide from the Gt ␥-subunit, Gt␥(50-71)farnesyl, can replace the holoprotein in stabilizing rhodopsin's active intermediate metarhodopsin II (MII). However, the peptide cannot replace the Gt␤␥ complex in direct activation assays. Competition by Gt␥(50-71)farnesyl with Gt for the active receptor suggests a pivotal role for Gt␤␥ in signal transfer from MII to Gt. MII stabilization and competition is also found for the C-terminal peptide from the Gt ␣-subunit, Gt␣(340-350), but the capacity of this peptide to interfere in MII-Gt interactions is paradoxically low compared with its activity to stabilize MII. Besides this disparity, the pH profiles of competition with Gt are characteristically different for the two peptides. We propose a two-site sequential fit model for signal transfer from the activated receptor, R*, to the G-protein.In the center of the model is specific recognition of conformationally distinct sites of R* by Gt␣(340-350) and Gt␥(50-71)farnesyl. One matching pair of domains on the proteins would, on binding, lead to a conformational change in the G-protein and͞or receptor, with subsequent binding of the second pair of domains. This process could be the structural basis for GDP release and the formation of a stable empty site complex that is ready to receive the activating cofactor, GTP.Rhodopsin is a prototypical G-protein-coupled receptor in retinal rods (1, 2). Available information supports a mechanism in which the initial isomerization of the chromophore 11-cis-retinal, and thus the formation of the agonistic all-transretinal, leads to crucial contacts between the ligand and the apoprotein opsin. These steric constraints result in a defined arrangement of donor and acceptor groups for proton translocations leading to subsequent tautomeric conformations of the receptor, identified as ''metarhodopsin'' photointermediates, each with a characteristic absorption spectrum. Metarhodopsin I (MI, max ϭ 478 nm) is in a pH-and temperaturedependent equilibrium with metarhodopsin II (MII, max ϭ 380 nm), distinguished by its deprotonated Schiff base linkage [and broken salt bridge (3, 4)] between the retinal and Lys 296 . MII has been shown to catalyze retina rod cell-specific Gprotein (Gt) activation through nucleotide exchange (5, 6).Despite recent progress in structure determination of both Gt and rhodopsin, the molecular mechanism of signal transfer between the two proteins is poorly understood. Interacting surfaces of rhodopsin and Gt include intracellular loops of the receptor and domains on both Gt ␣-and Gt ␥-subunits (1, 7-9). C-terminal domains of Gt ␣-and Gt ␥-subunits, Gt␣(340-350) and...

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“…In the present study, the binding signals are used as a tool to determine the state of membrane binding (prior to the flash) of a protein. The shift of protein mass from solution to the membrane becomes the larger the less of the protein that is bound to the membrane before receptor activation (30,42). No binding signal will be seen when the protein is completely bound to the membrane.…”

Section: Light-induced Interaction Of Arrestin and Its Variants Withmentioning

confidence: 99%

Arrestin and Its Splice Variant Arr1–370A(p44)

Schröder

Pulvermüller

Hofmann

2002

Journal of Biological Chemistry

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Kinetic study on the equilibrium between membrane-bound and free photoreceptor G-protein

Cited by 47 publications

References 23 publications

Maximal Rate and Nucleotide Dependence of Rhodopsin-catalyzed Transducin Activation

Maximal Rate and Nucleotide Dependence of Rhodopsin-catalyzed Transducin Activation

Signal transfer from rhodopsin to the G-protein: Evidence for a two-site sequential fit mechanism

Arrestin and Its Splice Variant Arr1–370A(p44)

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