Functional comparison of RGS9 splice isoforms in a living cell

Martemyanov, Kirill A.; Krispel, Claudia M.; Lishko, Polina V.; Burns, Marie E.; Arshavsky, Vadim Y.

doi:10.1073/pnas.0808941106

Cited by 27 publications

(35 citation statements)

References 48 publications

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“…5A,C), with levels ranging between 1.7 and 4.9-fold above the wild type RGS9-1 content. We noted, however, that measurements of protein content had unusual variability among mice of the same line, leading us to suggest that rods from ggR9AP mice exhibit mosaicism in their expression of the transgene, as occasionally observed in transgenic lines using this promoter (Lem et al, 1991) and encountered in one of our recent studies (Martemyanov et al, 2008). Staining of R9AP −/− ggR9AP retinal flatmounts for R9AP revealed that this was indeed the case, as patches of rhodopsin-positive outer segments without R9AP expression were easily identified (Fig.…”

Section: Resultsmentioning

confidence: 73%

Membrane Attachment Is Key to Protecting Transducin GTPase-Activating Complex from Intracellular Proteolysis in Photoreceptors

Gospe¹,

Baker²,

Kessler³

et al. 2011

J. Neurosci.

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The members of the R7 RGS protein sub-family are versatile regulators of G protein signaling throughout the nervous system. Recent studies indicate that they are often found in complexes with membrane anchor proteins which serve as versatile modulators of their activity, intracellular targeting and stability. One striking example is the interplay between the membrane anchor R9AP and the RGS9-1·Gβ5 GTPase activating complex responsible for the rapid inactivation of the G protein transducin in vertebrate photoreceptor cells during their recovery from light excitation. The amount of this complex in photoreceptors sets their temporal resolution and is precisely regulated by the expression level of R9AP, which serves to protect the RGS9-1 and Gβ5 subunits from intracellular proteolysis. In this study, we investigated the mechanism by which R9AP performs its protective function in mouse rods and found that it is entirely confined to recruiting RGS9-1·Gβ5 to cellular membranes. Furthermore, membrane attachment of RGS9-1·Gβ5 is sufficient for its stable expression in rods even in the absence of R9AP. Our second finding is that RGS9-1·Gβ5 possesses targeting information that specifies its exclusion from the outer segment and that this information is neutralized by association with R9AP to allow outer segment targeting. Finally, we demonstrate that the ability of R9AP·RGS9-1·Gβ5 to accelerate GTP hydrolysis on transducin is independent of its means of membrane attachment, since replacing the transmembrane domain of R9AP with a site for lipid modification did not impair the catalytic activity of this complex.

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Section: Resultsmentioning

confidence: 73%

Membrane Attachment Is Key to Protecting Transducin GTPase-Activating Complex from Intracellular Proteolysis in Photoreceptors

Gospe¹,

Baker²,

Kessler³

et al. 2011

J. Neurosci.

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“…The second, longer ‘dominant time constant’ (of 600–800 ms) observed in electrophysiological measurements on mouse rods has been proposed to reflect the time constant of such decay of free G* in vivo , on the basis of experiments incorporating RGS9-2 into rods [42]. We concur with that interpretation, and note that it conforms with the biochemical finding that, in the presence of the RGS domain of RGS9 but in the absence of PDE γ , the rate of GTP hydrolysis by activated transducin is around 1 s −1 [43] (in contrast to the much slower rate for purified transducin α-subunits, of around 0.05 s −1 [44]).…”

Section: Discussionmentioning

confidence: 99%

Implications of dimeric activation of PDE6 for rod phototransduction

2018

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We examine the implications of a recent report providing evidence that two transducins must bind to the rod phosphodiesterase to elicit significant hydrolytic activity. To predict the rod photoreceptor's electrical response, we use numerical simulation of the two-dimensional diffusional contact of interacting molecules at the surface of the disc membrane, and then we use the simulated PDE activity as the driving function for the downstream reaction cascade. The results account for a number of aspects of rod phototransduction that have previously been puzzling. For example, they explain the existence of a greater initial delay in rods than in cones. Furthermore, our analysis suggests that the ‘continuous’ noise recorded in rods in darkness is likely to arise from spontaneous activation of individual molecules of PDE at a rate of a few tens per second per rod, probably as a consequence of spontaneous activation of transducins at a rate of thousands per second per rod. Hence, the dimeric activation of PDE in rods provides immunity against spontaneous transducin activation, thereby reducing the continuous noise. Our analysis also provides a coherent quantitative explanation of the amplification underlying the single photon response. Overall, numerical analysis of the dimeric activation of PDE places rod phototransduction in a new light.

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“…45,47,48 A recent report showed that RGS9-2 can functionally substitute for RGS9-1 in photoreceptors and, in fact, appears to be a more efficient inhibitor of transducin than RGS9-1. 49 …”

Section: Structure Of Gβ5–r7 Complexes the Role Of Rgs Ggl Andmentioning

confidence: 99%

Chapter 6 Structure, Function, and Localization of Gβ5–RGS Complexes

Slepak

2009

Progress in Molecular Biology and Translational Science

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Members of the R7 subfamily of regulator of G protein signaling (RGS) proteins (RGS6, 7, 9, and 11) exist as heterodimers with the G protein beta subunit Gβ5. These protein complexes are only found in neurons and are defined by the presence of three domains: DEP/DHEX, Gβ5/GGL, and RGS. This article summarizes published work in the following areas: (1) the functional significance of structural organization of Gβ5–R7 complexes, (2) regional distribution of Gβ5–R7 in the nervous system and regulation of R7 family expression, (3) subcellular localization of Gβ5–R7 complexes, and (4) novel binding partners of Gβ5–R7 proteins. The review points out some contradictions between observations made by different research groups and highlights the importance of using alternative experimental approaches to obtain conclusive information about Gβ5–R7 function in vivo.

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Functional comparison of RGS9 splice isoforms in a living cell

Cited by 27 publications

References 48 publications

Membrane Attachment Is Key to Protecting Transducin GTPase-Activating Complex from Intracellular Proteolysis in Photoreceptors

Membrane Attachment Is Key to Protecting Transducin GTPase-Activating Complex from Intracellular Proteolysis in Photoreceptors

Implications of dimeric activation of PDE6 for rod phototransduction

Chapter 6 Structure, Function, and Localization of Gβ5–RGS Complexes

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