Characterization of a Phospholipase C β2-Binding Site Near the Amino-terminal Coiled-coil of G Protein βγ Subunits

Yoshikawa, Daniel M.; Bresciano, Karen; Hatwar, Mamata; Smrcka, Alan V.

doi:10.1074/jbc.m006073200

Cited by 19 publications

(22 citation statements)

References 22 publications

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“…The current data with AGS8 in both the yeast and mammalian systems along with the recent reports regarding direct regulation of G␤␥ (27,28) and diversity of G␤␥ binding partners (29,30) suggest that G␤␥ may possess additional protein binding sites for signal processing (28,31). Such G␤␥ binding partners may serve as effectors for mammalian G␤␥, influence receptor coupling to G␣␤␥ or localize G␤␥ within a larger signaling complex, where it can regulate specific signaling pathways independent of the classical heterotrimeric G␣␤␥.…”

Section: Resultsmentioning

confidence: 99%

Identification of a receptor-independent activator of G protein signaling (AGS8) in ischemic heart and its interaction with Gβγ

Sato

Cismowski

Toyota

et al. 2006

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

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As part of a broader effort to identify postreceptor signal regulators involved in specific diseases or organ adaptation, we used an expression cloning system in Saccharomyces cerevisiae to screen cDNA libraries from rat ischemic myocardium, human heart, and a prostate leiomyosarcoma for entities that activated G protein signaling in the absence of a G protein coupled receptor. We report the characterization of activator of G protein signaling (AGS) 8 (KIAA1866), isolated from a rat heart model of repetitive transient ischemia. AGS8 mRNA was induced in response to ventricular ischemia but not by tachycardia, hypertrophy, or failure. Hypoxia induced AGS8 mRNA in isolated adult ventricular cardiomyocytes but not in rat aortic smooth muscle cells, endothelial cells, or cardiac fibroblasts, suggesting a myocyte-specific adaptation mechanism involving remodeling of G protein signaling pathways. The bioactivity of AGS8 in the yeast-based assay was independent of guanine nucleotide exchange by G␣, suggesting an impact on subunit interactions. Subsequent studies indicated that AGS8 interacts directly with G␤␥ and this occurs in a manner that apparently does not alter the regulation of the effector PLC-␤ 2 by G␤␥. Mechanistically, AGS8 appears to promote G protein signaling by a previously unrecognized mechanism that involves direct interaction with G␤␥.accessory protein ͉ signal adaptation ͉ hypoxia

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Section: Resultsmentioning

confidence: 99%

Identification of a receptor-independent activator of G protein signaling (AGS8) in ischemic heart and its interaction with Gβγ

Sato

Cismowski

Toyota

et al. 2006

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

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“…Previous work has found that G␤␥ contains multiple binding sites for PLC␤2. In addition to the G␣ contact surface, the N-terminal coiled coil domain and the outer surface of the G␤ are also involved in binding PLC␤2 (22,31). In the absence of other constraints, G␤␥ activates PLC␤2 primarily through the G␣ t contact region (26).…”

Section: Discussionmentioning

confidence: 99%

WDR26 Functions as a Scaffolding Protein to Promote Gβγ-mediated Phospholipase C β2 (PLCβ2) Activation in Leukocytes

Sun¹,

Smrcka

Chen

2013

Journal of Biological Chemistry

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Background: It remains unclear how G␤␥ regulates diverse effectors in cells. Results: WDR26 exists in oligomers. It simultaneously binds both G␤␥ and PLC␤2 to enhance PLC␤2 membrane translocation and activation by G␤␥ in leukocytes. Conclusion: WDR26 functions as a scaffolding protein to promote G␤␥-mediated PLC␤2 activation. Significance: These findings uncover a novel mechanism of regulating G␤␥ signaling through a scaffolding protein.

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“…In line with this, by swapping the PH domain of PLC-β2 into the remainder of PLC-δ1, we obtained a chimera that binds non-specifically to membranes like PLC-β2, and moreover, binds and is responsive to Gβγ subunits [72]. In two distinct studies, it was found that the N-terminal region of PLC-β3 encompassing the PH domain and a part of the EF-hands region binds to Gβγ [73] whereas it was reported that Gβγ helps the recruitment of a GFP-tagged PH-β1 on subcellular membranes [74] Additionally, an independent series of studies located a solvent-accessible segment of nine residues (574-583 segment) in the Y region that is able to bind to Gβ [71,[75][76][77]. This segment, although partially-conserved in PLC-δ1, could govern the oscillation of the PLC-β2 between two distinct parts of Gβ subunit to be distal or proximal to the membrane surface [71].…”

Section: Gβγ Binding Site(s) In Plc-β2mentioning

confidence: 99%

“…Comparing a model structure of PH-β2 with the known structure of PH-δ1 suggests that the β5/β6 loop, which is longer than in PH-δ1, (Figure 3) could act as a regulatory domain for activation by Gβγ [41]. A peptide corresponding to this loop (PHβ [71][72][73][74][75][76][77][78][79][80][81][82][83][84][85][86][87][88] ) activates the enzyme, and this activation is competitive with Gβγ activation. The structure of PLC-β2 reveals that the β5/β6 loop does not belong to the surface that is tightly packed with the EF-hands and the catalytic regions, or to the hydrophobic ridge interacting with Rac2.…”

Section: Role Of the Ph Domain In Plc-δ1 And Plc-β2 Activationmentioning

confidence: 99%

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Stimulation of phospholipase Cβ by membrane interactions, interdomain movement, and G protein binding — How many ways can you activate an enzyme?

Drin

Scarlata

2007

Cellular Signalling

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Signaling proteins are usually composed of one or more conserved structural domains. These domains are usually regulatory in nature by binding to specific activators or effectors, or species that regulate cellular location, etc. Inositol-specific mammalian phospholipase C (PLC) enzymes are multidomain proteins whose activities are controlled by regulators, such as G proteins, as well as membrane interactions. One of these domains has been found to bind membranes, regulators, and activate the catalytic region. The recently solved structure of a major region of PLC-β2 together with the structure of PLC-δ1 and a wealth of biochemical studies poises the system towards an understanding of the mechanism through which their regulations occurs.

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Characterization of a Phospholipase C β2-Binding Site Near the Amino-terminal Coiled-coil of G Protein βγ Subunits

Cited by 19 publications

References 22 publications

Identification of a receptor-independent activator of G protein signaling (AGS8) in ischemic heart and its interaction with Gβγ

Identification of a receptor-independent activator of G protein signaling (AGS8) in ischemic heart and its interaction with Gβγ

WDR26 Functions as a Scaffolding Protein to Promote Gβγ-mediated Phospholipase C β2 (PLCβ2) Activation in Leukocytes

Stimulation of phospholipase Cβ by membrane interactions, interdomain movement, and G protein binding — How many ways can you activate an enzyme?

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