Literature DB >> 27355867

Arg188 drives RhoC membrane binding.

Aditi Patel1, Sophia Williams-Perez1, Nicole Peyton1, Amy Reicks1, Justin Buzick1, Janean Farley1, Sarah Shirar1, Shawn M Ellerbroek1.   

Abstract

RhoA and RhoC GTPases are 92% identical but demonstrate unique regulation and function. Phosphorylation of Ser188 has widely been reported to inhibit RhoA activity. RhoC possesses Arg188 in place of Ser188 but retains a canonical upstream PKA recognition sequence. We report here that RhoC-R188S was a PKA substrate in vitro and exhibited less GTP loading compared to wild-type RhoC when expressed in cells. Transiently expressed RhoC was found to be significantly more membrane associated than RhoA. Membrane association of RhoC-R188S and RhoC-R188A were similar to each other and wild-type RhoA, suggesting that Arg188 directly promotes RhoC membrane binding. The positive influence of Arg188 on RhoC membrane association was evident in a constitutively active (Q63L) background. In accordance, RhoA-S188R was significantly more membrane associated than either RhoA or RhoA-S188A. Altogether, these data suggest that swapping residue 188 identity effectively flips the membrane binding profile of wild-type RhoA and RhoC through positive arginine contribution rather than negative phosphoserine regulation.

Entities:  

Keywords:  RhoA; RhoC; arginine; membrane; serine

Mesh:

Substances:

Year:  2016        PMID: 27355867      PMCID: PMC5464120          DOI: 10.1080/21541248.2016.1205334

Source DB:  PubMed          Journal:  Small GTPases        ISSN: 2154-1248


  25 in total

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  1 in total

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