| Literature DB >> 26364583 |
Anna Dolnik1, Noreen Kanwal1,2, Sarah Mackert1,2, Sonja Halbedl1,2, Christian Proepper1, Juergen Bockmann1, Michael Schoen1, Tobias M Boeckers1, Susanne J Kühl3, Michael J Schmeisser1,4.
Abstract
Rap GTPase-activating proteins (RapGAPs) are essential for synaptic function as they tightly regulate synaptic Rap signaling. Among the most abundant synaptic RapGAPs in brain are the Spine-associated RapGAPs (SPARs) Sipa1l1/SPAR and Sipa1l2/SPAR2, whereas nothing has been reported on Sipa1l3/SPAR3. In this study, we show that Sipa1l3/SPAR3 is conserved across species, has a distinct expression pattern in the developing rat brain and is localized at excitatory postsynapses. We further demonstrate that the Sipa1l3/SPAR3 C-terminus is required for postsynaptic targeting and represents an interaction module for Fezzins such as ProSAPiP1/Lzts3, a binding partner of the postsynaptic scaffold protein Shank3. Taken together, our data imply that Sipa1l3/SPAR3 is a hitherto unknown synaptic RapGAP, which is targeted to postsynaptic specializations and interacts with Fezzins. Spine-associated RapGAPs (SPARs) are essential modulators of synaptic signaling. Our study is the first to characterize the SPAR family member Sipa1l3/SPAR3 in neuronal tissue. We show that Sipa1l3/SPAR3 is conserved across species, has a distinct expression pattern in brain and is localized to excitatory postsynapses via its C-terminus, which represents an interaction module for other postsynaptic proteins including the Fezzin ProSAPiP1/Lzts3.Entities:
Keywords: Lzts2; ProSAPiP1; Shank3; Sipa1l1; Sipa1l2; Sipa1l3
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Year: 2015 PMID: 26364583 DOI: 10.1111/jnc.13353
Source DB: PubMed Journal: J Neurochem ISSN: 0022-3042 Impact factor: 5.372