Curated Information

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PubMed Id: 15753124

This page summarizes selected information from the article referenced above and curated into PhosphoSitePlus^®, a comprehensive online resource for the study of protein post-translational modifications (NAR, 2012,40:D261-70). To learn more about the scope of PhosphoSitePlus^®, click here.

Yamada E, et al. (2005) Akt2 phosphorylates Synip to regulate docking and fusion of GLUT4-containing vesicles. J Cell Biol 168, 921-8 15753124

S99-p - STXBP4 (mouse)

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Orthologous residues

STXBP4 (human): S99‑p, STXBP4 iso4 (human): S24‑p, STXBP4 (mouse): S99‑p

Characterization

Methods used to characterize site in vivo: mutation of modification site, phospho-antibody

Cellular systems studied: cell lines

Species studied: hamster

Enzymes shown to modify site in vitro:

Type	Enzyme
KINASE	Akt2 (mouse)

Upstream Regulation

Potential in vivo enzymes for site:

Type	Enzyme	Evidence	Notes
KINASE	Akt2 (mouse)	transfection of wild-type enzyme, co-immunoprecipitation

Treatments, proteins and their effect on site modification:

Treatments	Referenced Treatments	Manipulated Protein	Referenced Protein	Effect	Notes
insulin				increase

Downstream Regulation

Effect of modification (function): molecular association, regulation

Modification regulates interactions with:

Interacting molecule	Interacting domains	Effect	Consequences (function)	Consequences (process)	Detection assays
GLUT4 (mouse)		Disrupts	intracellular localization		co-immunoprecipitation, electrophoretic visualization
STX4 (mouse)		Disrupts	intracellular localization		co-immunoprecipitation, electrophoretic visualization

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