BAIT

SEC17

RNS3, L000001841, YBL050W

Alpha-SNAP cochaperone; SNARE-complex adaptor for Sec18 (NSF) during the disassembly of postfusion cis-SNARE complexes; stimulates the ATPase activity of Sec18p; peripheral membrane protein required for vesicular transport between ER and Golgi, the 'priming' step in homotypic vacuole fusion, and autophagy; similar to mammalian alpha-SNAP

GO Process (4)

GO Function (2)

GO Component (4)

Gene Ontology Biological Process

SNARE complex disassembly [IDA]

autophagy [IMP]

vacuole fusion, non-autophagic [IDA]

vesicle fusion with Golgi apparatus [IDA]

Gene Ontology Molecular Function

ATPase activator activity [IDA]
soluble NSF attachment protein activity [IDA, IPI]

Gene Ontology Cellular Component

SNARE complex [IPI]

cytosol [IDA]

extrinsic component of membrane [IDA]

fungal-type vacuole membrane [IDA]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

PREY

SED5

L000001861, YLR026C

cis-Golgi t-SNARE syntaxin; required for vesicular transport between the ER and the Golgi complex; binds at least 9 SNARE proteins

GO Process (4)

GO Function (1)

GO Component (3)

Gene Ontology Biological Process

ER to Golgi vesicle-mediated transport [IMP]

intra-Golgi vesicle-mediated transport [IMP]

vesicle fusion [IDA]

vesicle fusion with Golgi apparatus [IMP]

Gene Ontology Molecular Function

SNAP receptor activity [IDA]

Gene Ontology Cellular Component

SNARE complex [IDA]

cis-Golgi network [IDA]

integral component of membrane [IDA]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

Affinity Capture-Western

An interaction is inferred when a bait protein is affinity captured from cell extracts by either polyclonal antibody or epitope tag and the associated interaction partner identified by Western blot with a specific polyclonal antibody or second epitope tag. This category is also used if an interacting protein is visualized directly by dye stain or radioactivity. Note that this differs from any co-purification experiment involving affinity capture in that the co-purification experiment involves at least one extra purification step to get rid of potential contaminating proteins.

Publication

Characterization of a novel yeast SNARE protein implicated in Golgi retrograde traffic.

Lupashin VV, Pokrovskaya ID, McNew JA, Waters MG

The protein trafficking machinery of eukaryotic cells is employed for protein secretion and for the localization of resident proteins of the exocytic and endocytic pathways. Protein transit between organelles is mediated by transport vesicles that bear integral membrane proteins (v-SNAREs) which selectively interact with similar proteins on the target membrane (t-SNAREs), resulting in a docked vesicle. A novel Saccharomyces cerevisiae ... [more]

Mol. Biol. Cell Dec. 01, 1997; 8(12);2659-76 [Pubmed: 9398683]

Throughput

Low Throughput

Related interactions

Interaction	Experimental Evidence Code	Dataset	Throughput	Score	Curated By	Notes
SED5 SEC17	Affinity Capture-Western Affinity Capture-Western An interaction is inferred when a bait protein is affinity captured from cell extracts by either polyclonal antibody or epitope tag and the associated interaction partner identified by Western blot with a specific polyclonal antibody or second epitope tag. This category is also used if an interacting protein is visualized directly by dye stain or radioactivity. Note that this differs from any co-purification experiment involving affinity capture in that the co-purification experiment involves at least one extra purification step to get rid of potential contaminating proteins.	Holthuis JC (1998)	Low	-	BioGRID	-
SED5 SEC17	Affinity Capture-Western Affinity Capture-Western An interaction is inferred when a bait protein is affinity captured from cell extracts by either polyclonal antibody or epitope tag and the associated interaction partner identified by Western blot with a specific polyclonal antibody or second epitope tag. This category is also used if an interacting protein is visualized directly by dye stain or radioactivity. Note that this differs from any co-purification experiment involving affinity capture in that the co-purification experiment involves at least one extra purification step to get rid of potential contaminating proteins.	Kosodo Y (2003)	Low	-	BioGRID	-
SED5 SEC17	Affinity Capture-Western Affinity Capture-Western An interaction is inferred when a bait protein is affinity captured from cell extracts by either polyclonal antibody or epitope tag and the associated interaction partner identified by Western blot with a specific polyclonal antibody or second epitope tag. This category is also used if an interacting protein is visualized directly by dye stain or radioactivity. Note that this differs from any co-purification experiment involving affinity capture in that the co-purification experiment involves at least one extra purification step to get rid of potential contaminating proteins.	Schindler C (2007)	Low	-	BioGRID	-
SED5 SEC17	Affinity Capture-Western Affinity Capture-Western An interaction is inferred when a bait protein is affinity captured from cell extracts by either polyclonal antibody or epitope tag and the associated interaction partner identified by Western blot with a specific polyclonal antibody or second epitope tag. This category is also used if an interacting protein is visualized directly by dye stain or radioactivity. Note that this differs from any co-purification experiment involving affinity capture in that the co-purification experiment involves at least one extra purification step to get rid of potential contaminating proteins.	Sogaard M (1994)	Low	-	BioGRID	202241
SED5 SEC17	Co-purification Co-purification An interaction is inferred from the identification of two or more protein subunits in a purified protein complex, as obtained by classical biochemical fractionation or affinity purification and one or more additional fractionation steps.	Inadome H (2005)	Low	-	BioGRID	-
SEC17 SED5	Negative Genetic Negative Genetic Mutations/deletions in separate genes, each of which alone causes a minimal phenotype, but when combined in the same cell results in a more severe fitness defect or lethality under a given condition. This term is reserved for high or low throughput studies with scores.	Costanzo M (2016)	High	-0.1936	BioGRID	1919506
SED5 SEC17	Negative Genetic Negative Genetic Mutations/deletions in separate genes, each of which alone causes a minimal phenotype, but when combined in the same cell results in a more severe fitness defect or lethality under a given condition. This term is reserved for high or low throughput studies with scores.	Costanzo M (2016)	High	-0.1224	BioGRID	1942921

Curated By

BioGRID

Interaction Summary

SEC17

Gene Ontology Biological Process

Gene Ontology Molecular Function

ATPase activator activity [IDA]soluble NSF attachment protein activity [IDA, IPI]

Gene Ontology Cellular Component

SED5

Gene Ontology Biological Process

Gene Ontology Molecular Function

SNAP receptor activity [IDA]

Gene Ontology Cellular Component

Affinity Capture-Western

Publication

Characterization of a novel yeast SNARE protein implicated in Golgi retrograde traffic.

Throughput

Related interactions

Curated By

ATPase activator activity [IDA]
soluble NSF attachment protein activity [IDA, IPI]