BAIT

DOA4

DOS1, MUT4, NPI2, SSV7, UBP4, L000000514, YDR069C

Ubiquitin hydrolase; deubiquitinates intralumenal vesicle (ILVs) cargo proteins; required for recycling ubiquitin from proteasome-bound ubiquitinated intermediates, acts at the late endosome/prevacuolar compartment to recover ubiquitin from ubiquitinated membrane proteins destined for the vacuole; DOA4 has a paralog, UBP5, that arose from the whole genome duplication

UPS Project

GO Process (7)

GO Function (1)

GO Component (3)

Gene Ontology Biological Process

endocytosis [IMP]

free ubiquitin chain depolymerization [IDA]

intralumenal vesicle formation [IGI]

regulation of DNA replication [IMP]

ubiquitin homeostasis [IMP]

ubiquitin-dependent protein catabolic process [IMP]

ubiquitin-dependent protein catabolic process via the multivesicular body sorting pathway [IMP]

Gene Ontology Molecular Function

ubiquitin-specific protease activity [IDA, IMP]

Gene Ontology Cellular Component

endosome [IDA]

mitochondrion [IDA]

proteasome complex [IPI]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

PREY

BRO1

ASI6, LPF2, NPI3, VPS31, L000003061, YPL084W

Cytoplasmic class E vacuolar protein sorting (VPS) factor; coordinates deubiquitination in the multivesicular body (MVB) pathway by recruiting Doa4p to endosomes

GO Process (6)

GO Function (1)

GO Component (2)

Gene Ontology Biological Process

intralumenal vesicle formation [IGI, IMP]

protein deubiquitination [IGI, IPI]

protein targeting to vacuole involved in ubiquitin-dependent protein catabolic process via the multivesicular body sorting pathway [IMP]

response to nutrient [IMP]

ubiquitin-dependent protein catabolic process [IMP]

vacuolar transport [IMP]

Gene Ontology Molecular Function

ubiquitin-specific protease activity [IDA]

Gene Ontology Cellular Component

cytoplasm [IDA]

endosome [IDA]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

Phenotypic Suppression

A genetic interaction is inferred when mutation or over expression of one gene results in suppression of any phenotype (other than lethality/growth defect) associated with mutation or over expression of another gene.

Publication

Regulation of yeast ESCRT-III membrane scission activity by the Doa4 ubiquitin hydrolase.

Johnson N, West M, Odorizzi G

ESCRT-III executes membrane scission during the budding of intralumenal vesicles (ILVs) at endosomes. The scission mechanism is unknown but appears to be linked to the cycle of assembly and disassembly of ESCRT-III complexes at membranes. Regulating this cycle is, therefore, expected to be important for determining the timing of ESCRT-III-mediated membrane scission. We show in Saccharomyces cerevisiae that ESCRT-III complexes ... [more]

Mol. Biol. Cell Jan. 05, 2017; 0(0); [Pubmed: 28057764]

Throughput

Low Throughput

Ontology Terms

protein/peptide accumulation (APO:0000149)

Additional Notes

BRO1 overexpression rescues ESCRT-III complex instability in doa4 mutant
Figure 1

Related interactions

Interaction	Experimental Evidence Code	Dataset	Throughput	Score	Curated By	Notes
DOA4 BRO1	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.	Luhtala N (2004)	Low	-	BioGRID	-
BRO1 DOA4	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.	Nikko E (2007)	Low	-	BioGRID	-
DOA4 BRO1	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.	Richter C (2007)	Low	-	BioGRID	-
DOA4 BRO1	Co-localization Co-localization Interaction inferred from two proteins that co-localize in the cell by indirect immunofluorescence only when in addition, if one gene is deleted, the other protein becomes mis-localized. Also includes co-dependent association of proteins with promoter DNA in chromatin immunoprecipitation experiments.	Luhtala N (2004)	Low	-	BioGRID	-
BRO1 DOA4	PCA PCA A Protein-Fragment Complementation Assay (PCA) is a protein-protein interaction assay in which a bait protein is expressed as fusion to one of the either N- or C- terminal peptide fragments of a reporter protein and prey protein is expressed as fusion to the complementary N- or C- terminal fragment of the same reporter protein. Interaction of bait and prey proteins bring together complementary fragments, which can then fold into an active reporter, e.g. the split-ubiquitin assay.	Nikko E (2007)	Low	-	BioGRID	237982
DOA4 BRO1	PCA PCA A Protein-Fragment Complementation Assay (PCA) is a protein-protein interaction assay in which a bait protein is expressed as fusion to one of the either N- or C- terminal peptide fragments of a reporter protein and prey protein is expressed as fusion to the complementary N- or C- terminal fragment of the same reporter protein. Interaction of bait and prey proteins bring together complementary fragments, which can then fold into an active reporter, e.g. the split-ubiquitin assay.	Nikko E (2007)	Low	-	BioGRID	237983
BRO1 DOA4	Phenotypic Suppression Phenotypic Suppression A genetic interaction is inferred when mutation or over expression of one gene results in suppression of any phenotype (other than lethality/growth defect) associated with mutation or over expression of another gene.	Johnson N (2017)	Low	-	BioGRID	2200769
BRO1 DOA4	Phenotypic Suppression Phenotypic Suppression A genetic interaction is inferred when mutation or over expression of one gene results in suppression of any phenotype (other than lethality/growth defect) associated with mutation or over expression of another gene.	Luhtala N (2004)	Low	-	BioGRID	163196
DOA4 BRO1	Two-hybrid Two-hybrid Bait protein expressed as a DNA binding domain (DBD) fusion and prey expressed as a transcriptional activation domain (TAD) fusion and interaction measured by reporter gene activation.	Richter C (2007)	Low	-	BioGRID	-

Curated By

BioGRID

Interaction Summary

DOA4

Gene Ontology Biological Process

Gene Ontology Molecular Function

ubiquitin-specific protease activity [IDA, IMP]

Gene Ontology Cellular Component

BRO1

Gene Ontology Biological Process

Gene Ontology Molecular Function

ubiquitin-specific protease activity [IDA]

Gene Ontology Cellular Component

Phenotypic Suppression

Publication

Regulation of yeast ESCRT-III membrane scission activity by the Doa4 ubiquitin hydrolase.

Throughput

Ontology Terms

Additional Notes

Related interactions

Curated By