BAIT

RPT3

YNT1, YTA2, proteasome regulatory particle base subunit RPT3, L000002556, L000002537, YDR394W

ATPase of the 19S regulatory particle of the 26S proteasome; one of ATPases of the regulatory particle; involved in the degradation of ubiquitinated substrates; substrate of N-acetyltransferase B

UPS Project

GO Process (3)

GO Function (1)

GO Component (1)

Gene Ontology Biological Process

positive regulation of RNA polymerase II transcriptional preinitiation complex assembly [IMP]

proteasome regulatory particle assembly [IMP]

ubiquitin-dependent protein catabolic process [IMP]

Gene Ontology Molecular Function

ATPase activity [ISS]

Gene Ontology Cellular Component

proteasome regulatory particle, base subcomplex [IDA]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

PREY

RPN2

SEN3, proteasome regulatory particle base subunit RPN2, L000001864, YIL075C

Subunit of the 26S proteasome; substrate of the N-acetyltransferase Nat1p; protein abundance increases in response to DNA replication stress

UPS Project

GO Process (2)

GO Function (2)

GO Component (3)

Gene Ontology Biological Process

proteasome assembly [IGI]

ubiquitin-dependent protein catabolic process [IMP, IPI]

Gene Ontology Molecular Function

endopeptidase activity [IMP]
protein binding, bridging [IPI]

Gene Ontology Cellular Component

nucleus [IDA]

proteasome regulatory particle, base subcomplex [IDA]

proteasome storage granule [IDA]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

Affinity Capture-MS

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 is identified by mass spectrometric methods.

Publication

The penultimate step of proteasomal ATPase assembly is mediated by a switch dependent on the chaperone Nas2.

Sekaran S, Park S

The proteasome holoenzyme is a complex molecular machine that degrades most proteins. In the proteasome holoenzyme, six distinct ATPase subunits (Rpt1 through Rpt6) enable protein degradation by injecting protein substrates into it. Individual Rpt subunits assemble into a heterohexameric "Rpt ring" in a stepwise manner, by binding to their cognate chaperones. Completion of the heterohexameric Rpt ring correlates with release ... [more]

J Biol Chem Feb. 01, 2023; 299(2);102870 [Pubmed: 36621624]

Throughput

Low Throughput

Related interactions

Interaction	Experimental Evidence Code	Dataset	Throughput	Score	Curated By	Notes
RPN2 RPT3	Affinity Capture-MS Affinity Capture-MS 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 is identified by mass spectrometric methods.	Babu M (2012)	High	-	BioGRID	694339
RPN2 RPT3	Affinity Capture-MS Affinity Capture-MS 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 is identified by mass spectrometric methods.	Krogan NJ (2006)	High	-	BioGRID	-
RPT3 RPN2	Affinity Capture-MS Affinity Capture-MS 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 is identified by mass spectrometric methods.	Michaelis AC (2023)	High	6	BioGRID	3612796
RPN2 RPT3	Co-crystal Structure Co-crystal Structure Interaction directly demonstrated at the atomic level by X-ray crystallography. Also used for NMR or Electron Microscopy (EM) structures. If there is no obvious bait-hit directionality to the interaction involving 3 or more proteins, then the co-crystallized proteins should be listed as a complex.	Lander GC (2012)	Low	-	BioGRID	-
RPN2 RPT3	Cross-Linking-MS (XL-MS) Cross-Linking-MS (XL-MS) An interaction is detected between two proteins using chemically reactive or photo-activatable cross-linking reagents that covalently link amino acids in close proximity, followed by mass spectrometry analysis to identify the linked peptides (reviewed in PMID 37406423, 37104977). Experiments may be carried with live cells or cell lysates in which all proteins are expressed at endogenous levels (e.g. PMID 34349018, 35235311) or with recombinant proteins (e.g., PMID 28537071).	Mintseris J (2020)	Low	-	BioGRID	3730225
RPN2 RPT3	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.	Breslow DK (2008)	High	-0.011	BioGRID	442993
RPT3 RPN2	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.	Breslow DK (2008)	High	-0.011	BioGRID	442994
RPT3 RPN2	Reconstituted Complex Reconstituted Complex An interaction is detected between purified proteins in vitro.	Bashore C (2015)	Low	-	BioGRID	-

Curated By

BioGRID

Interaction Summary

RPT3

Gene Ontology Biological Process

Gene Ontology Molecular Function

ATPase activity [ISS]

Gene Ontology Cellular Component

RPN2

Gene Ontology Biological Process

Gene Ontology Molecular Function

endopeptidase activity [IMP]protein binding, bridging [IPI]

Gene Ontology Cellular Component

Affinity Capture-MS

Publication

The penultimate step of proteasomal ATPase assembly is mediated by a switch dependent on the chaperone Nas2.

Throughput

Related interactions

Curated By

endopeptidase activity [IMP]
protein binding, bridging [IPI]