BAIT

NAP1

histone chaperone NAP1, L000001232, YKR048C

Histone chaperone; involved in histone exchange by removing and replacing histone H2A-H2B dimers or histone variant dimers from assembled nucleosomes; involved in the transport of H2A and H2B histones to the nucleus; required for the regulation of microtubule dynamics during mitosis; interacts with mitotic cyclin Clb2p; controls bud morphogenesis; phosphorylated by CK2; protein abundance increases in response to DNA replication stress

GO Process (7)

GO Function (3)

GO Component (2)

Gene Ontology Biological Process

budding cell bud growth [IGI, IMP]

nucleosome assembly [IDA, ISS]

nucleosome disassembly [IDA]

positive regulation of catalytic activity [IDA]

positive regulation of microtubule polymerization [IMP]

positive regulation of transcription elongation from RNA polymerase II promoter [IDA]

protein import into nucleus [IMP]

Gene Ontology Molecular Function

cyclin binding [IPI]
enzyme activator activity [IDA]
histone binding [IDA]

Gene Ontology Cellular Component

cytoplasm [IDA]

nucleus [IPI]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

PREY

NBP2

L000002861, YDR162C

Protein involved in the HOG (high osmolarity glycerol) pathway; negatively regulates Hog1p by recruitment of phosphatase Ptc1p the Pbs2p-Hog1p complex; interacts with Bck1p and down regulates the cell wall integrity pathway; found in the nucleus and cytoplasm, contains an SH3 domain and a Ptc1p binding domain (PBM)

GO Process (4)

GO Function (0)

GO Component (2)

Gene Ontology Biological Process

hyperosmotic response [IMP, IPI]

inactivation of MAPK activity involved in cell wall organization or biogenesis [IMP, IPI]

negative regulation of protein kinase activity [IDA]

response to heat [IMP]

Gene Ontology Cellular Component

cytoplasm [IDA]

nucleus [IDA]

SGD Alliance of Genome Resources Entrez Gene RefSeq UniprotKB

Saccharomyces cerevisiae (S288c)

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.

Publication

Systematic analysis of complex genetic interactions.

Kuzmin E, VanderSluis B, Wang W, Tan G, Deshpande R, Chen Y, Usaj M, Balint A, Mattiazzi Usaj M, van Leeuwen J, Koch EN, Pons C, Dagilis AJ, Pryszlak M, Wang JZY, Hanchard J, Riggi M, Xu K, Heydari H, San Luis BJ, Shuteriqi E, Zhu H, Van Dyk N, Sharifpoor S, Costanzo M, Loewith R, Caudy A, Bolnick D, Brown GW, Andrews BJ, Boone C, Myers CL

To systematically explore complex genetic interactions, we constructed ~200,000 yeast triple mutants and scored negative trigenic interactions. We selected double-mutant query genes across a broad spectrum of biological processes, spanning a range of quantitative features of the global digenic interaction network and tested for a genetic interaction with a third mutation. Trigenic interactions often occurred among functionally related genes, and ... [more]

Science Apr. 20, 2018; 360(6386); [Pubmed: 29674565]

Quantitative Score

-0.196986 [Confidence Score]

Throughput

High Throughput

Ontology Terms

colony size (APO:0000063)

Additional Notes

Digenic interaction: Query allele name: ho-delta+nap1-delta; Array allele name: nbp2-delta (GI score = -0.196986, p-value = 0.0347; Digenic)
Digenic interactions in this Synthetic genetic array (SGA) analysis were considered to be significant when epsilon > 0.08 and p < 0.05 (positive genetic interaction) and when epsilon < -0.08 and p < 0.05 (negative genetic interaction).

Related interactions

Interaction	Experimental Evidence Code	Dataset	Throughput	Score	Curated By	Notes
NAP1 NBP2	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.	Hruby A (2011)	High	-	BioGRID	485999
NBP2 NAP1	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.	Tarassov K (2008)	High	-	BioGRID	-
NBP2 NAP1	Synthetic Growth Defect Synthetic Growth Defect A genetic interaction is inferred when mutations in separate genes, each of which alone causes a minimal phenotype, result in a significant growth defect under a given condition when combined in the same cell.	Ohkuni K (2003)	Low	-	BioGRID	160802
NAP1 NBP2	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.	Ohkuni K (2003)	Low	-	BioGRID	-

Curated By

BioGRID

Interaction Summary

NAP1

Gene Ontology Biological Process

Gene Ontology Molecular Function

cyclin binding [IPI]enzyme activator activity [IDA]histone binding [IDA]

Gene Ontology Cellular Component

NBP2

Gene Ontology Biological Process

Gene Ontology Cellular Component

Negative Genetic

Publication

Systematic analysis of complex genetic interactions.

Quantitative Score

Throughput

Ontology Terms

Additional Notes

Related interactions

Curated By

cyclin binding [IPI]
enzyme activator activity [IDA]
histone binding [IDA]