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

Quantitative interaction proteomics and genome-wide profiling of epigenetic histone marks and their readers.

Vermeulen M, Eberl HC, Matarese F, Marks H, Denissov S, Butter F, Lee KK, Olsen JV, Hyman AA, Stunnenberg HG, Mann M

Trimethyl-lysine (me3) modifications on histones are the most stable epigenetic marks and they control chromatin-mediated regulation of gene expression. Here, we determine proteins that bind these marks by high-accuracy, quantitative mass spectrometry. These chromatin "readers" are assigned to complexes by interaction proteomics of full-length BAC-GFP-tagged proteins. ChIP-Seq profiling identifies their genomic binding sites, revealing functional properties. Among the main findings, ... [more]

Cell Sep. 17, 2010; 142(6);967-80 [Pubmed: 20850016]

Throughput

High Throughput

Curated By

BioGRID

Interaction Summary

C17ORF49

Gene Ontology Cellular Component

LMNA

Gene Ontology Biological Process

Gene Ontology Molecular Function

protein binding [IPI]
structural molecule activity [TAS]

Gene Ontology Cellular Component

Affinity Capture-MS

Publication

Quantitative interaction proteomics and genome-wide profiling of epigenetic histone marks and their readers.

Throughput

Curated By

Interaction Summary

C17ORF49

Gene Ontology Cellular Component

LMNA

Gene Ontology Biological Process

Gene Ontology Molecular Function

protein binding [IPI]structural molecule activity [TAS]

Gene Ontology Cellular Component

Affinity Capture-MS

Publication

Quantitative interaction proteomics and genome-wide profiling of epigenetic histone marks and their readers.

Throughput

Curated By

protein binding [IPI]
structural molecule activity [TAS]