Multiparameter screen optimizes immunoprecipitation

Biotechniques. 2024 Apr;76(4):145-152. doi: 10.2144/btn-2023-0051. Epub 2024 Feb 29.

Abstract

Immunoprecipitation (IP) coupled with mass spectrometry effectively maps protein-protein interactions when genome-wide, affinity-tagged cell collections are used. Such studies have recorded significant portions of the compositions of physiological protein complexes, providing draft 'interactomes'; yet many constituents of protein complexes still remain uncharted. This gap exists partly because high-throughput approaches cannot optimize each IP. A key challenge for IP optimization is stabilizing in vivo interactions during the transfer from cells to test tubes; failure to do so leads to the loss of genuine interactions during the IP and subsequent failure to detect. Our high-content screening method explores the relationship between in vitro chemical conditions and IP outcomes, enabling rapid empirical optimization of conditions for capturing target macromolecular assemblies.

Keywords: affinity proteomics; complexomics; interactomics; macromolecular assemblies.

MeSH terms

  • Immunoprecipitation
  • Mass Spectrometry* / methods