Degradome analysis to identify direct protein substrates of small-molecule degraders.

Cell Chem Biol

German Cancer Research Center (DKFZ), Heidelberg, Germany; Heidelberg University, Medical Faculty, Heidelberg, Germany. Electronic address:

Published: November 2024

AI Article Synopsis

  • - Targeted protein degradation (TPD) is a new method for selectively eliminating difficult-to-target proteins using small molecules, offering new therapeutic possibilities.
  • - One major challenge is to clearly identify the primary targets of TPD, separate from secondary effects that occur elsewhere in the cell's protein landscape.
  • - The researchers developed a mass spectrometry technique called DegMS that effectively analyzes protein degradation while controlling for changes in transcription and translation, demonstrated by studying various protein degraders and identifying FIZ1 as a target.

Article Abstract

Targeted protein degradation (TPD) has emerged as a powerful strategy to selectively eliminate cellular proteins using small-molecule degraders, offering therapeutic promise for targeting proteins that are otherwise undruggable. However, a remaining challenge is to unambiguously identify primary TPD targets that are distinct from secondary downstream effects in the proteome. Here we introduce an approach for selective analysis of protein degradation by mass spectrometry (DegMS) at proteomic scale, which derives its specificity from the exclusion of confounding effects of altered transcription and translation induced by target depletion. We show that the approach efficiently operates at the timescale of TPD (hours) and we demonstrate its utility by analyzing the cyclin K degraders dCeMM2 and dCeMM4, which induce widespread transcriptional downregulation, and the GSPT1 degrader CC-885, an inhibitor of protein translation. Additionally, we apply DegMS to characterize a previously uncharacterized degrader, and identify the zinc-finger protein FIZ1 as a degraded target.

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Source
http://dx.doi.org/10.1016/j.chembiol.2024.10.007DOI Listing

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