Protein tyrosine phosphatase inactivation by electrophilic tyrosine modification

Abstract

Covalent protein tyrosine phosphatase (PTP) inhibitors principally target the catalytic cysteine, which is highly conserved and presents challenges for achieving selectivity across the PTP family. Here, we identified a tyrosine-reactive covalent inhibitor for SHP2 (DML189) with secondary molecular glue activity via a ligand induced protein tethering (LIPT) mechanism. We detected ligand binding at Y279, which is in proximity to the catalytic cysteine on SHP2 and has known functional and pathogenic properties. Covalent SHP2 modification by DML189 induced reversible disulfide tethering and monomer loss that was not observed to the same extent on PTP1B, LYP, or SHP1. Crosslinking mass spectrometry detected unique tethering events involving regulatory cysteines after DML189 modification on SHP2. Together, we discovered a tyrosine reactive inhibitor that targets functional sites on SHP2 and exhibits molecular glue activity through LIPT.

Graphical abstract: Protein tyrosine phosphatase inactivation by electrophilic tyrosine modification

Supplementary files

Article information

Article type
Edge Article
Submitted
23 Sep 2025
Accepted
09 Jan 2026
First published
19 Jan 2026
This article is Open Access

All publication charges for this article have been paid for by the Royal Society of Chemistry
Creative Commons BY license

Chem. Sci., 2026, Advance Article

Protein tyrosine phosphatase inactivation by electrophilic tyrosine modification

M. L. Ware, D. M. Leace, Z. Qu, Q. Schaefer, S. D. Vaidya, M. L. Horvath, Z. Li, Y. Bai, Z. Zhang and K. Hsu, Chem. Sci., 2026, Advance Article , DOI: 10.1039/D5SC07398G

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