An in-cell approach to evaluate E3 ligases for use in targeted protein degradation.

降级(电信) 蛋白质降解 泛素 计算机科学 细胞生物学 计算生物学 化学 业务 生物 生物化学 电信 基因
作者
Yunan Zheng,Anamika Singh,Zeqi Niu,Violeta L. Marin,Jennifer A. Young,Paul L. Richardson,Marcus L. Hemshorn,Richard B. Cooley,P. Andrew Karplus,Scott E. Warder,Anil Vasudevan,Justin M. Reitsma,Ryan A. Mehl
标识
DOI:10.1101/2024.12.19.629291
摘要

Abstract One of the major challenges in evaluating the suitability of potential ∼700 E3 ligases for target protein degradation (TPD) is the lack of binders specific to each E3 ligase. Here we apply genetic code expansion (GCE) to encode a tetrazine-containing non-canonical amino acid (Tet-ncAA) site-specifically into the E3 ligase, which can be conjugated with strained trans-cyclooctene (sTCO) tethered to a neo-substrate protein binder by click chemistry within living cells. The resulting E3 ligase minimally modified and functionalized in an E3-ligand free (ELF) manner, can be evaluated for TPD of the neo-substrate. We demonstrate that CRBN encoded with clickable Tet-ncAA, either in the known immunomodulatory drug (IMiD)-binding pocket or across surface, can be covalently tethered to sTCO-linker-JQ1 and recruit BRD2/4 for CRBN mediated degradation, indicating the high plasticity of CRBN for TPD. The degradation efficiency is dependent on location of the Tet-ncAA encoding on CRBN as well as the length of the linker, showing the capability of this approach to map the surface of E3 ligase for identifying optimal TPD pockets. This ELF-degrader approach has the advantages of not only maintaining the native state of E3 ligase, but also allowing the interrogation of E3 ligases and target protein partners under intracellular conditions and can be applied to any known E3 ligase.

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