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Acylation of MLKL Impacts Its Function in Necroptosis

坏死性下垂 磷酸化 酰化 激酶 生物 化学 生物物理学 细胞生物学 生物化学 程序性细胞死亡 细胞凋亡 催化作用
作者
Apoorva J. Pradhan,Shweta Chitkara,Ricardo X. Ramirez,Viviana Monje‐Galvan,Yasemin Sancak,G. Ekin Atilla‐Gokcumen
出处
期刊:ACS Chemical Biology [American Chemical Society]
卷期号:19 (2): 407-418 被引量:4
标识
DOI:10.1021/acschembio.3c00603
摘要

Mixed lineage kinase domain-like (MLKL) is a key signaling protein of necroptosis. Upon activation by phosphorylation, MLKL translocates to the plasma membrane and induces membrane permeabilization, which contributes to the necroptosis-associated inflammation. Membrane binding of MLKL is initially initiated by electrostatic interactions between the protein and membrane phospholipids. We previously showed that MLKL and its phosphorylated form (pMLKL) are S-acylated during necroptosis. Here, we characterize the acylation sites of MLKL and identify multiple cysteines that can undergo acylation with an interesting promiscuity at play. Our results show that MLKL and pMLKL undergo acylation at a single cysteine, with C184, C269, and C286 as possible acylation sites. Using all-atom molecular dynamic simulations, we identify differences that the acylation of MLKL causes at the protein and membrane levels. Through investigations of the S-palmitoyltransferases that might acylate pMLKL in necroptosis, we showed that zDHHC21 activity has the strongest effect on pMLKL acylation, inactivation of which profoundly reduced the pMLKL levels in cells and improved membrane integrity. These results suggest that blocking the acylation of pMLKL destabilizes the protein at the membrane interface and causes its degradation, ameliorating the necroptotic activity. At a broader level, our findings shed light on the effect of S-acylation on MLKL functioning in necroptosis and MLKL-membrane interactions mediated by its acylation.

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