DPP8/9 processing of human AK2 unmasks an IAP binding motif.

IF 6.5 1区生物学 Q1 BIOCHEMISTRY & MOLECULAR BIOLOGY

EMBO Reports Pub Date : 2025-05-01 DOI:10.1038/s44319-025-00455-z

Kim J Lapacz, Konstantin Weiss, Franziska Mueller, Yuxing Xue, Simon Poepsel, Matthias Weith, Tanja Bange, Jan Riemer

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引用次数: 0

Abstract

Adenylate kinase 2 (AK2) is localized in the intermembrane space of mitochondria, where it ensures efficient adenine nucleotide exchange between cytosol and mitochondria. For mitochondrial import, AK2 relies on the MIA40 disulphide relay system. Its cytosolic stability is subject to regulation through N-terminal processing by the dipeptidyl peptidases DPP8 and DPP9, which sensitize AK2 for proteasomal degradation. Here, we find that cytosolic AK2 degradation is mediated by Inhibitors of Apoptosis (IAPs), a class of E3 ligases that interacts with target proteins by binding to IAP-binding motifs (IBM). We have identified an IBM at the very end of AK2's novel N-terminus, which becomes exposed due to processing by DPP8/9. N-terminal acetylation mediated by the N-acetyltransferase NatA prevents this AK2-IAP interaction, therefore stabilizing AK2 in the cytosol. Performing a genome-wide in silico screen, we could identify 129 potential substrates in which an IBM becomes potentially unmasked by DPP8/9 processing. For one of these potential substrates, EIF2A, we demonstrate its targeting to IAPs after IBM exposure by DPP8/9 indicating that DPP8/9-mediated unmasking of IBMs is a general phenomenon.

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DPP8/9处理人类AK2揭示了IAP结合基序。

腺苷酸激酶2 （Adenylate kinase 2, AK2）定位于线粒体的膜间空间，确保细胞质和线粒体之间有效的腺嘌呤核苷酸交换。对于线粒体进口，AK2依赖于MIA40二硫化物接力系统。其胞质稳定性受二肽基肽酶DPP8和DPP9的n端加工调控，使AK2对蛋白酶体降解敏感。在这里，我们发现胞质内AK2降解是由凋亡抑制剂（IAPs）介导的，IAPs是一类E3连接酶，通过结合iap结合基序与靶蛋白相互作用（IBM）。我们已经在AK2的新n末端发现了一个IBM，它由于DPP8/9的处理而暴露。n -乙酰转移酶NatA介导的n端乙酰化阻止了AK2- iap相互作用，从而稳定了胞浆中的AK2。在硅屏幕上执行全基因组，我们可以确定129个潜在的底物，其中IBM通过DPP8/9处理可能被揭示。对于其中一种潜在的底物EIF2A，我们证明了它在DPP8/9暴露IBM后靶向iap，这表明DPP8/9介导的IBM的揭露是一种普遍现象。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

EMBO Reports 生物-生化与分子生物学

CiteScore

11.20

自引率

1.30%

发文量

267

审稿时长

1 months

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