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信号肽酶样 2b(SPPL2b)体外切割肿瘤坏死因子 α(TNFα)类似于细胞内观察到的机制原理。

In vitro cleavage of tumor necrosis factor α (TNFα) by Signal-Peptide-Peptidase-like 2b (SPPL2b) resembles mechanistic principles observed in the cellular context.

机构信息

Biochemistry and Molecular Biology, Institute of Theoretical Medicine, Faculty of Medicine, University of Augsburg, Universitätsstrasse 2, D-86159, Augsburg, Germany.

Biochemistry and Molecular Biology, Institute of Theoretical Medicine, Faculty of Medicine, University of Augsburg, Universitätsstrasse 2, D-86159, Augsburg, Germany; Institut für Entwicklungsbiologie und Neurobiologie, Johannes Gutenberg-Universität Mainz, Hanns-Dieter-Hüsch-Weg 15, 55099, Mainz, Germany.

出版信息

Chem Biol Interact. 2024 May 25;395:111006. doi: 10.1016/j.cbi.2024.111006. Epub 2024 Apr 16.

DOI:10.1016/j.cbi.2024.111006
PMID:38636792
Abstract

Members of the Signal Peptide-Peptidase (SPP) and Signal Peptide-Peptidase-like (SPPL) family are intramembrane aspartyl-proteases like their well-studied homologs, the presenilins, which comprise the catalytically active subunit within the γ-secretase complex. The lack of in vitro cleavage assays for SPPL proteases limited their biochemical characterization as well as substrate identification and validation. So far, SPPL proteases have been analyzed exclusively in intact cells or membranes, restricting mechanistic analysis to co-expression of enzyme and substrate variants colocalizing in the same subcellular compartments. We describe the details of developing an in vitro cleavage assay for SPPL2b and its model substrate TNFα and analyzed the influence of phospholipids, detergent supplements, and cholesterol on the SPPL2b in vitro activity. SPPL2b in vitro activity resembles mechanistic principles that have been observed in a cellular context, such as cleavage sites and consecutive turnover of the TNFα transmembrane domain. The novel in vitro cleavage assay is functional with separately isolated protease and substrate and amenable to a high throughput plate-based readout overcoming previous limitations and providing the basis for studying enzyme kinetics, catalytic activity, substrate recognition, and the characteristics of small molecule inhibitors. As a proof of concept, we present the first biochemical in vitro characterization of the SPPL2a and SPPL2b specific small molecule inhibitor SPL-707.

摘要

信号肽肽酶(SPP)和信号肽肽酶样(SPPL)家族的成员是跨膜天冬氨酸蛋白酶,与研究较为充分的同源物早老素一样,它们构成了 γ-分泌酶复合物中的催化活性亚基。缺乏针对 SPPL 蛋白酶的体外切割测定限制了它们的生化特征分析,以及底物的鉴定和验证。到目前为止,SPPL 蛋白酶仅在完整细胞或膜中进行分析,将酶和底物变体的共表达限制在相同的亚细胞隔室中,从而限制了对机制的分析。我们描述了开发 SPPL2b 及其模型底物 TNFα 的体外切割测定的详细信息,并分析了磷脂、去污剂补充剂和胆固醇对 SPPL2b 体外活性的影响。SPPL2b 的体外活性类似于在细胞环境中观察到的机制原则,例如切割位点和 TNFα 跨膜结构域的连续周转。新型的体外切割测定与分离的蛋白酶和底物一起具有功能,并且适用于高通量基于平板的读出,克服了以前的限制,并为研究酶动力学、催化活性、底物识别和小分子抑制剂的特性提供了基础。作为概念验证,我们首次对 SPPL2a 和 SPPL2b 特异性小分子抑制剂 SPL-707 进行了生化体外表征。

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