An in vitro platform for the enzymatic characterization of the rhomboid protease RHBDL4.

IF 4 2区生物学 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY Journal of Biological Chemistry Pub Date : 2025-03-01 Epub Date: 2025-02-07 DOI:10.1016/j.jbc.2025.108275

Satarupa Bhaduri, Mac Kevin E Braza, Stancho Stanchev, Marina Tauber, Raghad Al-Bawab, Lawrence J Liu, Diego F Trujillo, Kristina Solorio-Kirpichyan, Ambuj Srivastava, Javier Sanlley-Hernandez, Anthony J O'Donoghue, Marius K Lemberg, Rommie Amaro, Kvido Strisovsky, Sonya E Neal

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Abstract

Rhomboid proteases are ubiquitous intramembrane serine proteases that can cleave transmembrane substrates within lipid bilayers. They exhibit many and diverse functions, such as but not limited to, growth factor signaling, immune and inflammatory response, protein quality control, and parasitic invasion. Human rhomboid protease RHBDL4 has been demonstrated to play a critical role in removing misfolded proteins from the endoplasmic reticulum and is implicated in severe diseases such as various cancers and Alzheimer's disease. Therefore, RHBDL4 is expected to constitute an important therapeutic target for such devastating diseases. Despite its critical role in many biological processes, the enzymatic properties of RHBDL4 remain largely unknown. To enable a comprehensive characterization of RHBDL4's kinetics, catalytic parameters, substrate specificity, and binding modality, we expressed and purified recombinant RHBDL4 and employed it in a Förster resonance energy transfer-based cleavage assay. Until now, kinetic studies have been limited mostly to bacterial rhomboid proteases. Our in vitro platform offers a new method for studying RHBDL4's enzymatic function and substrate preferences. Furthermore, we developed and tested potential inhibitors using our assay and successfully identified peptidyl α-ketoamide inhibitors of RHBDL4 that are highly effective against recombinant RHBDL4. We utilize ensemble docking and molecular dynamics simulations to explore the binding modality of substrate-derived peptides bound to RHBDL4. Our analysis focused on key interactions and dynamic movements within RHBDL4's active site that contributed to binding stability, offering valuable insights for optimizing the nonprime side of RHBDL4 ketoamide inhibitors. In summary, our study offers fundamental insights into RHBDL4's catalytic activities and substrate preferences, laying the foundation for downstream applications such as drug inhibitor screenings and structure-function studies, which will enable the identification of lead drug compounds for RHBDL4.

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菱形蛋白酶RHBDL4酶学表征的体外平台。

菱形蛋白酶是普遍存在的膜内丝氨酸蛋白酶，可以在脂质双层内切割跨膜底物。它们具有多种功能，如但不限于生长因子信号、免疫和炎症反应、蛋白质质量控制和寄生虫入侵。人类菱形蛋白酶RHBDL4已被证明在去除内质网错误折叠蛋白方面发挥关键作用，并与各种癌症和阿尔茨海默病等严重疾病有关。因此，RHBDL4有望成为这类毁灭性疾病的重要治疗靶点。尽管RHBDL4在许多生物过程中起着至关重要的作用，但其酶学特性在很大程度上仍然未知。为了全面表征RHBDL4的动力学、催化参数、底物特异性和结合方式，我们表达并纯化了重组RHBDL4，并将其用于Förster共振能量转移裂解实验。到目前为止，动力学研究主要局限于细菌菱形蛋白酶。我们的体外平台为研究RHBDL4的酶功能和底物偏好提供了一种新的方法。此外，我们利用我们的实验开发和测试了潜在的抑制剂，并成功鉴定了RHBDL4的肽基α-酮酰胺抑制剂，这些抑制剂对重组RHBDL4非常有效。我们利用集合对接和分子动力学（MD）模拟来探索底物衍生肽与RHBDL4的结合方式。我们的分析集中在RHBDL4活性位点的关键相互作用和动态运动，这些作用有助于结合稳定性，为优化RHBDL4酮酰胺抑制剂的非主要方面提供有价值的见解。总之，我们的研究为RHBDL4的催化活性和底物偏好提供了基本的见解，为下游应用如药物抑制剂筛选和结构-功能研究奠定了基础，这将使RHBDL4的先导药物化合物的鉴定成为可能。

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来源期刊

Journal of Biological Chemistry Biochemistry, Genetics and Molecular Biology-Biochemistry

自引率

4.20%

发文量

1233

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