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Electrostatic Map Of Proteasome α-Rings Encodes The Design of Allosteric Porphyrin-Based Inhibitors Able To Affect 20S Conformation By Cooperative Binding

机译:蛋白酶体α环的静电图编码能够通过协同结合影响20S构象的变构卟啉基抑制剂的设计

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The importance of allosteric proteasome inhibition in the treatment of cancer is becoming increasingly evident. Motivated by this urgent therapeutic need, we have recently identified cationic porphyrins as a highly versatile class of molecules able to regulate proteasome activity by interfering with gating mechanisms. In the present study, the mapping of electrostatic contacts bridging the regulatory particles with the α-rings of the human 20S proteasome led us to the identification of (meso-tetrakis(4-N-methylphenyl pyridyl)-porphyrin (pTMPyPP4) as a novel non-competitive inhibitor of human 20S proteasome. pTMPyPP4 inhibition mechanism implies a positive cooperative binding to proteasome, which disappears when a permanently open proteasome mutant (α-3ΔN) is used, supporting the hypothesis that the events associated with allosteric proteasome inhibition by pTMPyPP4 interfere with 20S gating and affect its “open-closed” equilibrium. Therefore, we propose that the spatial distribution of the negatively charged residues responsible for the interaction with regulatory particles at the α-ring surface of human 20S may be exploited as a blueprint for the design of allosteric proteasome regulators.
机译:变构蛋白酶体抑制在癌症治疗中的重要性越来越明显。出于这种迫切的治疗需求,我们最近确定了阳离子卟啉是一类高度通用的分子,能够通过干扰门控机制来调节蛋白酶体的活性。在本研究中,将调节颗粒与人类20S蛋白酶体的α环桥接的静电接触的映射导致我们鉴定了(间-四(4-N-甲基苯基吡啶基)-卟啉(pTMPyPP4) pTMPyPP4的非竞争性抑制剂,pTMPyPP4抑制机制暗示与蛋白酶体的正协同结合,当使用永久开放的蛋白酶体突变体(α-3ΔN)时消失,支持这一假设,即与pTMPyPP4抑制变构蛋白酶体有关的事件会干扰20S门控并影响其“开闭”平衡,因此,我们建议将负责与20S人α环表面上的调控粒子相互作用的带负电荷的残基的空间分布作为蓝图。变构蛋白酶体调节剂的设计。

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