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一种新型溶组织内阿米巴半胱氨酸蛋白酶EhCP4,是侵袭性阿米巴病的关键因素及治疗靶点。

A novel Entamoeba histolytica cysteine proteinase, EhCP4, is key for invasive amebiasis and a therapeutic target.

作者信息

He Chen, Nora George P, Schneider Eric L, Kerr Iain D, Hansell Elizabeth, Hirata Ken, Gonzalez David, Sajid Mohammed, Boyd Sarah E, Hruz Petr, Cobo Eduardo R, Le Christine, Liu Wei-Ting, Eckmann Lars, Dorrestein Pieter C, Houpt Eric R, Brinen Linda S, Craik Charles S, Roush William R, McKerrow James, Reed Sharon L

机构信息

Department of Pathology and Medicine, University of California, San Diego, California 92103-8416, USA.

出版信息

J Biol Chem. 2010 Jun 11;285(24):18516-27. doi: 10.1074/jbc.M109.086181. Epub 2010 Apr 8.

Abstract

Entamoeba histolytica cysteine proteinases (EhCPs) play a key role in disrupting the colonic epithelial barrier and the innate host immune response during invasion of E. histolytica, the protozoan cause of human amebiasis. EhCPs are encoded by 50 genes, of which ehcp4 (ehcp-a4) is the most up-regulated during invasion and colonization in a mouse cecal model of amebiasis. Up-regulation of ehcp4 in vivo correlated with our finding that co-culture of E. histolytica trophozoites with mucin-producing T84 cells increased ehcp4 expression up to 6-fold. We have expressed recombinant EhCP4, which was autocatalytically activated at acidic pH but had highest proteolytic activity at neutral pH. In contrast to the other amebic cysteine proteinases characterized so far, which have a preference for arginine in the P2 position, EhCP4 displayed a unique preference for valine and isoleucine at P2. This preference was confirmed by homology modeling, which revealed a shallow, hydrophobic S2 pocket. Endogenous EhCP4 localized to cytoplasmic vesicles, the nuclear region, and perinuclear endoplasmic reticulum (ER). Following co-culture with colonic cells, EhCP4 appeared in acidic vesicles and was released extracellularly. A specific vinyl sulfone inhibitor, WRR605, synthesized based on the substrate specificity of EhCP4, inhibited the recombinant enzyme in vitro and significantly reduced parasite burden and inflammation in the mouse cecal model. The unique expression pattern, localization, and biochemical properties of EhCP4 could be exploited as a potential target for drug design.

摘要

溶组织内阿米巴半胱氨酸蛋白酶(EhCPs)在溶组织内阿米巴(人类阿米巴病的原生动物病原体)入侵过程中破坏结肠上皮屏障和宿主固有免疫反应方面发挥关键作用。EhCPs由50个基因编码,其中ehcp4(ehcp-a4)在阿米巴病小鼠盲肠模型的入侵和定植过程中上调最为明显。ehcp4在体内的上调与我们的发现相关,即溶组织内阿米巴滋养体与产生粘蛋白的T84细胞共培养可使ehcp4表达增加高达6倍。我们表达了重组EhCP4,其在酸性pH下自动催化激活,但在中性pH下具有最高的蛋白水解活性。与迄今为止所表征的其他阿米巴半胱氨酸蛋白酶不同,后者在P2位置偏好精氨酸,而EhCP4在P2位置对缬氨酸和异亮氨酸表现出独特的偏好。通过同源建模证实了这种偏好,该模型揭示了一个浅的疏水S2口袋。内源性EhCP4定位于细胞质囊泡、核区域和核周内质网(ER)。与结肠细胞共培养后,EhCP4出现在酸性囊泡中并释放到细胞外。基于EhCP4的底物特异性合成的一种特异性乙烯砜抑制剂WRR605在体外抑制了重组酶,并显著降低了小鼠盲肠模型中的寄生虫负荷和炎症。EhCP4独特的表达模式、定位和生化特性可被用作药物设计的潜在靶点。

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