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与常染色体隐性帕金森病相关的人类DJ-1/PARK7 L166P蛋白稳定性降低,是由于蛋白酶体直接进行内蛋白水解切割所致。

Reduced protein stability of human DJ-1/PARK7 L166P, linked to autosomal recessive Parkinson disease, is due to direct endoproteolytic cleavage by the proteasome.

作者信息

Alvarez-Castelao Beatriz, Muñoz Carolina, Sánchez Isabel, Goethals Marc, Vandekerckhove Joël, Castaño José G

机构信息

Departamento de Bioquímica, Instituto de Investigaciones Biomédicas Alberto Sols, UAM-CSIC, Madrid, Spain.

出版信息

Biochim Biophys Acta. 2012 Feb;1823(2):524-33. doi: 10.1016/j.bbamcr.2011.11.010. Epub 2011 Dec 8.

Abstract

Parkinson's disease (PD) is characterized by dopaminergic dysfunction and degeneration. DJ-1/PARK7 mutations have been linked with a familial form of early onset PD. In this study, we found that human DJ-1 wild type and the missense mutants M26I, R98Q, A104T and D149A were stable proteins in cells, only the L166P mutant was unstable. In parallel, the former were not degraded and the L166P mutant was directly degraded in vitro by proteasome-mediated endoproteolytic cleavage. Furthermore, genetic evidence in fission yeast showed the direct involvement of proteasome in the degradation of human DJ-1 L166P and the corresponding L169P mutant of SPAC22E12.03c, the human orthologue of DJ-1 in Schizosaccharomyces Pombe, as their protein levels were increased at restrictive temperature in fission yeast (mts4 and pts1-732) harboring temperature sensitive mutations in proteasomal subunits. In total, our results provide evidence that direct proteasomal endoproteolytic cleavage of DJ-1 L166P is the mechanism of degradation contributing to the loss-of-function of the mutant protein, a property not shared by other DJ-1 missense mutants associated with PD.

摘要

帕金森病(PD)的特征是多巴胺能功能障碍和变性。DJ-1/PARK7突变与家族性早发性PD有关。在本研究中,我们发现人类DJ-1野生型以及错义突变体M26I、R98Q、A104T和D149A在细胞中是稳定的蛋白质,只有L166P突变体不稳定。同时,前者不会被降解,而L166P突变体在体外通过蛋白酶体介导的内蛋白水解切割直接被降解。此外,裂殖酵母中的遗传学证据表明,蛋白酶体直接参与了人类DJ-1 L166P以及SPAC22E12.03c(裂殖酵母中DJ-1的人类同源物)相应的L169P突变体的降解,因为在蛋白酶体亚基中携带温度敏感突变的裂殖酵母(mts4和pts1-732)中,它们的蛋白质水平在限制温度下会升高。总之,我们的结果提供了证据,即DJ-1 L166P的直接蛋白酶体内蛋白水解切割是导致突变蛋白功能丧失的降解机制,这一特性并非与PD相关的其他DJ-1错义突变体所共有。

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