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抗锑和抗米替福新的线粒体蛋白质组学

Mitochondrial Proteomics of Antimony and Miltefosine Resistant .

作者信息

Vincent Isabel M, Racine Gina, Légaré Danielle, Ouellette Marc

机构信息

Centre de Recherche en Infectiologie du CHU de Québec, Université Laval, Québec City, QC G1V 4G2, Canada.

出版信息

Proteomes. 2015 Oct 21;3(4):328-346. doi: 10.3390/proteomes3040328.

Abstract

Antimony (SbIII) and miltefosine (MIL) are important drugs for the treatment of parasite infections. The mitochondrion is likely to play a central role in SbIII and MIL induced cell death in this parasite. Enriched mitochondrial samples from promastigotes selected step by step for resistance to SbIII and MIL were subjected to differential proteomic analysis. A shared decrease in both mutants in the levels of pyruvate dehydrogenase, dihydrolipoamide dehydrogenase, and isocitrate dehydrogenase was observed, as well as a differential abundance in two calcium-binding proteins and the unique dynamin-1-like protein of the parasite. Both mutants presented a shared increase in the succinyl-CoA:3-ketoacid-coenzyme A transferase and the abundance of numerous hypothetical proteins was also altered in both mutants. In general, the proteomic changes observed in the MIL mutant were less pronounced than in the SbIII mutant, probably due to the early appearance of a mutation in the miltefosine transporter abrogating the need for a strong mitochondrial adaptation. This study is the first analysis of the mitochondrial proteome and offers powerful insights into the adaptations to this organelle during SbIII and MIL drug resistance.

摘要

锑(SbIII)和米替福新(MIL)是治疗寄生虫感染的重要药物。线粒体可能在该寄生虫中SbIII和MIL诱导的细胞死亡中起核心作用。对逐步选择出的对SbIII和MIL具有抗性的前鞭毛体的富集线粒体样本进行差异蛋白质组分析。观察到两个突变体中丙酮酸脱氢酶、二氢硫辛酰胺脱氢酶和异柠檬酸脱氢酶水平均共同下降,以及两种钙结合蛋白和该寄生虫独特的动力蛋白1样蛋白丰度存在差异。两个突变体中琥珀酰辅酶A:3-酮酸辅酶A转移酶均共同增加,并且两个突变体中许多假定蛋白的丰度也发生了改变。总体而言,在MIL突变体中观察到的蛋白质组变化不如在SbIII突变体中明显,这可能是由于米替福新转运蛋白中早期出现的突变消除了对线粒体强烈适应的需求。本研究是对线粒体蛋白质组的首次分析,并为在SbIII和MIL耐药过程中对该细胞器的适应性提供了有力见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2965/5217391/41f9ee111c0c/proteomes-03-00328-g001.jpg

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