Oxidative Stress Induced Dysfunction of Protein Synthesis in 661W Mice Photoreceptor Cells.

IF 4 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY
Liting Deng, Vivek Gupta, Morteza Abyadeh, Nitin Chitranshi, Kanishka Pushpitha, Yunqi Wu, Veer Gupta, Yuyi You, Joao A Paulo, Stuart L Graham, Mehdi Mirzaei, Paul A Haynes
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引用次数: 0

Abstract

Photoreceptor cells are highly susceptible to oxidative-stress-induced damage due to their high metabolic rate. Oxidative stress plays a key role in driving pathological events in several different ocular diseases, which lead to retinal degeneration and ultimately blindness. A growing number of studies have been performed to understand downstream events caused by ROS induced oxidative stress in photoreceptor cells; however, the underlying mechanisms of ROS toxicity are not fully understood. To shed light on ROS induced downstream pathological events, we employed a tandem mass tag (TMT) labelling-based quantitative mass-spectrometric approach to determine proteome changes in 661W photoreceptor cells following oxidative stress induction via the application of different concentrations of H2O2 at different time points. Overall, 5920 proteins were identified and quantified, and 450 differentially expressed proteins (DEPs) were identified, which were altered in a dose and time dependent manner in all treatment groups compared to the control group. These proteins were involved in several biological pathways, including spliceosome and ribosome response, activated glutathione metabolism, decreased ECM-receptor interaction, oxidative phosphorylation, abnormally regulated lysosome, apoptosis, and ribosome biogenesis. Our results highlighted ECM receptor interaction, oxidative phosphorylation and spliceosome pathways as the major targets of oxidative stress that might mediate vascular dysfunction and cellular senescence.

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氧化应激诱导 661W 小鼠感光细胞蛋白质合成障碍
感光细胞的新陈代谢率很高,因此极易受到氧化应激引起的损伤。氧化应激在多种眼部疾病的病理过程中起着关键作用,导致视网膜变性,最终导致失明。为了了解 ROS 在感光细胞中诱导氧化应激所导致的下游事件,已经开展了越来越多的研究。为了揭示 ROS 诱导的下游病理事件,我们采用了一种基于串联质量标签(TMT)标记的定量质谱方法,来确定 661W 光感受器细胞在不同时间点应用不同浓度的 H2O2 诱导氧化应激后蛋白质组的变化。总共鉴定和量化了 5920 个蛋白质,并鉴定了 450 个差异表达蛋白质(DEPs),与对照组相比,这些蛋白质在所有处理组中都发生了与剂量和时间相关的变化。这些蛋白质参与了多个生物学通路,包括剪接体和核糖体反应、激活的谷胱甘肽代谢、ECM 与受体相互作用的减少、氧化磷酸化、异常调控的溶酶体、细胞凋亡和核糖体生物发生。我们的研究结果突出表明,ECM 受体相互作用、氧化磷酸化和剪接体途径是氧化应激的主要靶点,可能介导血管功能障碍和细胞衰老。
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来源期刊
Proteomes
Proteomes Biochemistry, Genetics and Molecular Biology-Clinical Biochemistry
CiteScore
6.50
自引率
3.00%
发文量
37
审稿时长
11 weeks
期刊介绍: Proteomes (ISSN 2227-7382) is an open access, peer reviewed journal on all aspects of proteome science. Proteomes covers the multi-disciplinary topics of structural and functional biology, protein chemistry, cell biology, methodology used for protein analysis, including mass spectrometry, protein arrays, bioinformatics, HTS assays, etc. Our aim is to encourage scientists to publish their experimental and theoretical results in as much detail as possible. Therefore, there is no restriction on the length of papers. Scope: -whole proteome analysis of any organism -disease/pharmaceutical studies -comparative proteomics -protein-ligand/protein interactions -structure/functional proteomics -gene expression -methodology -bioinformatics -applications of proteomics
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