Literature DB >> 28177569

The oxidized thiol proteome in aging and cataractous mouse and human lens revealed by ICAT labeling.

Benlian Wang1, Grant Hom2, Sheng Zhou3, Minfei Guo4, Binbin Li5, Jing Yang3, Vincent M Monnier2,6, Xingjun Fan2.   

Abstract

Age-related cataractogenesis is associated with disulfide-linked high molecular weight (HMW) crystallin aggregates. We recently found that the lens crystallin disulfidome was evolutionarily conserved in human and glutathione-depleted mouse (LEGSKO) cataracts and that it could be mimicked by oxidation in vitro (Mol. Cell Proteomics, 14, 3211-23 (2015)). To obtain a comprehensive blueprint of the oxidized key regulatory and cytoskeletal proteins underlying cataractogenesis, we have now used the same approach to determine, in the same specimens, all the disulfide-forming noncrystallin proteins identified by ICAT proteomics. Seventy-four, 50, and 54 disulfide-forming proteins were identified in the human and mouse cataracts and the in vitro oxidation model, respectively, of which 17 were common to all three groups. Enzymes with oxidized cysteine at critical sites include GAPDH (hGAPDH, Cys247), glutathione synthase (hGSS, Cys294), aldehyde dehydrogenase (hALDH1A1, Cys126 and Cys186), sorbitol dehydrogenase (hSORD, Cys140, Cys165, and Cys179), and PARK7 (hPARK7, Cys46 and Cys53). Extensive oxidation was also present in lens-specific intermediate filament proteins, such as BFSP1 and BFSP12 (hBFSP1 and hBFSP12, Cys167, Cys65, and Cys326), vimentin (mVim, Cys328), and cytokeratins, as well as microfilament and microtubule filament proteins, such as tubulin and actins. While the biological impact of these modifications for lens physiology remains to be determined, many of these oxidation sites have already been associated with either impaired metabolism or cytoskeletal architecture, strongly suggesting that they have a pathogenic role in cataractogenesis. By extrapolation, these findings may be of broader significance for age- and disease-related dysfunctions associated with oxidant stress.
© 2016 The Authors. Aging Cell published by the Anatomical Society and John Wiley & Sons Ltd.

Entities:  

Keywords:  aging; cataractogenesis; disulfide; mass spectrometry; proteomics; reactive oxygen species

Mesh:

Substances:

Year:  2016        PMID: 28177569      PMCID: PMC5334568          DOI: 10.1111/acel.12548

Source DB:  PubMed          Journal:  Aging Cell        ISSN: 1474-9718            Impact factor:   9.304


  46 in total

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Authors:  K R Rogers; H Herrmann; W W Franke
Journal:  J Struct Biol       Date:  1996 Jul-Aug       Impact factor: 2.867

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Authors:  V A Padgaonkar; L R Lin; V R Leverenz; A Rinke; V N Reddy; F J Giblin
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3.  Proteome-transcriptome analysis and proteome remodeling in mouse lens epithelium and fibers.

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4.  MS/MS in silico subtraction-based proteomic profiling as an approach to facilitate disease gene discovery: application to lens development and cataract.

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5.  Aging lens epithelium is susceptible to ferroptosis.

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Review 6.  Proteomic characterization of the human lens and Cataractogenesis.

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Review 7.  Proteomic Applications in Antimicrobial Resistance and Clinical Microbiology Studies.

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8.  Dynamic disulfide exchange in a crystallin protein in the human eye lens promotes cataract-associated aggregation.

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Review 9.  Protein Posttranslational Modifications: Roles in Aging and Age-Related Disease.

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Review 10.  DJ-1 in Ocular Diseases: A Review.

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