Literature DB >> 3196285

Mitochondria contain a proteolytic system which can recognize and degrade oxidatively-denatured proteins.

O Marcillat1, Y Zhang, S W Lin, K J Davies.   

Abstract

When incubated with mitochondria in an air atmosphere, menadione and doxorubicin (which redox cycle with the respiratory chain to produce oxygen radicals), as well as xanthine oxidase plus xanthine (which generate superoxide and H2O2), stimulated the degradation of newly-synthesized [( 3H]leucine-labelled) mitochondrial polypeptides. No stimulation was observed in an N2 atmosphere, ATP was not required, and xanthine oxidase was not effective without xanthine. Various forms of oxidative stress induced varying degrees of protein cross-linking, protein fragmentation and proteolysis, as judged by gel electrophoresis and amino acid analysis. To learn more about the proteolytic enzymes involved in degradation, we undertook studies with purified protein substrates which had been exposed to oxidative stress (OH or H2O2) in vitro. Despite mitochondrial contamination with acid proteases of lysosomal (and other) origin, pH profiles revealed distinct proteolytic activities at both pH 4 and pH 8. The pH 8 activity preferentially degraded the oxidatively-denatured forms of haemoglobin, albumin and superoxide dismutase; was unaffected by digitonin; and exhibited a several-fold increase in activity upon mitochondrial disruption (highest activity being found in the matrix). In contrast, the pH 4 activity was dramatically decreased by digitonin treatment (to reduce lysosomal contamination); was unaffected by mitochondrial disruption; and showed no preference for oxidatively-denatured proteins. The pH 8 activity was not stimulated by ATP, but was inhibited by EDTA, haemin and phenylmethylsulphonyl fluoride. In contrast, the contaminating pH 4 activity was only inhibited by pepstatin and leupeptin. Thus, our experiments reveal a distinct mitochondrial (matrix) proteolytic pathway which can preferentially degrade oxidatively-denatured proteins.

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Year:  1988        PMID: 3196285      PMCID: PMC1135138          DOI: 10.1042/bj2540677

Source DB:  PubMed          Journal:  Biochem J        ISSN: 0264-6021            Impact factor:   3.857


  42 in total

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Authors:  S M Rapoport; T Schewe; R Wiesner; W Halangk; P Ludwig; M Janicke-Höhne; C Tannert; C Hiebsch; D Klatt
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3.  Hydroperoxide metabolism in mammalian organs.

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4.  The interaction of bovine erythrocyte superoxide dismutase with hydrogen peroxide: inactivation of the enzyme.

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6.  Turnover of bacterial glutamine synthetase: oxidative inactivation precedes proteolysis.

Authors:  R L Levine; C N Oliver; R M Fulks; E R Stadtman
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7.  Mitochondrial NADH dehydrogenase-catalyzed oxygen radical production by adriamycin, and the relative inactivity of 5-iminodaunorubicin.

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8.  A novel proteinase associated with mitochondrial membranes.

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Journal:  Biochem Biophys Res Commun       Date:  1978-08-14       Impact factor: 3.575

9.  A novel SH-type carboxypeptidase in the inner membrane of rat-liver mitochondria.

Authors:  R Haas; P C Heinrich
Journal:  Eur J Biochem       Date:  1979-05-02

10.  Proteolysis of the products of mitochondrial protein synthesis in yeast mitochondria and submitochondrial particles.

Authors:  S L Kalnov; L A Novikova; A S Zubatov; V N Luzikov
Journal:  Biochem J       Date:  1979-07-15       Impact factor: 3.857

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  13 in total

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Review 5.  Biochemistry and pathology of radical-mediated protein oxidation.

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9.  Tolerance of rats to hyperoxia. Lung antioxidant enzyme gene expression.

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10.  Increased formation and degradation of malondialdehyde-modified proteins under conditions of peroxidative stress.

Authors:  H Mahmoodi; M Hadley; Y X Chang; H H Draper
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