Literature DB >> 23233448

Deletion of cysteine cathepsins B or L yields differential impacts on murine skin proteome and degradome.

Stefan Tholen1, Martin L Biniossek, Martina Gansz, Alejandro Gomez-Auli, Fee Bengsch, Agnes Noel, Jayachandran N Kizhakkedathu, Melanie Boerries, Hauke Busch, Thomas Reinheckel, Oliver Schilling.   

Abstract

Numerous studies highlight the fact that concerted proteolysis is essential for skin morphology and function. The cysteine protease cathepsin L (Ctsl) has been implicated in epidermal proliferation and desquamation, as well as in hair cycle regulation. In stark contrast, mice deficient in cathepsin B (Ctsb) do not display an overt skin phenotype. To understand the systematic consequences of deleting Ctsb or Ctsl, we determined the protein abundances of >1300 proteins and proteolytic cleavage events in skin samples of wild-type, Ctsb(-/-), and Ctsl(-/-) mice via mass-spectrometry-based proteomics. Both protease deficiencies revealed distinct quantitative changes in proteome composition. Ctsl(-/-) skin revealed increased levels of the cysteine protease inhibitors cystatin B and cystatin M/E, increased cathepsin D, and an accumulation of the extracellular glycoprotein periostin. Immunohistochemistry located periostin predominantly in the hypodermal connective tissue of Ctsl(-/-) skin. The proteomic identification of proteolytic cleavage sites within skin proteins revealed numerous processing sites that are underrepresented in Ctsl(-/-) or Ctsb(-/-) samples. Notably, few of the affected cleavage sites shared the canonical Ctsl or Ctsb specificity, providing further evidence of a complex proteolytic network in the skin. Novel processing sites in proteins such as dermokine and Notch-1 were detected. Simultaneous analysis of acetylated protein N termini showed prototypical mammalian N-alpha acetylation. These results illustrate an influence of both Ctsb and Ctsl on the murine skin proteome and degradome, with the phenotypic consequences of the absence of either protease differing considerably.

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Year:  2012        PMID: 23233448      PMCID: PMC3591655          DOI: 10.1074/mcp.M112.017962

Source DB:  PubMed          Journal:  Mol Cell Proteomics        ISSN: 1535-9476            Impact factor:   5.911


  97 in total

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  19 in total

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4.  Matrix Metalloproteinase 10 Degradomics in Keratinocytes and Epidermal Tissue Identifies Bioactive Substrates With Pleiotropic Functions.

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6.  Cathepsin L Regulates Metabolic Networks Controlling Rapid Cell Growth and Proliferation.

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8.  Fibroblast activation protein-α, a stromal cell surface protease, shapes key features of cancer associated fibroblasts through proteome and degradome alterations.

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9.  Double deficiency of cathepsins B and L results in massive secretome alterations and suggests a degradative cathepsin-MMP axis.

Authors:  Stefan Tholen; Martin L Biniossek; Martina Gansz; Theresa D Ahrens; Manuel Schlimpert; Jayachandran N Kizhakkedathu; Thomas Reinheckel; Oliver Schilling
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10.  Identification of Novel Natural Substrates of Fibroblast Activation Protein-alpha by Differential Degradomics and Proteomics.

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Journal:  Mol Cell Proteomics       Date:  2018-09-26       Impact factor: 5.911

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