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Molecular & Cellular Proteomics

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Research

Targeted analysis of lysosomal directed proteins and their sites of mannose-6-phosphate modification

View ORCID ProfileTomislav Caval, Jing Zhu, View ORCID ProfileWeihua Tian, Sanne N Remmelzwaal, Zhang Yang, Henrik Clausen and View ORCID ProfileAlbert J. R. Heck  Correspondence email
Molecular & Cellular Proteomics September 20, 2018, mcp.RA118.000967; https://doi.org/10.1074/mcp.RA118.000967
Tomislav Caval
Utrecht University, Netherlands
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Jing Zhu
Utrecht University, Netherlands
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Weihua Tian
University of Copenhagen, Denmark
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Sanne N Remmelzwaal
Utrecht University, Netherlands
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Zhang Yang
University of Copenhagen
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Henrik Clausen
University of Copenhagen
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Albert J. R. Heck
Biomolecular Mass Spectrometry and Proteomics, Utrecht University, Netherlands
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  • ORCID record for Albert J. R. Heck
  • For correspondence: a.j.r.heck@uu.nl
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Abstract

Mannose-6-phosphate (M6P) is a distinctive post-translational modification critical for trafficking of lysosomal acid hydrolases into the lysosome. Improper trafficking into the lysosome, and/or lack of certain hydrolases, results in a toxic accumulation of their substrates within the lysosomes. To gain insight into the enzymes destined to the lysosome these glycoproteins can be distinctively enriched and studied using their unique M6P tag. Here we demonstrate, by adapting a protocol optimized for the enrichment of phosphopeptides using Fe3+-IMAC chromatography, that proteome-wide M6P glycopeptides can be selectively enriched and subsequently analyzed by mass spectrometry, taking advantage of exclusive phosphomannose oxonium fragment marker ions. As proof-of-concept of this protocol, applying it to HeLa cells, we identified hundreds of M6P-modified glycopeptides on 35 M6P-modified glycoproteins. We next targeted CHO cells, either wild-type or cells deficient in Acp2 and Acp5, which are acid phosphatases targeting M6P. In the KO CHO cells we observed a 20-fold increase of the abundance of the M6P-modification on endogenous CHO glycoproteins but also on the recombinantly over-expressed lysosomal human alpha-galactosidase. We conclude that our approach could thus be of general interest for characterization of M6P glycoproteomes as well as characterization of lysosomal enzymes used as treatment in enzyme replacement therapies targeting lysosomal storage diseases.

  • lysosome
  • lysosomal disorders
  • mannose-6-phosphate
  • mannose-6-phosphate receptors
  • targeted degradation
  • Cellular organelles*
  • Glycoprotein Pathways*
  • Glycoproteins*
  • Glycoproteomics
  • Phosphorylation

Footnotes

  • Author contributions: T.C. and A.J.R.H. designed research; T.C., J.Z., and S.N.R. performed research; T.C. and J.Z. analyzed data; T.C., J.Z., H.C., and A.J.R.H. wrote the paper; W.T., Z.Y., and H.C. contributed new reagents/analytic tools.

  • Received July 12, 2018.
  • Revision received September 20, 2018.
  • Accepted September 20, 2018.
  • Published under license by The American Society for Biochemistry and Molecular Biology, Inc.
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Targeted analysis of lysosomal directed proteins and their sites of mannose-6-phosphate modification
Tomislav Caval, Jing Zhu, Weihua Tian, Sanne N Remmelzwaal, Zhang Yang, Henrik Clausen, Albert J. R. Heck
Molecular & Cellular Proteomics September 20, 2018, mcp.RA118.000967; DOI: 10.1074/mcp.RA118.000967

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Targeted analysis of lysosomal directed proteins and their sites of mannose-6-phosphate modification
Tomislav Caval, Jing Zhu, Weihua Tian, Sanne N Remmelzwaal, Zhang Yang, Henrik Clausen, Albert J. R. Heck
Molecular & Cellular Proteomics September 20, 2018, mcp.RA118.000967; DOI: 10.1074/mcp.RA118.000967
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