Proteomic Analysis of Microtubule-associated Proteins during Macrophage Activation

doi:10.1074/mcp.M900190-MCP200

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Originally published In Press as doi:10.1074/mcp.M900190-MCP200 on August 2, 2009.

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Molecular & Cellular Proteomics 8:2500-2514, 2009.
© 2009 by The American Society for Biochemistry and Molecular Biology, Inc.

Research

Proteomic Analysis of Microtubule-associated Proteins during Macrophage Activation^*^,

Prerna C. Patel, Katherine H. Fisher^,¶, Eric C. C. Yang^||, Charlotte M. Deane^,¶ and Rene E. Harrison^,**

From the ${ddagger}$ Department of Biological Sciences, University of Toronto Scarborough, 1265 Military Trail, Toronto, Ontario M1C 1A4, Canada,
$§$ Department of Statistics, University of Oxford, Oxford OX1 3TG, United Kingdom,
¶Oxford Doctoral Training Centre, University of Oxford, Oxford OX1 3QD, United Kingdom, and
||Proteomics Core Facility, Sunnybrook Research Institute, Sunnybrook Health Sciences Centre and University of Toronto, Toronto, Ontario M4N 3M5, Canada

Classical activation of macrophages induces a wide range ofsignaling and vesicle trafficking events to produce a more aggressivecellular phenotype. The microtubule (MT) cytoskeleton is crucialfor the regulation of immune responses. In the current study,we used a large scale proteomics approach to analyze the changein protein composition of the MT-associated protein (MAP) networkby macrophage stimulation with the inflammatory cytokine interferon- ${gamma}$ and the endotoxin lipopolysaccharide. Overall the analysis identified409 proteins that bound directly or indirectly to MTs. Of these,52 were up-regulated 2-fold or greater and 42 were down-regulated2-fold or greater after interferon- ${gamma}$ /lipopolysaccharide stimulation.Bioinformatics analysis based on publicly available binary proteininteraction data produced a putative interaction network ofMAPs in activated macrophages. We confirmed the up-regulationof several MAPs by immunoblotting and immunofluorescence analysis.More detailed analysis of one up-regulated protein revealeda role for HSP90β in stabilization of the MT cytoskeletonduring macrophage activation.

** Recipient of an Ontario early researcher award and CIHR new investigator award. To whom correspondence should be addressed: Dept. of Cell and Systems Biology, University of Toronto Scarborough, Toronto, Ontario M1C 1A4, Canada. Tel.: 416-287-7377; Fax: 416-287-7676; E-mail: harrison{at}utsc.utoronto.ca.