Literature DB >> 16210410

Differential expression profiling of membrane proteins by quantitative proteomics in a human mesenchymal stem cell line undergoing osteoblast differentiation.

Leonard J Foster1, Patricia A Zeemann, Chen Li, Matthias Mann, Ole Nørregaard Jensen, Moustapha Kassem.   

Abstract

One of the major limitations for understanding the biology of human mesenchymal stem cells (hMSCs) is the absence of prospective markers needed for distinguishing them from other cells and for monitoring lineage-specific differentiation. Mass spectrometry (MS)-based proteomics has proven extremely useful for analyzing complex protein expression patterns and, when applied quantitatively, can be used to resolve subtle differences between samples. Thus, we used MS to characterize changes in expression of membrane protein markers before and after short-term induction of osteoblast (OB) differentiation in a cell model of hMSCs established by overexpression of human telomerase reverse-transcriptase gene. We identified 463 unique proteins with extremely high confidence, including all known markers of hMSCs (e.g., SH3 [CD71], SH2 [CD105], CD166, CD44, Thy1, CD29, and HOP26 [CD63]) among 148 integral membrane or membrane-anchored proteins and 159 membrane-associated proteins. Twenty-nine integrins and cell adhesion molecules, 20 receptors, and 18 Ras-related small GTPases were also identified. Upon OB differentiation, the expression levels of 83 proteins increased by at least twofold whereas the levels of another 21 decreased by at least twofold. For example, alkaline phosphatase (ALP), versican core protein, and tenascin increased 27-, 12-, and 4-fold, respectively, and fatty acid synthase decreased sixfold. The observed increases in veriscan and ALP were confirmed using immunocytochemistry and cytochemistry. Quantitative real-time reverse transcription-polymerase chain reaction confirmed the presence of mRNA of these membrane proteins. However, with the exception of ALP, no concordance was detected between the changes in levels of gene and protein expression during OB differentiation. In conclusion, MS-based proteomics can reveal novel markers for MSCs that can be used for their isolation and for monitoring OB differentiation.

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Year:  2005        PMID: 16210410     DOI: 10.1634/stemcells.2004-0372

Source DB:  PubMed          Journal:  Stem Cells        ISSN: 1066-5099            Impact factor:   6.277


  65 in total

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2.  Altered membrane dynamics of quantum dot-conjugated integrins during osteogenic differentiation of human bone marrow derived progenitor cells.

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Review 3.  Organellar proteomics: turning inventories into insights.

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5.  Proteomic Profiling of Native Unpassaged and Culture-Expanded Mesenchymal Stromal Cells (MSC).

Authors:  Erika Moravcikova; E Michael Meyer; Mirko Corselli; Vera S Donnenberg; Albert D Donnenberg
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6.  A novel role for proteomics in the discovery of cell-surface markers on stem cells: Scratching the surface.

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Journal:  J Proteome Res       Date:  2008-04-15       Impact factor: 4.466

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Authors:  Chen Wang; Fangfang Guo; Heng Zhou; Yun Zhang; Zhigang Xiao; Lei Cui
Journal:  Tissue Eng Part A       Date:  2012-11-14       Impact factor: 3.845

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Journal:  Dig Dis Sci       Date:  2017-04-22       Impact factor: 3.199

10.  Quantitative proteomics analysis of chondrogenic differentiation of C3H10T1/2 mesenchymal stem cells by iTRAQ labeling coupled with on-line two-dimensional LC/MS/MS.

Authors:  Yu-hua Ji; Ju-ling Ji; Fen-yong Sun; Yao-ying Zeng; Xian-hui He; Jing-xian Zhao; Yu Yu; Shou-he Yu; Wei Wu
Journal:  Mol Cell Proteomics       Date:  2009-12-15       Impact factor: 5.911

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