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Improved In-gel Reductive β-Elimination for Comprehensive O-linked and Sulfo-glycomics by Mass Spectrometry
Authors:David B Nix  Tadahiro Kumagai  Toshihiko Katoh  Michael Tiemeyer  Kazuhiro Aoki
Institution:1.Complex Carbohydrate Research Center, University of Georgia;2.Department of Biochemistry and Molecular Biology, University of Georgia;3.Research Institute for Bioresources and Biotechnology, Ishikawa Prefectural University
Abstract:Separation of proteins by SDS-PAGE followed by in-gel proteolytic digestion of resolved protein bands has produced high-resolution proteomic analysis of biological samples. Similar approaches, that would allow in-depth analysis of the glycans carried by glycoproteins resolved by SDS-PAGE, require special considerations in order to maximize recovery and sensitivity when using mass spectrometry (MS) as the detection method. A major hurdle to be overcome in achieving high-quality data is the removal of gel-derived contaminants that interfere with MS analysis. The sample workflow presented here is robust, efficient, and eliminates the need for in-line HPLC clean-up prior to MS. Gel pieces containing target proteins are washed in acetonitrile, water, and ethyl acetate to remove contaminants, including polymeric acrylamide fragments. O-linked glycans are released from target proteins by in-gel reductive β-elimination and recovered through robust, simple clean-up procedures. An advantage of this workflow is that it improves sensitivity for detecting and characterizing sulfated glycans. These procedures produce an efficient separation of sulfated permethylated glycans from non-sulfated (sialylated and neutral) permethylated glycans by a rapid phase-partition prior to MS analysis, and thereby enhance glycomic and sulfoglycomic analyses of glycoproteins resolved by SDS-PAGE.
Keywords:Chemistry  Issue 93  glycoprotein  glycosylation  in-gel reductive β  -elimination  O-linked glycan  sulfated glycan  mass spectrometry  protein ID  SDS-PAGE  glycomics  sulfoglycomics
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