MS Western, a Method of Multiplexed Absolute Protein Quantification is a 
Practical Alternative to Western Blotting.

Kumar, Mukesh; Joseph, Shai; Augsburg, Martina; Bogdanova, Aliona; Drechsel, David N.; Vastenhouw, Nadine; Buchholz, Frank; Gentzel, Marc; Shevchenko, Andrej

doi:10.1074/mcp.O117.067082

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MS Western, a Method of Multiplexed Absolute Protein Quantification is a Practical Alternative to Western Blotting.

MPG-Autoren

/persons/resource/persons219357

Kumar, Mukesh
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons219279

Joseph, Shai
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons218985

Augsburg, Martina
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons78966

Bogdanova, Aliona
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons219118

Drechsel, David N.
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons219759

Vastenhouw, Nadine
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons219042

Buchholz, Frank
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons219180

Gentzel, Marc
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

/persons/resource/persons218972

Shevchenko, Andrej
Max Planck Institute for Molecular Cell Biology and Genetics, Max Planck Society;

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Zitation

Kumar, M., Joseph, S., Augsburg, M., Bogdanova, A., Drechsel, D. N., Vastenhouw, N., et al. (2018). MS Western, a Method of Multiplexed Absolute Protein Quantification is a Practical Alternative to Western Blotting. Molecular & cellular proteomics: MCP, 17(2), 384-396. doi:10.1074/mcp.O117.067082.

Zitierlink: https://hdl.handle.net/21.11116/0000-0003-F626-D

Zusammenfassung

Absolute quantification of proteins elucidates the molecular composition, regulation and dynamics of multiprotein assemblies and networks. Here we report on a method termed MS Western that accurately determines the molar abundance of dozens of user-selected proteins at the subfemtomole level in whole cell or tissue lysates without metabolic or chemical labeling and without using specific antibodies. MS Western relies on GeLC-MS/MS and quantifies proteins by in-gel codigestion with an isotopically labeled QconCAT protein chimera composed of concatenated proteotypic peptides. It requires no purification of the chimera and relates the molar abundance of all proteotypic peptides to a single reference protein. In comparative experiments, MS Western outperformed immunofluorescence Western blotting by the protein detection specificity, linear dynamic range and sensitivity of protein quantification. To validate MS Western in an in vivo experiment, we quantified the molar content of zebrafish core histones H2A, H2B, H3 and H4 during ten stages of early embryogenesis. Accurate quantification (CV<10%) corroborated the anticipated histones equimolar stoichiometry and revealed an unexpected trend in their total abundance.