Proteomic analysis of organ-specific post-translational lysine acetylation and -methylation in mice by use of anti-acetyllysine and -methyllysine mouse monoclonal antibodies
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作者:
Iwabata, H
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机构:Adv Life Sci Inst, Div Res & Dev, Wako, Saitama 3510112, Japan
Iwabata, H
Yoshida, M
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机构:Adv Life Sci Inst, Div Res & Dev, Wako, Saitama 3510112, Japan
Yoshida, M
Komatsu, Y
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机构:Adv Life Sci Inst, Div Res & Dev, Wako, Saitama 3510112, Japan
Komatsu, Y
机构:
[1] Adv Life Sci Inst, Div Res & Dev, Wako, Saitama 3510112, Japan
[2] Japan Sci & Technol Agcy, CREST Res Project, Saitama, Saitama, Japan
[3] RIKEN, Chem Genet Lab, Wako, Saitama 35101, Japan
Post-translational lysine-acetylation and -methylation are two major PTMs of lysine residues in proteins. Recently, we established pan-reactive anti-acetyllysine mouse mAbs, which can bind to N epsilon-acetylated lysine residues in various contexts of amino acid sequences. In the present study, we established pan-reactive anti-methyllysine mouse mAbs comparable to the anti-acetyllysine ones. By using these anti-acetyllysine and -methyllysine antibodies, we found that the pattern of lysine-acetylated and -methylated proteins in mouse organs showed extreme variation from organ to organ. We selected brain and skeletal muscle as model cases to be further analyzed by 2-DE followed by Westem blotting. In brain, alpha-tubulin at its basal level was found to be extremely acetylated; and alpha-enolase was shown to be a newly recognized possibly acetylated protein. NF-L protein, Hsc70, alpha-tubulin fragments, beta-actin, and brain-type creatine kinase were identified as putative lysine-methylated proteins in mouse brain. In skeletal muscle, lysine-methylation of alpha-actin and both lysine-acetylation and -methylation of muscle-type creatine kinase were found as novel putative lysine-modified proteins. The approach presented here might be useful to find novel disease markers and/or drug target molecules that would not be noticed by use of the traditional proteomic approach only.