Protein Microarray Characterization of the S-Nitrosoproteome*□S

نویسندگان

  • Yun-Il Lee
  • Daniel Giovinazzo
  • Ho Chul Kang
  • Yunjong Lee
  • Jun Seop Jeong
  • Paschalis-Thomas Doulias
  • Zhi Xie
  • Jianfei Hu
  • Mehdi Ghasemi
  • Harry Ischiropoulos
  • Jiang Qian
  • Heng Zhu
  • Seth Blackshaw
  • Valina L. Dawson
  • Ted M. Dawson
چکیده

Nitric oxide (NO) mediates a substantial part of its physiologic functions via S-nitrosylation, however the cellular substrates for NO-mediated S-nitrosylation are largely unknown. Here we describe the S-nitrosoproteome using a high-density protein microarray chip containing 16,368 unique human proteins. We identified 834 potentially Snitrosylated human proteins. Using a unique and highly specific labeling and affinity capture of S-nitrosylated proteins, 138 cysteine residues on 131 peptides in 95 proteins were determined, defining critical sites of NO’s actions. Of these cysteine residues 113 are novel sites of S-nitrosylation. A consensus sequence motif from these 834 proteins for S-nitrosylation was identified, suggesting that the residues flanking the S-nitrosylated cysteine are likely to be the critical determinant of whether the cysteine is S-nitrosylated. We identify eight ubiquitin E3 ligases, RNF10, RNF11, RNF41, RNF141, RNF181, RNF208, WWP2, and UBE3A, whose activities are modulated by S-nitrosylation, providing a unique regulatory mechanism of the ubiquitin proteasome system. These results define a new and extensive set of proteins that are susceptible to NO regulation via S-nitrosylation. Similar approaches could be used to identify other post-translational modification proteomes. Molecular & Cellular Proteomics 13: 10.1074/ mcp.M113.032235, 63–72, 2014.

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تاریخ انتشار 2013