| Mapping the Binding Site of P53 on UBC9 by NMR Spectroscopy |
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| 作者姓名: | 林东海 |
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| 作者单位: | DepartmentofBiochemistry,TheHongKongUniversityofScienceandTechnology,HongKong,china |
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| 基金项目: | ProjectsupportedbytheNationalNaturalScienceFoundationofChina (No.19975 0 38) |
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| 摘 要: | Human UBCP9 is a member of the E2 family of proteins.However,instead of conjugating to ubiquitin,it conjugates to a ubiquitin bomologue SUMO-1(also known as UBL1,GMP1,SMTP3,PICT-1 and sentrin).The SUMO-1 conjugation pathway is very similar to that of ubiquin with regard to the primary sequences of the ubiquitin activating enzymes(E1),the three-dimensional structures of the ubiquitin conjugating enzymes(E2),and the chemistry of the overall conjugation pathway.The interactiov of p53 and UBC9,the E2 of the SUMO-1 pathway,has heen studied by nuclear magnetic resonance spectroscopy.A peptide corresponding to the nuclear localization domain of p53 specifically interacts with UBC9 and this interaction is likely to be important for conjugation of p53 with SUMO-1.The largest chemical shift changes on UBC9 occur at residues94 and 129-135.This region is adjacent to the active site and has slgniflcant dynamic behavior on the μs-ms and ps-ns timescales.Correlation of chemical shift changes and mobility of these residues further suggest the importance of these residues in substrate recognition.
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| 关 键 词: | P53 UBC9 NMR DNA 蛋白质 修复 细胞因子 人体 |
Mapping the Binding Site of P53 on UBC9 by NMR Spectroscopy |
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| LIN,Dong-Hai a.Mapping the Binding Site of P53 on UBC9 by NMR Spectroscopy[J].Chinese Journal of Chemistry,2002,20(10):937-943. |
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| Authors: | LIN Dong-Hai a |
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| Institution: | LIN,Dong-Hai a Department of Biochemistry,The Hong Kong University of Science & Technology,Hong Kong,China b Center for Drug Discovery and Design,State Key Laboratory of Drug Research,Shanghai Institute of Meteria Medica,Shanghai Institutes |
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| Abstract: | Human UBC9 is a member of the E2 family of proteins. However, instead of conjugating to ubiquitin, it conjugates to a ubiquitin homologue SUMO‐1 (also known as UBL1, GMP1, SMTP3, PICT‐1 and sentrin). The SUMO‐1 conjugation pathway is very similar to that of ubiquitin with regard to the primary sequences of the ubiquitin activating enzymes (E1), the three‐dimensional structures of the ubiquitin conjugating enzymes (E2), and the chemistry of the overall conjugation pathway. The interaction of p53 and UBC9, the E2 of the SUMO‐1 pathway, has been studied by nuclear magnetic resonance spectroscopy. A peptide corresponding to the nuclear localization domain of p53 specifically interacts with UBC9 and this interaction is likely to be important for conjugation of p53 with SUMO‐1. The largest chemical shift changes on UBC9 occur at residues 94 and 129–135. This region is adjacent to the active site and has significant dynamic behavior on the μs—ms and ps—ns timescales. Correlation of chemical shift changes and mobility of these residues further suggest the importance of these residues in substrate recognition. |
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| Keywords: | NMR protein-peptide interaction SUMO-1 pathway E2 enzyme p53 |
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