| The in vitro reconstitution of nucleosome and its binding patterns with HMG1/2 and HMG14/17 proteins |
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| 作者姓名: | Zhang SB Huang J Zhao H Zhang Y Hou CH Cheng XD Jiang C Li MQ Hu J Qian RL |
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| 作者单位: | [1]GroupofGlobinGeneExpressionandRegulation,StateKeyLaboratoryofMolecularBiology,InstituteofBiochemistryandCellBiology,ShanghaiInstitutesforBiologicalSciences,ChineseAcademyofSciences,Shanghal200031,China [2]ShanghaiInstituteofNuclearResearch,ChineseAcademyofSciences,Shanghai201800,China |
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| 摘 要: | Using atomic force microscopy (AFM), the dynamic process of the in vitro nucleosome reconstitution followed by slow dilution from high salt to low salt was visualized. Data showed that the histone octamers were dissociatedfrom DNA at 1M NaC1. When the salt concentration was slowly reduced to 650 mM and 300 mM, the core histones bound to the naked DNA gradually. Once the salt concentration was reduced to 50 mM the classic “beads-on-a-string“ structure was clearly visualized. Furthermore, using the technique of the in vitro reconstitution of nucleosome,the mono- and di- nucleosomes were assembled in vitro with both HS2core (-10681 to -10970 bp) and NCR2 (-372to -194 bp) DNA sequences in the 5‘flanking sequence of human b-globin gene. Data revealed that HMG 1/2 and HMG 14/17 proteins binding to both DNA sequences are changeable following the assembly and disassembly of nucleosomes. We suggest that the changeable binding patterns of HMG 14/17 and HMG1/2 proteins with these regulatory elements may be critical in the process of nucleosome assembly, recruitment of chromatin-modifying activities, and the regulation of human b-globin gene expression.
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| 关 键 词: | 原子力显微镜 核小体 组蛋白 体外装配 |
The in vitro reconstitution of nucleosome and its binding patterns with HMG1/2 and HMG14/17 proteins |
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| Zhang SB,Huang J,Zhao H,Zhang Y,Hou CH,Cheng XD,Jiang C,Li MQ,Hu J,Qian RL.The in vitro reconstitution of nucleosome and its binding patterns with HMG1/2 and HMG14/17 proteins[J].Cell Research,2003,13(5):351-360. |
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| Authors: | Zhang Shu Bing Huang Jian Zhao Hui Zhang Yi Hou Chun Hui Cheng Xiao Dong Jiang Chu Li Min Qian Hu Jun Qian Ruo Lan |
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| Institution: | Group of Globin Gene Expression and Regulation, State Key Laboratory of Molecular Biology, Institute of Biochemistry and Cell Biology, Shanghai Institutes for Biological Sciences, Chinese Academy of Sciences, Shanghai 200031, China. |
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| Abstract: | Using atomic force microscopy (AFM), the dynamic process of the in vitro nucleosome reconstitution followed by slow dilution from high salt to low salt was visualized. Data showed that the histone octamers were dissociated from DNA at 1M NaCl. When the salt concentration was slowly reduced to 650 mM and 300 mM, the core histones bound to the naked DNA gradually. Once the salt concentration was reduced to 50 mM the classic "beads-on-astring" structure was clearly visualized. Furthermore, using the technique of the in vitro reconstitution of nucleosome, the mono- and di- nucleosomes were assembled in vitro with both HS2core (-10681 to -10970 bp) and NCR2 (-372 to -194 bp) DNA sequences in the 5'flanking sequence of human b-globin gene. Data revealed that HMG 1/2 and HMG 14/17 proteins binding to both DNA sequences are changeable following the assembly and disassembly of nucleosomes. We suggest that the changeable binding patterns of HMG 14/17 and HMG1/2 proteins with these regulatory elements may be critical in the process of nucleosome assembly, recruitment of chromatin-modifying activities, and the regulation of human b-globin gene expression. |
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