The degree of oligomerization of the H-NS nucleoid structuring protein is related to specific binding to DNA

被引:67
作者
Badaut, C
Williams, R
Arluison, V
Bouffartigues, E
Robert, B
Buc, H
Rimsky, S
机构
[1] Inst Pasteur, CNRS, URA 1773, F-75724 Paris 15, France
[2] Inst Gustave Roussy, F-94805 Villejuif, France
[3] Inst Gustave Roussy, CNRS, Ecole Normale Super Cachan, UMR 8532, F-94805 Villejuif, France
[4] Commissariat Energie Atom Saclay, CNRS, Sect Biophys Fonct Membranaires, DBJC CEA, F-91191 Gif Sur Yvette, France
[5] Commissariat Energie Atom Saclay, CNRS, URA 2096, F-91191 Gif Sur Yvette, France
关键词
D O I
10.1074/jbc.M206037200
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
At several E. coli promoters, initiation of transcription is repressed by a tight nucleoprotein complex formed by the assembly of the H-NS protein. In order to characterize the relationship between the structure of H-NS oligomers in solution and on relevant DNA fragments, we have compared wild-type H-NS and several transdominant H-NS mutants using gel shift assays, DNase I footprinting, analytical ultracentrifugation, and reactivity toward a cross-linking reagent. In solution, oligomerization occurs through two protein interfaces, one necessary to construct a dimeric core (and involving residues 1-64) and the other required for subsequent assembly of these dimers. We show that, as well as region 64-95, residues present in the NH2-terminal coiled coil domain also participate in this second interface. Our results support the view that the same interacting interfaces are also involved on the DNA. We propose that the dimeric core recognizes specific motifs, with the second interface being critical for their correct head to tail assembly. The COOH-terminal domain of the protein contains the DNA binding motif essential for the discrimination of this specific functional assembly over competitive nonspecific H-NS polymers.
引用
收藏
页码:41657 / 41666
页数:10
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