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本文引用的文献

1
Fast large-scale purification of tetracycline repressor variants from overproducing Escherichia coli strains.从过量表达的大肠杆菌菌株中快速大规模纯化四环素阻遏物变体
J Chromatogr A. 1996 Aug 23;742(1-2):95-105. doi: 10.1016/0021-9673(96)00232-4.
2
Raman spectroscopy of DNA-metal complexes. I. Interactions and conformational effects of the divalent cations: Mg, Ca, Sr, Ba, Mn, Co, Ni, Cu, Pd, and Cd.DNA-金属络合物的拉曼光谱。I. 二价阳离子:镁、钙、锶、钡、锰、钴、镍、铜、钯和镉的相互作用及构象效应
Biophys J. 1993 Nov;65(5):1916-28. doi: 10.1016/S0006-3495(93)81263-3.
3
Structure of the Tet repressor-tetracycline complex and regulation of antibiotic resistance.四环素阻遏蛋白 - 四环素复合物的结构与抗生素抗性调控
Science. 1994 Apr 15;264(5157):418-20. doi: 10.1126/science.8153629.
4
An altered specificity mutation in the lambda repressor induces global reorganization of the protein-DNA interface.λ阻遏物中的特异性改变突变诱导蛋白质-DNA界面的全局重组。
J Biol Chem. 1994 Apr 8;269(14):10869-78.
5
Secondary structure and interaction of phage D108 Ner repressor with a 61-base-pair operator: evidence for altered protein and DNA structures in the complex.噬菌体D108 Ner阻遏物与一个61碱基对操纵基因的二级结构及相互作用:复合物中蛋白质和DNA结构改变的证据
Biochemistry. 1994 Sep 6;33(35):10701-10. doi: 10.1021/bi00201a018.
6
Proximity probing of Tet repressor to tet operator by dimethylsulfate reveals protected and accessible functions for each recognized base-pair in the major groove.
J Mol Biol. 1995 Feb 3;245(5):538-48. doi: 10.1006/jmbi.1994.0044.
7
Mechanisms underlying expression of Tn10 encoded tetracycline resistance.Tn10编码的四环素抗性表达的潜在机制。
Annu Rev Microbiol. 1994;48:345-69. doi: 10.1146/annurev.mi.48.100194.002021.
8
Proximity mapping of the Tet repressor-tetracycline-Fe2+ complex by hydrogen peroxide mediated protein cleavage.通过过氧化氢介导的蛋白质裂解对四环素阻遏物 - 四环素 - Fe2+ 复合物进行邻近作图。
Biochemistry. 1995 Jan 10;34(1):22-31. doi: 10.1021/bi00001a004.
9
The complex formed between Tet repressor and tetracycline-Mg2+ reveals mechanism of antibiotic resistance.四环素阻遏蛋白与四环素-Mg2+形成的复合物揭示了抗生素耐药机制。
J Mol Biol. 1995 Mar 24;247(2):260-80. doi: 10.1006/jmbi.1994.0138.
10
Spectroscopic investigation of Tet repressor tryptophan-43 upon specific and nonspecific DNA binding.特异性及非特异性DNA结合时Tet阻遏蛋白色氨酸-43的光谱学研究
Biochemistry. 1995 Oct 10;34(40):13007-15. doi: 10.1021/bi00040a011.

通过红外光谱和拉曼光谱研究四环素阻遏物与操纵基因DNA以及与四环素的相互作用。

Interaction of Tet repressor with operator DNA and with tetracycline studied by infrared and Raman spectroscopy.

作者信息

Krafft C, Hinrichs W, Orth P, Saenger W, Welfle H

机构信息

Max-Delbrück-Centrum für Molekulare Medizin, Berlin, Germany.

出版信息

Biophys J. 1998 Jan;74(1):63-71. doi: 10.1016/S0006-3495(98)77767-7.

DOI:10.1016/S0006-3495(98)77767-7
PMID:9449310
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1299362/
Abstract

Tet repressor (TetR) is involved in the most abundant mechanism of tetracycline (Tc) resistance of gram-negative bacteria. Raman spectra were measured for the class D TetR protein, for an oligodeoxyribonucleotide with sequence corresponding to operator site O1, and for the TetR:oligonucleotide complex. TetR forms a complex with [Ni-Tc]+, which does not bind to operator DNA. Raman and infrared measurements indicate nearly identical conformations of TetR with and without [Ni-Tc]+. Differences between the experimental spectrum of the TetR:operator DNA complex and the computed sum of the component spectra provide direct spectroscopic evidence for changes in DNA backbone torsions and base stacking, rearrangement of protein backbone, and specific contacts between TetR residues and DNA bases. Complex formation is connected with intensity decrease at 1376 cm(-1) (participation of thymine methyl groups), intensity increase at 1467 cm(-1) (hydrogen bond formation at guanine N7), decreased intensity ratio I854/I823 (increased hydrophobicity of tyrosine environment), increased intensity at 1363 cm(-1) (increased hydrophobicity of tryptophan ring environment), differences in the range 670-833 cm(-1) (changes in B-DNA backbone torsions and base stacking), and decreased intensity of the amide I band (structural rearrangement of TetR backbone consistent with a reduction of the distance between the two binding helices).

摘要

四环素阻遏蛋白(TetR)参与革兰氏阴性菌对四环素(Tc)耐药的最主要机制。我们测量了D类TetR蛋白、与操纵位点O1序列对应的寡脱氧核糖核苷酸以及TetR:寡核苷酸复合物的拉曼光谱。TetR与[Ni-Tc]+形成复合物,该复合物不与操纵子DNA结合。拉曼光谱和红外光谱测量表明,有无[Ni-Tc]+时TetR的构象几乎相同。TetR:操纵子DNA复合物的实验光谱与各组分光谱计算总和之间的差异,为DNA主链扭转和碱基堆积的变化、蛋白质主链的重排以及TetR残基与DNA碱基之间的特异性接触提供了直接的光谱证据。复合物的形成与1376 cm-1处强度降低(胸腺嘧啶甲基基团的参与)、1467 cm-1处强度增加(鸟嘌呤N7处形成氢键)、强度比I854/I823降低(酪氨酸环境疏水性增加)、1363 cm-1处强度增加(色氨酸环环境疏水性增加)、670 - 833 cm-1范围内的差异(B-DNA主链扭转和碱基堆积的变化)以及酰胺I带强度降低(TetR主链的结构重排与两个结合螺旋之间距离的减小一致)有关。