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DNA-组蛋白复合物的结构研究。一项自旋标记研究。

Structural investigations of DNA-histone complexes. A spin label study.

作者信息

Sinha B K, Chignell C F, Wee V T

出版信息

Nucleic Acids Res. 1979 Aug 10;6(11):3703-13. doi: 10.1093/nar/6.11.3703.

Abstract

We have prepared two acridine spin labels, 6-chloro-9-[4-(2,2,6,6-tetramethyl-1-piperidinyloxy)amino]-2-methoxyacridine (I) and 9-[4-(2,2,6,6-tetramethyl-1-piperidinyloxy)amino]-acridine (II) and have used them to study the binding of lysine-rich histone (H1) to DNA using electron spin resonance (ESR). ESR spectra of I in the presence of DNA, polydA-polydT and polydG-polydC were characteristic of highly immobilized radicals with maximum hyperfine splitting (2T11) of 59G, 62.5G and 59G respectively. However, the 2T11 values for II in the same systems were 55.5G, 55.5G and 62.5G respectively. Addition of H1 at a low P/D released ionically bound I and II from DNA. In the presence of 0.1 M NaCl, which prevents ionic binding, H1 still caused a significant release of bound II but not I from DNA. At a high P/D (with or without NaCl) H1 caused no displacement of either I or II. Our findings suggest that H1 does not affect the intercalating sites and probably binds to one of the grooves of DNA, most probably the major groove, and specifically in the A-T-rich regions.

摘要

我们制备了两种吖啶自旋标记物,6-氯-9-[4-(2,2,6,6-四甲基-1-哌啶氧基)氨基]-2-甲氧基吖啶(I)和9-[4-(2,2,6,6-四甲基-1-哌啶氧基)氨基]吖啶(II),并使用它们通过电子自旋共振(ESR)研究富含赖氨酸的组蛋白(H1)与DNA的结合。在DNA、聚dA-聚dT和聚dG-聚dC存在下,I的ESR光谱具有高度固定化自由基的特征,最大超精细分裂(2T11)分别为59G、62.5G和59G。然而,在相同体系中II的2T11值分别为55.5G、55.5G和62.5G。在低P/D下添加H1会使离子结合的I和II从DNA上释放出来。在0.1M NaCl存在下(可防止离子结合),H1仍会导致结合的II从DNA上显著释放,但不会导致I释放。在高P/D(有或无NaCl)下,H1不会使I或II发生位移。我们的研究结果表明,H1不会影响嵌入位点,可能与DNA的一个沟槽结合,很可能是大沟槽,并且特别结合在富含A-T的区域。

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本文引用的文献

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A model for particulate structure in chromatin.染色质中颗粒结构的模型。
Nucleic Acids Res. 1974 Nov;1(11):1579-86. doi: 10.1093/nar/1.11.1579.
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Physics and chemistry of spin labels.自旋标记物的物理与化学
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Science. 1974 May 24;184(4139):868-71. doi: 10.1126/science.184.4139.868.
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Aflatoxin B1 and actinomycin D effects on histone: acetylation and deacetylation in the liver.
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