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低pH诱导的多线染色体DNA结构变化的拉曼显微光谱研究

Raman microspectroscopic study of low-pH-induced changes in DNA structure of polytene chromosomes.

作者信息

Puppels G J, Otto C, Greve J, Robert-Nicoud M, Arndt-Jovin D J, Jovin T M

机构信息

Department of Applied Physics, University of Twente, AE Enschede, The Netherlands.

出版信息

Biochemistry. 1994 Mar 22;33(11):3386-95. doi: 10.1021/bi00177a032.

Abstract

The effects of low-pH treatments on DNA structure in polytene chromosomes of Chironomus thummi thummi have been studied by Raman microspectroscopy. Measurements were carried out on chromosomes at low pH and on chromosomes reneutralized after a short exposure to low pH. Protonation of adenine residues and subsequent unpairing of adenine (A) and thymine (T) were found to commence already above pH 3.6 and are completed at pH 2.2. Protonation of the cytosine-guanine base pair also starts above pH 3.6. It leads to an intermediate protonated, most likely Hoogsteen-type, guanine-cytosine base pair. Unpairing of G and C residues starts between pH 2.6 and 2.2 and continues below pH 2.2. Brief treatment of chromosomes at a pH < or = 2.2, i.e., at a pH where both AT and GC base pairs are disrupted, was found to lead to irreversible changes in DNA conformation upon return to neutral pH. These were most pronounced after treatment with 45% acetic acid. More than 10% of the A and T residues was found to have adopted a non-B-DNA conformation. Evidence was found for denaturation of the B-form backbone. The amount of protein extracted from the chromosomes was strongly pH-dependent. Treatment at pH 3.6 did not cause noticeable protein extraction, while treatment with 45% acetic acid extracted more than 50% (by weight) of the chromosomal proteins.

摘要

通过拉曼光谱研究了低pH处理对嗜尸摇蚊多线染色体中DNA结构的影响。对处于低pH值的染色体以及短暂暴露于低pH值后再恢复中性pH值的染色体进行了测量。发现腺嘌呤残基的质子化以及随后腺嘌呤(A)和胸腺嘧啶(T)的解配对在pH值高于3.6时就已开始,并在pH值为2.2时完成。胞嘧啶-鸟嘌呤碱基对的质子化也在pH值高于3.6时开始。它导致形成一种中间质子化的、很可能是Hoogsteen型的鸟嘌呤-胞嘧啶碱基对。G和C残基的解配对在pH值2.6至2.2之间开始,并在pH值低于2.2时继续。发现染色体在pH≤2.2(即AT和GC碱基对均被破坏的pH值)下短暂处理后,恢复到中性pH值时会导致DNA构象发生不可逆变化。在用45%乙酸处理后这种变化最为明显。发现超过10%的A和T残基呈现出非B-DNA构象。有证据表明B型主链发生了变性。从染色体中提取的蛋白质量强烈依赖于pH值。在pH值3.6下处理不会导致明显的蛋白提取,而用45%乙酸处理则提取了超过50%(按重量计)的染色体蛋白。

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