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化学探针识别的超螺旋和线性化质粒的同型嘌呤-同型嘧啶区域中异常的质子化结构。

Unusual protonated structure in the homopurine.homopyrimidine tract of supercoiled and linearized plasmids recognized by chemical probes.

作者信息

Vojtisková M, Palecek E

机构信息

Institute of Biophysics Czechoslovak Academy of Sciences, Brno.

出版信息

J Biomol Struct Dyn. 1987 Oct;5(2):283-96. doi: 10.1080/07391102.1987.10506394.

DOI:10.1080/07391102.1987.10506394
PMID:2856029
Abstract

Plasmid pEJ4, which is a derivative of pUC19 containing an insert with 60-bp-long homopurine.homopyrimidine tract from sea urchin P. miliaris histone gene spacer, was studied by chemical probes of the DNA structure osmium tetroxide and glyoxal. The former probe reacts with pyrimidine bases, while the latter forms a stable product only with guanine residues. These probes can thus be applied as specific probes for the homopyrimidine and homopurine strands, respectively. At pH 6.0 the site-specific modification of the homopurine.homopyrimidine tract by both probes was observed at native superhelical density of the plasmid. In the linear plasmid under the same conditions this modification was absent; it appeared, however, at more acid pH values. In supercoiled DNA the hypersensitivity of the homopurine.homopyrimidine tract to osmium tetroxide did not substantially change when pH was decreased from 6.0 to 4.0. Changes in NaCl concentration at pH 4.5 did not influence the hypersensitivity to osmium tetroxide; at pH 6.0 this hypersensitivity decreased with increasing NaCl concentration. These results thus show that the chemical probes recognize an unusual protonated structure containing unpaired bases or non-Watson-Crick base pairs. At pH 5.6 the site-specific modification occurred at or near to the middle of the homopurine.homopyrimidine tract, suggesting that a hairpin may be involved in the unusual structure under the given conditions. From the models suggested so far for the unusual structure of homopurine.homopyrimidine tracts our results fit best the protonated triplex H form suggest by V.I. Lyamichev, S.M. Mirkin and M.D. Frank-Kamenetskii, J. Biomol. Struct. Dyn. 3,667 (1986).

摘要

质粒pEJ4是pUC19的衍生物,其含有来自海胆粗点海胆组蛋白基因间隔区的60个碱基对长的同型嘌呤-同型嘧啶序列的插入片段,通过四氧化锇和乙二醛对DNA结构进行化学探针研究。前一种探针与嘧啶碱基反应,而后一种仅与鸟嘌呤残基形成稳定产物。因此,这些探针可分别用作同型嘧啶链和同型嘌呤链的特异性探针。在pH 6.0时,在质粒的天然超螺旋密度下观察到两种探针均对同型嘌呤-同型嘧啶序列进行位点特异性修饰。在相同条件下,线性质粒中不存在这种修饰;然而,在更酸性的pH值下会出现这种修饰。在超螺旋DNA中,当pH从6.0降至4.0时,同型嘌呤-同型嘧啶序列对四氧化锇的超敏性没有实质性变化。在pH 4.5时NaCl浓度的变化不影响对四氧化锇的超敏性;在pH 6.0时,这种超敏性随NaCl浓度的增加而降低。因此,这些结果表明化学探针识别出一种含有未配对碱基或非沃森-克里克碱基对的异常质子化结构。在pH 5.6时,位点特异性修饰发生在同型嘌呤-同型嘧啶序列的中部或附近,这表明在给定条件下可能存在发夹结构参与异常结构。从目前提出的同型嘌呤-同型嘧啶序列异常结构的模型来看,我们的结果最符合V.I.利亚米切夫、S.M.米尔金和M.D.弗兰克-卡门涅茨基在《生物分子结构与动力学杂志》3,667(1986年)中提出的质子化三链体H形式。

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