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对特定限制性内切酶-DNA复合物形成的独特31P光谱响应。

Unique 31P spectral response to the formation of a specific restriction enzyme-DNA complex.

作者信息

Dupureur Cynthia M

机构信息

Department of Chemistry and Biochemistry, One University Blvd., University of Missouri-St. Louis, St. Louis, MO 63121, USA.

出版信息

Nucleosides Nucleotides Nucleic Acids. 2006;25(7):747-64. doi: 10.1080/15257770600725978.

Abstract

Protein-induced distortion is a dramatic but not universally observed feature of sequence-specific DNA interactions. This is illustrated by the crystal structures of restriction enzyme-DNA complexes: While some of these structures exhibit DNA distortion, others do not. Among the latter is Pvull endonuclease, a small enzyme that is also amenable to NMR spectroscopic studies. Here 31P NMR spectroscopy is applied to demonstrate the unique spectral response of DNA to sequence-specific protein interactions. The 31P NMR spectrum of a noncognate DNA exhibits only spectral broadening upon the addition of enzyme. However, when enzyme is added to target DNA, a number of 31P resonances shift dramatically. The magnitudes of the chemical shifts (2-3 ppm) are among the largest observed. Site-specific substitution with phosphoramidates and phosphorothioates are used analyze these effects. While such spectral features have been interpreted as indicative of DNA backbone distortions, FRET analysis indicates that this does not occur in PvuII-cognate DNA complexes in solution. The distinct 31P spectral signature observed for cognate DNA mirrors that observed for the enzyme, underscoring the unique features of cognate complex formation.

摘要

蛋白质诱导的畸变是序列特异性DNA相互作用中一个显著但并非普遍观察到的特征。限制性内切酶-DNA复合物的晶体结构说明了这一点:虽然其中一些结构表现出DNA畸变,但其他结构则没有。后者包括PvuII核酸内切酶,这是一种小型酶,也适用于核磁共振光谱研究。在此,应用31P核磁共振光谱来证明DNA对序列特异性蛋白质相互作用的独特光谱响应。非同源DNA的31P核磁共振谱在加入酶后仅表现出光谱展宽。然而,当将酶加入到靶DNA中时,一些31P共振会发生显著位移。化学位移的幅度(2-3 ppm)是观察到的最大幅度之一。使用氨基磷酸酯和硫代磷酸酯进行位点特异性取代来分析这些效应。虽然这种光谱特征被解释为表明DNA主链畸变,但荧光共振能量转移分析表明,在溶液中的PvuII同源DNA复合物中不会发生这种情况。同源DNA观察到的独特31P光谱特征与酶观察到的特征相似,突出了同源复合物形成的独特特征。

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