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小牛胸腺解旋蛋白与核酸相互作用的物理学研究。

Physical studies of the interaction of a calf thymus helix-destablizing protein with nucleic acids.

作者信息

Karpel R L, Burchard A C

出版信息

Biochemistry. 1980 Sep 30;19(20):4674-82. doi: 10.1021/bi00561a021.

DOI:10.1021/bi00561a021
PMID:6252954
Abstract

UP1, a calf thymus protein that destabilizes both DNA and RNA helices, dramatically accelerates the conversion of the inactive conformers of several small RNA molecules to their biologically active forms [Karpel, R. L., Swistel, D. G., Miller, N. S., Geroch, M. E., Lu, C., & Fresco, J. R. (1974) Brookhaven Symp. Biol. 26, 165-174]. Using circular dichroic and spectrophotometric methods, we have studied the interaction of this protein with a variety of synthetic polynucleotides and yeast tRNA3Leu. As judged by perturbations in polynucleotide ellipticity or ultraviolet absorbance, the secondary structures of the single-stranded helices poly(A) and poly(C), as well as the double-stranded helices poly[d(A-T)] and poly(U.U), are largely destroyed upon interaction with UP1 at low ionic strength. This effect can be reversed by an increase in [Na+]: half the UP1-induced perturbation of the poly(A) CD spectrum is removed at 0.05 M Na+. The variation of poly(A) ellipticity and ultraviolet absorbance with [UP1]/[poly(A)]p is used to determine the length of single-stranded polynucleotide chain covered by the protein: 7 +/- 1 residues. A model is presented in which the specificity of UP1 for single strands and their concomitant distortion are a consequence of maximal binding of nucleic acid phosphates to a unique matrix of basic residues on the protein. Analogous to the effect on polynucleotides, UP1-facilitated renaturation of yeast tRNA3Leu follows the partial destruction of the inactive tRNA's secondary structure. At the tRNA absorbance maximum, UP1 effects a hyperchromic change of 10%, representing one-third of the secondary structure of the inactive conformer. This change is also clearly observable as a perturbation of the tRNA's circular dichroism spectrum.

摘要

UP1是一种能使DNA和RNA螺旋结构不稳定的小牛胸腺蛋白,它能显著加速几种小RNA分子的无活性构象向生物活性形式的转变[卡尔佩尔,R.L.,斯威斯特尔,D.G.,米勒,N.S.,杰罗奇,M.E.,卢,C.,&弗雷斯科,J.R.(1974年)《布鲁克海文生物学研讨会论文集》26卷,165 - 174页]。我们使用圆二色性和分光光度法研究了这种蛋白质与多种合成多核苷酸以及酵母tRNA3Leu的相互作用。根据多核苷酸椭圆率或紫外吸收的扰动判断,在低离子强度下,单链螺旋多聚腺苷酸(poly(A))和多聚胞苷酸(poly(C))以及双链螺旋多聚[d(A - T)]和聚(U.U)的二级结构在与UP1相互作用时大部分被破坏。这种效应可通过增加[Na⁺]来逆转:在0.05 M Na⁺时,UP1引起的多聚腺苷酸圆二色性光谱扰动的一半被消除。多聚腺苷酸椭圆率和紫外吸收随[UP1]/[多聚腺苷酸]p的变化用于确定被蛋白质覆盖的单链多核苷酸链的长度:7 ± 1个残基。提出了一个模型,其中UP1对单链的特异性及其伴随的扭曲是核酸磷酸基团与蛋白质上独特的碱性残基基质最大程度结合的结果。与对多核苷酸的作用类似;UP1促进酵母tRNA3Leu复性的过程伴随着无活性tRNA二级结构的部分破坏。在tRNA吸收最大值处,UP1引起10%的增色变化,代表无活性构象二级结构的三分之一。这种变化也可作为tRNA圆二色性光谱扰动清晰地观察到。

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