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哺乳动物异质核糖核蛋白A1及其组成结构域。核酸相互作用、结构稳定性和自我缔合。

Mammalian heterogeneous ribonucleoprotein A1 and its constituent domains. Nucleic acid interaction, structural stability and self-association.

作者信息

Casas-Finet J R, Smith J D, Kumar A, Kim J G, Wilson S H, Karpel R L

机构信息

Department of Chemistry and Biochemistry, University of Maryland Baltimore County 21228.

出版信息

J Mol Biol. 1993 Feb 20;229(4):873-89. doi: 10.1006/jmbi.1993.1093.

DOI:10.1006/jmbi.1993.1093
PMID:8445653
Abstract

With a view toward further understanding the structure-function relationships of the eukaryotic heterogeneous ribonucleoprotein (hnRNP) A1, and in particular its multiplicity of nucleic acid-interactive domains, we have studied the nucleic acid binding properties of the globular N-domain (UP1) and sequence-repetitive, flexible C-domain, the thermal denaturation of UP1 and the concomitant effects of binding polynucleotide, and the self-associative properties of the full-length protein. Utilizing protein tryptophan fluorescence as a probe, polynucleotide binding was shown to stabilize UP1 against thermal unfolding. The denaturation profile of UP1-poly(thymidylic acid) complexes was biphasic, suggesting that unfolding of the two subdomains of UP1 can occur independently. This is in agreement with a previously proposed structure in which only one of the two UP1 subdomains binds the nucleic acid. The subdomains of UP1 can be prepared by controlled proteolysis of A1, further indicating that these two globular segments within A1 are connected by an exposed, flexible linkage. Circular dichroism measurements on UP1 confirm previous data that this portion of A1 binds single-stranded nucleic acids non-co-operatively. UP1 clearly shows a preference for single-stranded nucleic acids with a 2'-OH, since its affinity for poly(U) is three times higher than for poly(dU), and five times higher than its affinity for poly(2'-OCH3U). The nucleic acid-interactive properties of the C-domain were further examined by preparing a synthetic peptide polymer (M(r) approximately 12,000) containing about seven repeats of a 16-residue sequence, GNFGGGRGGNYGGSRG, which in turn comprises two copies of the C-terminal consensus, GN(F/Y)GG(G/S)RG. The polymer of this sequence exhibited significant affinity for the fluorescent polyribonucleotide, poly(ethenoadenylic acid), binding stoichiometrically at < or = 0.2 M-Na+. Complex formation was accompanied by an increase in aggregate formation, as indicated by the appearance of scattering. For purposes of comparison, the data were analyzed via the linear co-operative model of McGhee and von Hippel, though this model may not be fully descriptive of the protein-nucleic acid complex(es) formed in this case. In contrast to the non-co-operative binding mode of the UP1 domain, the C-polymer exhibited moderate co-operativity, comparable to that seen with full-length A1. Although addition of sufficient NaCl reversed the interaction, a sigmoidal binding isotherm could still be observed (with sufficient added polymer) at 0.8 M-NaCl. This suggests that non-electrostatic interactions contribute significantly to the free energy of binding.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

为了进一步了解真核生物异质性核糖核蛋白(hnRNP)A1的结构-功能关系,特别是其多个核酸相互作用结构域,我们研究了球状N结构域(UP1)和序列重复、柔性C结构域的核酸结合特性、UP1的热变性以及结合多核苷酸的伴随效应,以及全长蛋白的自缔合特性。利用蛋白质色氨酸荧光作为探针,结果表明多核苷酸结合可稳定UP1使其免于热解折叠。UP1-聚(胸苷酸)复合物的变性曲线是双相的,这表明UP1的两个亚结构域的解折叠可以独立发生。这与先前提出的结构一致,即UP1的两个亚结构域中只有一个与核酸结合。UP1的亚结构域可以通过对A1进行可控的蛋白酶解来制备,这进一步表明A1内的这两个球状片段通过一个暴露的柔性连接相连。对UP1的圆二色性测量证实了先前的数据,即A1的这部分与单链核酸的结合是非协同性的。UP1明显表现出对具有2'-OH的单链核酸的偏好,因为它对聚(U)的亲和力比对聚(dU)高3倍,比对聚(2'-OCH3U)的亲和力高5倍。通过制备一种合成肽聚合物(相对分子质量约为12,000)来进一步研究C结构域的核酸相互作用特性,该聚合物包含约七个16个残基序列GNFGGGRGGNYGGSRG的重复序列,该序列又包含两个C末端共有序列GN(F/Y)GG(G/S)RG的拷贝。该序列的聚合物对荧光聚核糖核苷酸聚(乙烯腺苷酸)表现出显著的亲和力,在≤0.2M-Na+时以化学计量方式结合。复合物的形成伴随着聚集体形成的增加,这通过散射的出现得以表明。为了进行比较,数据通过McGhee和von Hippel的线性协同模型进行分析,尽管该模型可能不能完全描述在这种情况下形成的蛋白质-核酸复合物。与UP1结构域的非协同结合模式相反,C聚合物表现出适度的协同性,与全长A1的情况相当。尽管加入足够的NaCl会逆转这种相互作用,但在0.8M-NaCl时(加入足够的聚合物)仍可观察到S形结合等温线。这表明非静电相互作用对结合自由能有显著贡献。(摘要截短于400字)

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