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发夹状核酶的折叠:对环和连接区的依赖性。

The folding of the hairpin ribozyme: dependence on the loops and the junction.

作者信息

Zhao Z Y, Wilson T J, Maxwell K, Lilley D M

机构信息

Department of Biochemistry, The University of Dundee, United Kingdom.

出版信息

RNA. 2000 Dec;6(12):1833-46. doi: 10.1017/s1355838200001230.

Abstract

In its natural context, the hairpin ribozyme is constructed around a four-way helical junction. This presents the two loops that interact to form the active site on adjacent arms, requiring rotation into an antiparallel structure to bring them into proximity. In the present study we have compared the folding of this form of the ribozyme and subspecies lacking either the loops or the helical junction using fluorescence resonance energy transfer. The complete ribozyme as a four-way junction folds into an antiparallel structure by the cooperative binding of magnesium ions, requiring 20-40 microM for half-maximal extent of folding ([Mg2+]1/2) and a Hill coefficient n = 2. The isolated junction (lacking the loops) also folds into a corresponding antiparallel structure, but does so noncooperatively (n = 1) at a higher magnesium ion concentration ([Mg2+]1/2 = 3 mM). Introduction of a G + 1A mutation into loop A of the ribozyme results in a species with very similar folding to the simple junction, and complete loss of ribozyme activity. Removal of the junction from the ribozyme, replacing it either with a strand break (serving as a hinge) or a GC5 bulge, results in greatly impaired folding, with [Mg2+]1/2 > 20 mM. The results indicate that the natural form of the ribozyme undergoes ion-induced folding by the cooperative formation of an antiparallel junction and loop-loop interaction to generate the active form of the ribozyme. The four-way junction thus provides a scaffold in the natural RNA that facilitates the folding of the ribozyme into the active form.

摘要

在自然环境中,发夹状核酶围绕着一个四链螺旋连接结构构建而成。这使得两个环相互作用,在相邻臂上形成活性位点,需要旋转成反平行结构才能使它们靠近。在本研究中,我们使用荧光共振能量转移比较了这种形式的核酶与缺少环或螺旋连接结构的亚种的折叠情况。作为四链连接结构的完整核酶通过镁离子的协同结合折叠成反平行结构,折叠达到最大程度的一半时需要20 - 40微摩尔的镁离子浓度([Mg2+]1/2),希尔系数n = 2。分离出的连接结构(缺少环)也折叠成相应的反平行结构,但在较高的镁离子浓度下([Mg2+]1/2 = 3毫摩尔)以非协同方式进行(n = 1)。在核酶的环A中引入G + 1A突变会产生一种折叠情况与简单连接结构非常相似的物种,并且核酶活性完全丧失。从核酶中去除连接结构,用链断裂(作为铰链)或GC5凸起取代它,会导致折叠严重受损,[Mg2+]1/2 > 20毫摩尔。结果表明,核酶的天然形式通过反平行连接结构的协同形成和环 - 环相互作用进行离子诱导折叠,从而产生核酶的活性形式。因此,四链连接结构在天然RNA中提供了一个支架,有助于核酶折叠成活性形式。

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