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RecA蛋白自组装及其与单链DNA相互作用的动态光散射研究

Dynamic light scattering investigations of RecA self-assembly and interactions with single strand DNA.

作者信息

Benight A S, Wilson D H, Budzynski D M, Goldstein R F

机构信息

Department of Chemistry, University of Illinois, Chicago 60680.

出版信息

Biochimie. 1991 Feb-Mar;73(2-3):143-55. doi: 10.1016/0300-9084(91)90197-9.

Abstract

Dynamic light scattering (DLS) measurements were performed on self-assembled solutions of RecA as a function of assembly time under strand exchange ionic strength conditions (10 mM MgCl2, 65 mM NaCl, 10 mM Tris-HCl, pH = 7.5, 1 mM DTT, 3-4 microM RecA) in the absence of ATP. These measurements yield distributions of the translational diffusion coefficients of the changing populations of assembling protein species. Interpretations of results of DLS measurements are made in terms of model hydrodynamic calculations that indicate, under the solution conditions employed, the smallest fundamental quaternary subunit of RecA is a hexamer in a toroidal or lock-washer configuration. Interactions of M13mp19 circular single strand DNA (ssDNA) with RecA assembled to different stages were also investigated. Additions of ssDNA to self-assembled solutions of RecA acts to dissociate the associated structures into hexamer subunits. However, the effect of ssDNA on assembled RecA is highly dependent on the RecA self-assembly state. The longer the assembly time, the less reversible the self-assembled structures of RecA become. Binding isotherms of titrated mixtures of ssDNA with RecA self-assembled to various stages were also determined. Evaluated dissociation constants of RecA/ssDNA complexes were found to increase with increases of the associated state of RecA. These results strongly suggest that, under the solvent conditions employed, the active ssDNA binding form of RecA is a hexamer.

摘要

在无ATP的情况下,于链交换离子强度条件(10 mM MgCl₂、65 mM NaCl、10 mM Tris-HCl,pH = 7.5、1 mM DTT、3 - 4 μM RecA)下,对RecA的自组装溶液进行了动态光散射(DLS)测量,测量结果为组装时间的函数。这些测量得出了正在组装的蛋白质种类不断变化的群体的平移扩散系数分布。DLS测量结果的解释是基于模型流体动力学计算做出的,该计算表明,在所采用的溶液条件下,RecA最小的基本四级亚基是呈环形或锁垫圈构型的六聚体。还研究了M13mp19环状单链DNA(ssDNA)与组装到不同阶段的RecA之间的相互作用。向RecA的自组装溶液中添加ssDNA会使相关结构解离成六聚体亚基。然而,ssDNA对组装后的RecA的影响高度依赖于RecA的自组装状态。组装时间越长,RecA的自组装结构变得越不可逆。还测定了ssDNA与自组装到不同阶段的RecA的滴定混合物的结合等温线。发现评估的RecA/ssDNA复合物的解离常数随着RecA相关状态的增加而增加。这些结果有力地表明,在所采用的溶剂条件下,RecA的活性ssDNA结合形式是六聚体。

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