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High-resolution AFM imaging of single-stranded DNA-binding (SSB) protein-DNA complexes

机译:单链DNA结合(SSB)蛋白-DNA复合物的高分辨率AFM成像

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DNA in living cells is generally processed via the generation and the protection of single-stranded DNA involving the binding of ssDNA-binding proteins (SSBs). The studies of SSB-binding mode transition and cooperativity are therefore critical to many cellular processes like DNA repair and replication. However, only a few atomic force microscopy (AFM) investigations of ssDNA nucleoprotein filaments have been conducted so far. The point is that adsorption of ssDN A-SSB complexes on mica, necessary for AFM imaging, is not an easy task. Here, we addressed this issue by using spermidine as a binding agent. This trivalent cation induces a stronger adsorption on mica than divalent cations, which are commonly used by AFM users but are ineffective in the adsorption of ssDNA-SSB complexes. At low spermidine concentration (50.3 mM), we obtained AFM images of ssDNA-SSB complexes (E. coli SSB, gp32 and yRPA) on mica at both low and high ionic strengths. In addition, partially or fully saturated nucleoprotein filaments were studied at various monovalent salt concentrations thus allowing the observation of SSB-binding mode transition. In association with conventional biochemical techniques, this work should make it possible to study the dynamics of DNA processes involving DNA-SSB complexes as intermediates by AFM.
机译:活细胞中的DNA通常通过涉及ssDNA结合蛋白(SSBs)结合的单链DNA的产生和保护来加工。因此,对SSB结合模式转变和协同作用的研究对于许多细胞过程(如DNA修复和复制)至关重要。然而,到目前为止,仅对ssDNA核蛋白丝进行了原子力显微镜(AFM)研究。关键是,对于AFM成像而言,在云母上吸附ssDN A-SSB复合物并非易事。在这里,我们通过使用亚精胺作为粘合剂解决了这个问题。这种三价阳离子比二价阳离子对云母的吸附更强,二价阳离子是AFM用户常用的,但对ssDNA-SSB复合物的吸附无效。在低亚精胺浓度(50.3 mM)下,我们在低离子强度和高离子强度下都获得了云母上ssDNA-SSB复合物(大肠杆菌SSB,gp32和yRPA)的AFM图像。另外,在各种单价盐浓度下研究了部分或完全饱和的核蛋白丝,因此可以观察到SSB结合模式的转变。与传统的生化技术相结合,这项工作将有可能研究涉及AFM的DNA-SSB复合物作为中间体的DNA过程的动力学。

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