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使用置换离子法对单价抗衡离子与随机序列双链DNA的结合进行定量分析。

Quantitative analysis of monovalent counterion binding to random-sequence, double-stranded DNA using the replacement ion method.

作者信息

Stellwagen Earle, Dong Qian, Stellwagen Nancy C

机构信息

Department of Biochemistry, University of Iowa, Iowa City, Iowa 52242, USA.

出版信息

Biochemistry. 2007 Feb 20;46(7):2050-8. doi: 10.1021/bi062132w. Epub 2007 Jan 25.

Abstract

A variation of affinity capillary electrophoresis, called the replacement ion (RI) method, has been developed to measure the binding of monovalent cations to random sequence, double-stranded (ds) DNA. In this method, the ionic strength is kept constant by gradually replacing a non-binding ion in the solution with a binding ion and measuring the mobility of binding and non-binding analytes as a function of binding ion concentration. The method was validated by measuring the binding of Li+ ions to adenosine nucleotides; the apparent dissociation constants obtained by the RI method are comparable to literature values obtained by other methods. The binding of Tris+, NH4+, Li+, Na+, and K+ to dsDNA was then investigated. The apparent dissociation constants observed for counterion binding to a random-sequence 26-base pair (bp) oligomer ranged from 71 mM for Tris+ to 173 mM for Na+ and K+. Hence, positively charged Tris buffer ions will compete with other monovalent cations in Tris-buffered solutions. The bound cations identified in this study may correspond to the strongly correlated, tightly bound ions recently postulated to exist as a class of ions near the surface of dsDNA (Tan, Z.-J., and Chen, S.-J. (2006) Biophys. J. 91, 518-536). Monovalent cation binding to random-sequence dsDNA would be expected to occur in addition to any site-specific binding of cations to A-tracts or other DNA sequence motifs. Single-stranded DNA oligomers do not bind the five tested cations under the conditions investigated here.

摘要

一种称为置换离子(RI)法的亲和毛细管电泳变体已被开发出来,用于测量单价阳离子与随机序列双链(ds)DNA的结合。在该方法中,通过用结合离子逐渐替代溶液中的非结合离子并测量结合和非结合分析物的迁移率作为结合离子浓度的函数,使离子强度保持恒定。该方法通过测量Li⁺离子与腺苷核苷酸的结合进行了验证;通过RI法获得的表观解离常数与通过其他方法获得的文献值相当。然后研究了Tris⁺、NH₄⁺、Li⁺、Na⁺和K⁺与dsDNA的结合。观察到的反离子与随机序列26碱基对(bp)寡聚物结合的表观解离常数范围从Tris⁺的71 mM到Na⁺和K⁺的173 mM。因此,带正电的Tris缓冲离子将在Tris缓冲溶液中与其他单价阳离子竞争。本研究中鉴定出的结合阳离子可能对应于最近推测存在于dsDNA表面附近的一类离子,即强相关、紧密结合的离子(Tan,Z.-J.,和Chen,S.-J.(2006)《生物物理杂志》91,518 - 536)。除了阳离子与A序列或其他DNA序列基序的任何位点特异性结合外,预计单价阳离子还会与随机序列dsDNA结合。在这里研究的条件下,单链DNA寡聚物不结合所测试的五种阳离子。

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