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利用 3’-反向去氧胸苷进行 TBA 环映射,以精细调整对 α-凝血酶的结合亲和力。

TBA loop mapping with 3'-inverted-deoxythymidine for fine-tuning of the binding affinity for α-thrombin.

机构信息

School of Pharmaceutical Sciences, Guizhou University, Guizhou 550025, China.

出版信息

Org Biomol Chem. 2019 Feb 27;17(9):2403-2412. doi: 10.1039/c9ob00053d.

Abstract

TBA is a 15-mer DNA aptamer for human α-thrombin, and its three T-rich loops are involved in the binding interactions with thrombin differently. In order to clarify their specific spatial locations in the binding interactions and search for more favourable positions, here a systematic investigation of all the loop residues was conducted with 3'-inverted thymidine (iT), by which both unnatural 3'-3'- and 5'-5'-linkages for each incorporation were introduced in the tertiary structure. The changes in Tm values and CD spectra revealed that motifs T3T12 and T4T13 are structurally distinct. Longer anti-clotting time was obtained for the T3 and T12 modifications, respectively, while T4 and T13 were completely intolerant with such changes, in terms of stability and binding to thrombin. In particular, the increased affinity bindings and longer anti-clotting time were obtained with the replacement on the central loop T7G8T9, which were closely related to the existence of a monovalent ion, K+ or Na+, consistently with the supposed binding site of these ions in TBA. It is worthwhile to note that both the subtle variations of the loop residues induced by iT and the monovalent ions determined the interacting residues of TBA and the binding strength rather than the thermal stability of the TBA structure.

摘要

TBA 是一种针对人凝血酶的 15 -mer DNA 适体,其三个富含 T 的环以不同的方式参与与凝血酶的结合相互作用。为了阐明它们在结合相互作用中的特定空间位置,并寻找更有利的位置,在这里通过引入 3'- 反转胸腺嘧啶核苷(iT)对所有环残基进行了系统研究,从而在三级结构中引入了每个掺入物的非天然 3'-3'- 和 5'-5'- 键。Tm 值和 CD 光谱的变化表明,T3T12 和 T4T13 基序在结构上是不同的。T3 和 T12 的修饰分别导致更长的抗凝血时间,而 T4 和 T13 对这些变化完全不能容忍,无论是在稳定性还是与凝血酶的结合方面。特别是,用中心环 T7G8T9 的替换获得了结合亲和力的增加和更长的抗凝血时间,这与假定的 TBA 中这些离子的结合位点密切相关。值得注意的是,iT 诱导的环残基的细微变化和单价离子决定了 TBA 的相互作用残基和结合强度,而不是 TBA 结构的热稳定性。

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