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SELEX条件对筛选与细菌细胞结合的适体过程中所得适体库的影响。

The Effects of SELEX Conditions on the Resultant Aptamer Pools in the Selection of Aptamers Binding to Bacterial Cells.

作者信息

Hamula Camille L A, Peng Hanyong, Wang Zhixin, Newbigging Ashley M, Tyrrell Gregory J, Li Xing-Fang, Le X Chris

机构信息

Division of Analytical and Environmental Toxicology, Department of Laboratory Medicine and Pathology, Faculty of Medicine and Dentistry, University of Alberta, 10-102 Clinical Sciences Building, Edmonton, AB, T6G 2G3, Canada.

Mount Sinai Hospital, Icahn School of Medicine at Mount Sinai, 1425 Madison Avenue, New York City, NY, 10029, USA.

出版信息

J Mol Evol. 2015 Dec;81(5-6):194-209. doi: 10.1007/s00239-015-9711-y. Epub 2015 Nov 4.

Abstract

Aptamers of high affinity and specificity have a wide range of analytic and clinical applications. Selection of DNA or RNA aptamer molecules usually involves systematic evolution of ligands via exponential enrichment (SELEX), in which a random DNA or RNA library is incubated with a target molecule, and the oligonucleotides that bind the target are then separated from the nonbinders, PCR amplified, and used as refined libraries in the next round of selection. Conventional SELEX methodologies require the use of purified target molecules and their immobilization onto a solid support. However, purified targets from cells are not always available, and fixing the target to a support may alter its conformation. To overcome these problems, we have developed a SELEX technique using live bacterial cells in suspension as targets, for selecting DNA aptamers specific to cell-surface molecules. Through the selection of aptamers binding to Lactobacillus acidophilus and Streptococcus pyogenes, we report here optimization of this technique and show how varying selection conditions impact the characteristics of resultant aptamer pools, including the binding affinity, selectivity, and the secondary structures. We found that the use of larger starting library sequence diversity, gel purification of the subsequent pools, and the introduction of counter-selection resulted in a more efficient SELEX process and more selective aptamers. A SELEX protocol with lower starting sequence diversity, the use of heat denaturation, and the absence of counter-selection still resulted in high-affinity aptamer sequences specific to the target cell types; however, the SELEX process was inefficient, requiring 20 rounds, and the aptamers were not specific to the strain of the bacterial cells. Strikingly, two different SELEX methodologies yielded the same sequence that bound strongly to the target S. pyogenes cells, suggesting the robustness of the bacterial cell-SELEX technique.

摘要

高亲和力和特异性的适配体具有广泛的分析和临床应用。DNA或RNA适配体分子的筛选通常涉及通过指数富集系统进化技术(SELEX),即将一个随机的DNA或RNA文库与目标分子一起孵育,然后将与目标结合的寡核苷酸与未结合的寡核苷酸分离,进行PCR扩增,并用作下一轮筛选的优化文库。传统的SELEX方法需要使用纯化的目标分子并将其固定在固体支持物上。然而,并非总能从细胞中获得纯化的目标分子,并且将目标固定在支持物上可能会改变其构象。为了克服这些问题,我们开发了一种以悬浮状态的活细菌细胞为目标的SELEX技术,用于筛选细胞表面分子特异性的DNA适配体。通过筛选与嗜酸乳杆菌和化脓性链球菌结合的适配体,我们在此报告了该技术的优化,并展示了不同的筛选条件如何影响所得适配体库的特性,包括结合亲和力、选择性和二级结构。我们发现,使用更大的起始文库序列多样性、对后续文库进行凝胶纯化以及引入反筛选可导致更有效的SELEX过程和更具选择性的适配体。起始序列多样性较低、使用热变性且不存在反筛选的SELEX方案仍可产生对目标细胞类型具有高亲和力的适配体序列;然而,SELEX过程效率低下,需要20轮,并且适配体对细菌细胞的菌株不具有特异性。引人注目的是,两种不同的SELEX方法产生了与目标化脓性链球菌细胞强烈结合的相同序列,这表明细菌细胞SELEX技术的稳健性。

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