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重新设计适体以支持无试剂、自我报告的电化学传感器。

Re-engineering aptamers to support reagentless, self-reporting electrochemical sensors.

机构信息

Department of Chemistry and Biochemistry, University of California, Santa Barbara, Santa Barbara, CA 93106, USA.

出版信息

Analyst. 2010 Mar;135(3):589-94. doi: 10.1039/b921253a. Epub 2010 Jan 12.

Abstract

Electrochemical aptamer-based (E-AB) sensors have emerged as a promising and versatile new biosensor platform. Combining the generality and specificity of aptamer-ligand interactions with the selectivity and convenience of electrochemical readouts, this approach affords the detection of a wide variety of targets directly in complex, contaminant-ridden samples, such as whole blood, foodstuffs and crude soil extracts, without the need for exogenous reagents or washing steps. Signaling in this class of sensors is predicated on target-induced changes in the conformation of an electrode-bound probe aptamer that, in turn, changes the efficiency with which a covalently attached redox tag exchanges electrons with the interrogating electrode. Aptamer selection strategies, however, typically do not select for the conformation-switching architectures, and as such several approaches have been reported to date by which aptamers can be re-engineered such that they undergo the binding-induced switching required to support efficient E-AB signaling. Here, we systematically compare the merits of these re-engineering approaches using representative aptamers specific to the small molecule adenosine triphosphate and the protein human immunoglobulin E. We find that, while many aptamer architectures support E-AB signaling, the observed signal gain (relative change in signal upon target binding) varies by more than two orders of magnitude across the various constructs we have investigated (e.g., ranging from -10% to 200% for our ATP sensors). Optimization of the switching architecture is thus an important element in achieving maximum E-AB signal gain and we find that this optimal geometry is specific to the aptamer sequence upon which the sensor is built.

摘要

电化学适体传感器(E-AB)作为一种有前途且多功能的新型生物传感器平台已经出现。将适体-配体相互作用的通用性和特异性与电化学读出的选择性和便利性相结合,这种方法可以直接在复杂的、受污染的样品(如全血、食品和粗土提取物)中检测到各种各样的目标,而无需外源性试剂或洗涤步骤。这类传感器的信号是基于电极结合探针适体的构象变化,这种构象变化反过来又改变了共价连接的氧化还原标记与检测电极之间电子交换的效率。然而,适体选择策略通常不会选择构象转换结构,因此迄今为止已经报道了几种方法,可以对适体进行重新设计,使其经历结合诱导的转换,以支持有效的 E-AB 信号。在这里,我们使用针对小分子三磷酸腺苷和蛋白质人免疫球蛋白 E 的代表性适体,系统地比较了这些重新设计方法的优点。我们发现,虽然许多适体结构支持 E-AB 信号,但在我们研究的各种构建体中,观察到的信号增益(目标结合时信号的相对变化)差异超过两个数量级(例如,我们的 ATP 传感器的范围从-10%到 200%)。因此,优化开关结构是实现最大 E-AB 信号增益的重要因素,我们发现这种最佳几何形状是针对构建传感器的适体序列特异性的。

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