Department of Chemistry, North Carolina State University, 2620 Yarbrough Dr., Raleigh, North Carolina 27695, United States.
Acc Chem Res. 2023 Jul 4;56(13):1731-1743. doi: 10.1021/acs.accounts.3c00113. Epub 2023 Jun 14.
Aptamers are short, single-stranded nucleic acids that have been selected from random libraries to bind specific molecules with high affinity via an method termed systematic evolution of ligands by exponential enrichment (SELEX). They have been generated for diverse targets ranging from metal ions to small molecules to proteins and have demonstrated considerable promise as biorecognition elements in sensors for applications including medical diagnostics, environmental monitoring, food safety, and forensic analysis. While aptamer sensors have made great strides in terms of sensitivity, specificity, turnaround time, and ease of use, several challenges have hindered their broader adoption. These include inadequate sensitivity, bottlenecks in aptamer binding characterization, and the cost and labor associated with aptamer engineering. In this Account, we describe our successes in using nuclease enzymes to address these problems. While working with nucleases to enhance the sensitivity of split aptamer sensors via enzyme-assisted target recycling, we serendipitously discovered that the digestion of DNA aptamers by exonucleases is inhibited when an aptamer is bound to a ligand. This finding served as the foundation for the development of three novel aptamer-related methodologies in our laboratory. First, we used exonucleases to truncate nonessential nucleotides from aptamers to generate structure-switching aptamers in a single step, greatly simplifying the aptamer engineering process. Second, we used exonucleases to develop a label-free aptamer-based detection platform that can utilize aptamers directly obtained from selection to detect analytes with ultralow background and high sensitivity. Through this approach, we were able to detect analytes at nanomolar levels in biological samples, with the capacity for achieving multiplexed detection by using molecular beacons. Finally, we used exonucleases to develop a high throughput means of characterizing aptamer affinity and specificity for a variety of ligands. This approach has enabled more comprehensive analysis of aptamers by greatly increasing the number of aptamer candidates and aptamer-ligand pairs that can be tested in a single experiment. We have also demonstrated the success of this method as a means for identifying new mutant aptamers with augmented binding properties and for quantifying aptamer-target affinity. Our enzymatic technologies can greatly streamline the aptamer characterization and sensor development process, and with the adoption of robotics or liquid handling systems in the future, it should be possible to rapidly identify the most suitable aptamers for a particular application from hundreds to thousands of candidates.
适体是通过一种称为指数富集的配体系统进化(SELEX)的方法从随机文库中筛选出来的短的、单链核酸,它们与特定分子具有高亲和力。它们已经针对从金属离子到小分子、蛋白质等各种靶标生成,并且作为生物识别元件在传感器中的应用中表现出了相当大的应用前景,包括医学诊断、环境监测、食品安全和法医学分析。虽然适体传感器在灵敏度、特异性、周转时间和易用性方面取得了很大的进展,但一些挑战阻碍了它们的更广泛采用。这些挑战包括灵敏度不足、适体结合特性的瓶颈以及与适体工程相关的成本和劳动力。在本报告中,我们描述了使用核酸酶来解决这些问题的成功经验。在使用核酸酶通过酶辅助目标回收来提高分裂适体传感器的灵敏度的过程中,我们偶然发现当适体与配体结合时,外切核酸酶对 DNA 适体的消化被抑制。这一发现为我们实验室中三种新的适体相关方法的发展奠定了基础。首先,我们使用外切核酸酶从适体中截断非必需核苷酸,以单步生成结构切换适体,大大简化了适体工程过程。其次,我们使用外切核酸酶开发了一种无标记的基于适体的检测平台,可以直接使用从选择中获得的适体来检测超低背景和高灵敏度的分析物。通过这种方法,我们能够在生物样品中检测到纳摩尔级别的分析物,并且可以通过使用分子信标实现多重检测的能力。最后,我们使用外切核酸酶开发了一种高通量的方法来表征适体与各种配体的亲和力和特异性。这种方法可以通过大大增加单个实验中可以测试的适体候选物和适体-配体对的数量,对适体进行更全面的分析。我们还证明了这种方法是一种识别具有增强结合特性的新突变适体的方法,并可以定量适体-靶标亲和力。我们的酶技术可以大大简化适体表征和传感器开发过程,并且随着未来在机器人或液体处理系统中的采用,应该有可能从数百到数千个候选物中快速识别出最适合特定应用的适体。
