Department of Bioengineering, Rice University, Houston, Texas, United States of America.
PLoS One. 2024 Aug 22;19(8):e0305002. doi: 10.1371/journal.pone.0305002. eCollection 2024.
The ability to both sensitively and specifically assess the sequence composition of a nucleic acid strand is an ever-growing field. Designing a detection scheme that can perform this function when the sequence of the target being detected deviates significantly from the canonical sequence however is difficult in part because probe/primer design is based on established Watson-Crick base-pairing rules. We present here a robust and tunable toehold-based exchange probe that can detect a sequence with a variable number of SNPs of unknown identity by inserting a series of controlled, sequential mismatches into the protector seal of the toehold probe, in an effort to make the protector seal "sloppy". We show that the mismatch-tolerant system follows predicted behavior closely even with targets containing up to four mismatches that thermodynamically deviate from the canonical sequence by up to 15 kcal/mole. The system also performs faithfully regardless of the global mismatch position on either the protector seal or target. Lastly, we demonstrate the generalizability of the approach by testing the increasingly mismatch-tolerant protectors on HIV clinical samples to show that the system is capable of resolving multiple, iteratively mutated sequences derived from numerous HIV sub-populations with remarkable precision.
能够灵敏且特异性地评估核酸链的序列组成是一个不断发展的领域。然而,当被检测目标的序列与典型序列有很大差异时,设计能够执行此功能的检测方案在某种程度上是困难的,因为探针/引物设计基于已建立的沃森-克里克碱基配对规则。我们在这里提出了一种稳健且可调的基于引发链置换的交换探针,通过在引发链探针的保护密封处插入一系列受控的、连续的错配,可以检测具有未知身份的 SNP 数量可变的序列,从而使保护密封变得“宽松”。我们表明,即使在包含多达四个与典型序列热力学偏差高达 15 千卡/摩尔的错配的靶标中,错配容忍系统也能紧密遵循预测的行为。该系统还能忠实地执行,无论保护密封或靶标上的全局错配位置如何。最后,我们通过在 HIV 临床样本上测试越来越耐受错配的保护剂来证明该方法的通用性,表明该系统能够以惊人的精度解析来自许多 HIV 亚群的多个、迭代突变序列。
