Department of Health Technology, DTU Health Tech, Technical University of Denmark, Building 345C, 2800, Kongens Lyngby, Denmark.
BluSense Diagnostics ApS, Fruebjergvej 3, DK-2100, Copenhagen, Denmark.
Anal Bioanal Chem. 2020 May;412(12):2705-2710. doi: 10.1007/s00216-020-02568-x. Epub 2020 Mar 10.
Detection of a single base mutation in Mycobacterium tuberculosis DNA can provide fast and highly specific diagnosis of antibiotic-resistant tuberculosis. Mutation-specific ligation of padlock probes (PLPs) on the target followed by rolling circle amplification (RCA) is highly specific, but challenging to integrate in a simple microfluidic device due to the low temperature stability of the phi29 polymerase and the interference of phi29 with the PLP annealing and ligation. Here, we utilized the higher operation temperature and temperature stability of Equiphi29 polymerase to simplify the integration of the PLP ligation and RCA steps of an RCA assay in two different strategies performed at uniform temperature. In strategy I, PLP annealing took place off-chip and the PLP ligation and RCA were performed in one pot and the two reactions were clocked by a change of the temperature. For a total assay time of about 1.5 h, we obtained a limit of detection of 2 pM. In strategy II, the DNA ligation mixture and the RCA mixture were separated into two chambers on a microfluidic disc. After on-disc PLP annealing and ligation, the disc was spun to mix reagents and initiate RCA. For a total assay time of about 2 h, we obtained a limit of detection of 5 pM. Graphical abstract.
结核分枝杆菌 DNA 中单碱基突变的检测可快速、高度特异性地诊断耐药性结核。目标上的锁式探针(PLP)的突变特异性连接,然后进行滚环扩增(RCA),特异性很高,但由于 phi29 聚合酶的低温稳定性以及 phi29 对 PLP 退火和连接的干扰,难以整合到简单的微流控装置中。在这里,我们利用 Equiphi29 聚合酶的更高操作温度和温度稳定性,以两种不同的策略在统一温度下简化了 RCA 检测中 PLP 连接和 RCA 步骤的整合。在策略 I 中,PLP 退火在芯片外进行,PLP 连接和 RCA 在一个管中进行,两个反应通过温度变化进行计时。总检测时间约为 1.5 小时,我们获得了 2 pM 的检测限。在策略 II 中,将 DNA 连接混合物和 RCA 混合物分离到微流控盘上的两个腔室中。在盘上进行 PLP 退火和连接后,旋转圆盘以混合试剂并启动 RCA。总检测时间约为 2 小时,我们获得了 5 pM 的检测限。
