Double blocking gap-filling-ligation coupled with cascade isothermal amplification for ultrasensitive quantification of N 6 -methyladenosine.

We developed a method for quantifying -methyladenosine at one-nucleotide resolution based on double blocking gap-filling-ligation and cascade isothermal amplification. This proposed method can detect as low as 1 fM target RNA, achieving selectivity up to approximately 100-fold between mA and A, and has been successfully applied to the analysis of mA at specific sites in cell samples.