Sensitive detection of fusion transcripts with padlock probe-based continuous cascade amplification (P-CCA)

环介导等温扩增 融合基因 级联 滚动圆复制 结扎 化学 基因 融合 分子生物学 重组酶聚合酶扩增 DNA 计算生物学 生物 遗传学 聚合酶 哲学 色谱法 语言学
作者
Yutong Chen,Fengxia Su,Yongqiang Cheng,Xiaofei He,Zhengping Li
出处
期刊:Analyst [Royal Society of Chemistry]
卷期号:147 (10): 2207-2214 被引量:1
标识
DOI:10.1039/d2an00341d
摘要

Gene fusion, resulting from chromosomal rearrangements, is the juxtaposition of two or more original genes into the same set to form a functional gene. The significant specificity of fusion genes for tumor cells makes them promising candidates for diagnostic biomarkers and therapeutic targets. The sensitive detection of fusion transcripts is of great significance in biological research and disease diagnosis. Here, we propose a method for the sensitive detection of PML-RARα gene fusion transcripts by the direct ligation of the padlock probe at the junction site, and the cyclized DNA then triggers a continuous cascade amplification of two subsequent amplification reactions: rolling circle amplification (RCA) and loop-mediated isothermal amplification (LAMP). Due to the ability of the ligation reaction to differentiate mismatched sequences and the high amplification efficiency of continuous cascade amplification reactions, the proposed method can detect as low as 1 fM targets with high specificity, and has been successfully applied to real samples. Through a facile design of the triggering sequence in padlock probes, the cascade RCA and LAMP can be integrated into one-tube isothermal reactions with a simple one-step operation. Therefore, this work provides a convenient padlock probe-based continuous cascade amplification (P-CCA) method for the detection of fusion transcripts, and offers a fast and reliable platform for the early clinical diagnosis of gene fusion-related cancers.
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