College of Medicine and Health Science, Wuhan Polytechnic University, Wuhan, China.
Huaren Technology Co., Ltd, Wuhu, China.
Anal Methods. 2024 Sep 12;16(35):5999-6010. doi: 10.1039/d4ay00831f.
Eliminating errors in next-generation sequencing has proven to be challenging. Here we present a novel strategy for DNA sequencing, called correctable two-color fluorogenic DNA decoding sequencing, which can significantly improve sequencing accuracy and throughput by employing a dual-nucleotide addition combined with fluorogenic sequencing-by-synthesis (SBS) chemistry. This sequencing method involves introducing a mixture of natural nucleotide X, labeled unblocked nucleotide X', 3' blocked nucleotide Y*, and labeled 3' blocked nucleotide Y* into each reaction cycle. By cyclically interrogating a template twice with different nucleotide combinations, two sets of base-encoding are sequentially obtained, enabling accurate deduction of base sequence. We demonstrate the remarkable efficacy of this approach in detecting and correcting sequencing errors, achieving a theoretical error rate of 0.0005%, which is twice as accurate as Sanger sequencing. Furthermore, we show the capability to detect known mutation sites using information from only a single sequencing run. The correctable two-color fluorogenic DNA decoding sequencing approach should enable accurate identification of extremely rare genomic variations in diverse applications in biology and medicine.
在下一代测序中消除错误已被证明具有挑战性。在这里,我们提出了一种新的 DNA 测序策略,称为可纠正双色荧光 DNA 解码测序,它通过采用双核苷酸添加结合荧光测序合成 (SBS) 化学,可显著提高测序准确性和通量。这种测序方法涉及在每个反应循环中引入天然核苷酸 X 的混合物、标记的未封闭核苷酸 X'、3'封闭核苷酸 Y和标记的 3'封闭核苷酸 Y。通过用不同的核苷酸组合循环两次询问模板,可顺序获得两组碱基编码,从而准确推断碱基序列。我们证明了这种方法在检测和纠正测序错误方面的显著效果,达到了理论错误率为 0.0005%,比 Sanger 测序准确两倍。此外,我们还展示了仅使用单个测序运行的信息来检测已知突变位点的能力。可纠正双色荧光 DNA 解码测序方法应该能够在生物学和医学的各种应用中准确识别极其罕见的基因组变异。
