One-pot DTECT enables rapid and efficient capture of genetic signatures for precision genome editing and clinical diagnostics

一锅法DTECT能够快速高效地捕获基因特征,用于精准基因组编辑和临床诊断。

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作者:Lou Baudrier ,Orléna Benamozig ,Jethro Langley ,Sanchit Chopra ,Tatiana Kalashnikova ,Sacha Benaoudia ,Gurpreet Singh ,Douglas J Mahoney ,Nicola A M Wright ,Pierre Billon

Abstract

The detection of genomic sequences and their alterations is crucial for basic research and clinical diagnostics. However, current methodologies are costly and time-consuming and require outsourcing sample preparation, processing, and analysis to genomic companies. Here, we establish One-pot DTECT, a platform that expedites the detection of genetic signatures, only requiring a short incubation of a PCR product in an optimized one-pot mixture. One-pot DTECT enables qualitative, quantitative, and visual detection of biologically relevant variants, such as cancer mutations, and nucleotide changes introduced by prime editing and base editing into cancer cells and human primary T cells. Notably, One-pot DTECT achieves quantification accuracy for targeted genetic signatures comparable with Sanger and next-generation sequencing. Furthermore, its effectiveness as a diagnostic platform is demonstrated by successfully detecting sickle cell variants in blood and saliva samples. Altogether, One-pot DTECT offers an efficient, versatile, adaptable, and cost-effective alternative to traditional methods for detecting genomic signatures.

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