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Taqman-mgb nanopcr for highly specific detection of single-base mutations

  • Zhenrui Xue
  • , Minli You
  • , Ping Peng
  • , Haoyang Tong
  • , Wanghong He
  • , Ang Li
  • , Ping Mao
  • , Ting Xu
  • , Feng Xu
  • , Chunyan Yao
  • Army Medical University
  • Xi'an Jiaotong University

科研成果: 期刊稿件文章同行评审

28 引用 (Scopus)

摘要

Purpose: Detection of single-base mutations is important for real-time monitoring of tumor progression, therapeutic effects, and drug resistance. However, the specific detection of single-base mutations from excessive wild-type background sequences with routine PCR technology remains challenging. Our objective is to develop a simple and highly specific qPCR-based single-base mutation detection method. Methods: Using EGRF T790M as a model, gold nanoparticles at different concentrations were separately added into the Taqman-MGB qPCR system to test specificity improvement, leading to the development of the optimal Taqman-MGB nanoPCR system. Then, these optimal conditions were used to test the range of improvement in the specificity of mutant-type and wild-type templates and the detection limit of mutation abundances in a spiked sample. Results: The Taqman-MGB nanoPCR was established based on the traditional qPCR, with significantly suppressed background noise and improved specificity for single-base mutation detection. With EGFR T790M as a template, we demonstrated that our Taqman-MGB nanoPCR system could improve specificity across a wide concentration range from 10−9 μM to 10 μM and detect as low as 0.95% mutation abundance in spiked samples, which is lower than what the traditional Taqman-MGB qPCR and existing PCR methods can detect. Moreover, we also proposed an experimentally validated barrier hypothesis for the mechanism of improved specificity. Conclusion: The developed Taqman-MGB nanoPCR system could be a powerful tool for clinical single-base mutation detection.

源语言英语
页(从-至)3695-3705
页数11
期刊International Journal of Nanomedicine
16
DOI
出版状态已出版 - 2021

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