Ultraspecific and Amplification-Free Quantification of Mutant DNA by Single-Molecule Kinetic Fingerprinting

被引:43
|
作者
Hayward, Stephen L. [1 ]
Lund, Paul E. [2 ]
Kang, Qing [1 ]
Johnson-Buck, Alexander [1 ,2 ,3 ]
Tewari, Muneesh [1 ,3 ,4 ,5 ,6 ]
Walter, Nils G. [2 ,3 ,5 ]
机构
[1] Univ Michigan, Dept Internal Med, Div Hematol Oncol, Ann Arbor, MI 48109 USA
[2] Univ Michigan, Dept Chem, Single Mol Anal Grp, Ann Arbor, MI 48109 USA
[3] Univ Michigan, Ctr RNA Biomed, Ann Arbor, MI 48109 USA
[4] Univ Michigan, Dept Biomed Engn, Ann Arbor, MI 48109 USA
[5] Univ Michigan, Ctr Computat Med & Bioinformat, Ann Arbor, MI 48109 USA
[6] Univ Michigan, Biointerfaces Inst, Ann Arbor, MI 48109 USA
关键词
CIRCULATING TUMOR DNA; NUCLEIC-ACID DETECTION; TRANSRENAL DNA; FETAL DNA; HYBRIDIZATION; URINE; DESIGN; CANCER; DISCRIMINATION; LOCALIZATION;
D O I
10.1021/jacs.8b06685
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Conventional techniques for detecting rare DNA sequences require many cycles of PCR amplification for high sensitivity and specificity, potentially introducing significant biases and errors. While amplification-free methods exist, they rarely achieve the ability to detect single molecules, and their ability to discriminate between single-nucleotide variants is often dictated by the specificity limits of hybridization thermodynamics. Here we show that a direct detection approach using single-molecule kinetic fingerprinting can surpass the thermodynamic discrimination limit by 3 orders of magnitude, with a dynamic range of up to S orders of magnitude with optional super-resolution analysis. This approach detects mutations as subtle as the drug-resistance conferring cancer mutation EGFR T790M (a single C -> T substitution) with an estimated specificity of 99.99999%, surpassing even the leading PCR-based methods and enabling detection of 1 mutant molecule in a background of at least 1 million wild type molecules. This level of specificity revealed rare, heat-induced cytosine deamination events that introduce false positives in PCR-based detection, but which can be overcome in our approach through milder thermal denaturation and enzymatic removal of damaged nucleobases.
引用
收藏
页码:11755 / 11762
页数:8
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