Double base mismatches mediated catalytic hairpin assembly for enzyme-free single-base mutation detection: integrating signal recognition and amplification in one

Lanyue Wang; Sisi Bu; Shijie Xu; Tuo Huang; Fang Yang; Qianglong Tan; Minxin Deng; Wenlin Xie; Bobo Cai; Jian Chen

doi:10.1007/s00604-024-06366-5

Double base mismatches mediated catalytic hairpin assembly for enzyme-free single-base mutation detection: integrating signal recognition and amplification in one

Mikrochim Acta. 2024 May 17;191(6):334. doi: 10.1007/s00604-024-06366-5.

Authors

Lanyue Wang¹, Sisi Bu¹, Shijie Xu¹, Tuo Huang¹, Fang Yang¹, Qianglong Tan¹, Minxin Deng¹, Wenlin Xie², Bobo Cai³, Jian Chen⁴

Affiliations

¹ School of Chemistry and Chemical Engineering, Hunan University of Science and Technology, Xiangtan, 411201, Hunan, China.
² School of Chemistry and Chemical Engineering, Hunan University of Science and Technology, Xiangtan, 411201, Hunan, China. Xwl2000zsu@163.com.
³ Zhejiang Hospital, Hangzhou, 310013, China. caibobo@zju.edu.cn.
⁴ School of Chemistry and Chemical Engineering, Hunan University of Science and Technology, Xiangtan, 411201, Hunan, China. chenjianpharm@hnust.edu.cn.

PMID: 38758362
DOI: 10.1007/s00604-024-06366-5

Abstract

Single nucleotide polymorphism (SNP) biosensors are emerging rapidly for their promising applications in human disease prevention diagnosis, treatment, and prognosis. However, it remains a bottleneck in equipping simple and stable biosensors with the traits of high sensitivity, non-enzyme, and low cost. Double base mismatches mediated chain displacement reactions have attracted fascinating advantages of tailorable thermodynamics stability, non-enzyme, and excellent assembly compliance to involvement in SNP identification. As the base mismatch position and amount in DNA sequence can be artificially adjusted, it provides plenty of selectivity and specificity for exploring perfect biosensors. Herein, a biosensor with double base mismatches mediated catalytic hairpin assembly (CHA) is designed via one base mismatch in the toehold domain and the other base mismatch in the stem sequence of hairpin 1 (H1) by triggering CHA reaction to achieve selective amplification of the mutation target (MT) and fluorescence resonance energy transfer (FRET) effect that is composed of Cy3 and Cy5 terminally attached H1 and hairpin 2 (H2). Depending on the rationally designed base mismatch position and toehold length, the fabricated biosensors show superior SNP detection performance, exhibiting a good linearity with high sensitivity of 6.6 fM detection limit and a broad detection abundance of 1%. The proposed biosensor can be used to detect the KRAS mutation gene in real samples and obtain good recoveries between 106 and 116.99%. Remarkably, these extendible designs of base mismatches can be used for more types of SNP detection, providing flexible adjustment based on base mismatch position and toehold length variations, especially for their thermodynamic model for DNA-strand displacement reactions.

Keywords: Catalytic hairpin assembly; Double base mismatches; Fluorescence resonance energy transfer; KRAS mutation gene; Single nucleotide polymorphism.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Base Pair Mismatch*
Biosensing Techniques* / methods
Catalysis
DNA / chemistry
DNA / genetics
Fluorescence Resonance Energy Transfer* / methods
Humans
Inverted Repeat Sequences
Limit of Detection
Mutation
Nucleic Acid Amplification Techniques* / methods
Polymorphism, Single Nucleotide*
Proto-Oncogene Proteins p21(ras) / genetics

Substances

KRAS protein, human

Abstract

Publication types

MeSH terms

Substances

Grants and funding