Site-Specific mRNA Cleavage for Selective and Quantitative Profiling of Alternative Splicing with Label-Free Optical Biosensors

被引:9
|
作者
Huertas, Cesar S. [1 ,2 ,3 ]
Bonnal, Sophie [4 ,5 ,6 ]
Soler, Maria [1 ,2 ,7 ]
Escuela, Alfonso M. [8 ]
Valcarcel, Juan [4 ,5 ,6 ,9 ]
Lechuga, Laura M. [1 ,2 ]
机构
[1] CSIC, BIST, Catalan Inst Nanosci & Nanotechnol ICN2, Nanobiosensors & Bioanalyt Applicat Grp, Barcelona 08193, Spain
[2] CIBER BBN, Barcelona 08193, Spain
[3] RMIT Univ, Integrated Photon & Applicat Ctr, Sch Engn, Melbourne, Vic 3001, Australia
[4] Ctr Regulacio Genom, Barcelona 08003, Spain
[5] BIST, Barcelona 08003, Spain
[6] Univ Pompeu Fabra, Barcelona 08003, Spain
[7] Networking Res Ctr Bioengn Biomat & Nanomed CIBER, Madrid 28029, Spain
[8] Univ Las Palmas Gran Canaria, Inst Appl Microelect IUMA, E-35017 Las Palmas Gran Canaria, Spain
[9] Inst Catalana Recerca & Estudis Avancats, Barcelona 08010, Spain
基金
欧洲研究理事会;
关键词
DNA; FAS; OLIGONUCLEOTIDES; EVENTS; TIA-1;
D O I
10.1021/acs.analchem.9b03898
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Alternative splicing of mRNA precursors is a key process in gene regulation, contributing to the diversity of proteomes by the alternative selection of exonic sequences. Alterations in this mechanism are associated with most cancers, enhancing their proliferation and survival, and can be employed as cancer biomarkers. Label-free optical biosensors are ideal tools for the highly sensitive and label-free analysis of nucleic acids. However, their application for alternative splicing analysis has been hampered due to the formation of complex and intricate long-range base pairing interactions which make the direct detection in mRNA isoforms difficult. To solve this bottleneck, we introduce a methodology for the generation of length controlled RNA fragments from purified total RNA, which can be easily detected by the biosensor. The methodology seizes RNase H enzyme activity to degrade the upstream and downstream RNA segments flanking the target sequence upon hybridization to specific DNA oligos. It allows the fast and direct monitoring of Fas gene alternative splicing in real time, employing a surface plasmon resonance biosensor. We demonstrate the selective and specific detection of mRNA fragments in the pM-nM concentration range, reducing quantification errors and showing 81% accuracy when compared to RT-qPCR The site-specific cleavage outperformed random RNA hydrolysis by increasing the detection accuracy by 20%, making this methodology particularly appropriate for label-free quantification of alternative splicing events in complex samples.
引用
收藏
页码:15138 / 15146
页数:9
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