An Interfacial Affinity Interaction-Based Method for Detecting HOTAIR lncRNA in Cancer Plasma Samples

被引:1
|
作者
Clack, Kimberley [1 ,2 ]
Soda, Narshone [2 ]
Kasetsirikul, Surasak [2 ,3 ]
Kline, Richard [4 ]
Salomon, Carlos [4 ,5 ,6 ]
Shiddiky, Muhammad J. A. [1 ,2 ]
机构
[1] Griffith Univ, Sch Environm & Sci, Nathan Campus, Nathan, Qld 4111, Australia
[2] Griffith Univ, Queensland Micro & Nanotechnol Ctr, Nathan Campus, Nathan, Qld 4111, Australia
[3] Griffith Univ, Sch Engn & Built Environm EBE, Nathan Campus, Nathan, Qld 4111, Australia
[4] Ochsner Clin Fdn, Sect Gynaecol Oncol, New Orleans, LA 70121 USA
[5] Univ Queensland, Royal Brisbane & Womens Hosp, Ctr Clin Res, Exosome Biol Lab,Ctr Clin Diagnost, Brisbane, Qld 4029, Australia
[6] Univ Alba, Fac Ciencias Salud, Dept Invest Postgrad & Educ Continua DIPEC, Santiago 8320000, Chile
来源
BIOSENSORS-BASEL | 2022年 / 12卷 / 05期
基金
澳大利亚研究理事会; 澳大利亚国家健康与医学研究理事会;
关键词
HOTAIR lncRNA; interfacial biosensing; affinity interaction; RNA biosensor; electrochemical detection; ovarian cancer; LONG NONCODING RNA; DNA METHYLATION; BIOSENSOR; AMPLIFICATION;
D O I
10.3390/bios12050287
中图分类号
O65 [分析化学];
学科分类号
070302 ; 081704 ;
摘要
Long non-coding RNA Homeobox transcript antisense intergenic RNA (HOTAIR) is recognized as a participant in different processes of normal cell development. Aberrant overexpression of HOTAIR contributes to the initiation, growth, and invasiveness of ovarian cancer. Using the affinity interaction of target HOTAIR lncRNA sequences towards a screen-printed gold electrode (SPE-Au), herein we report on a novel, rapid and simple method to detect HOTAIR sequences. HOTAIR lncRNA sequences were first extracted from ovarian cancer cell lines and patient plasma samples and were magnetically captured and purified by complimentary capture probe-functionalized magnetic beads. Isolated target HOTAIR lncRNAs were directly adsorbed onto unmodified screen-printed gold electrodes (SPE-Au) for direct quantification with [Fe(CN)(6)](3-/4-) redox couple. Our assay achieved a linear dynamic range of 100 nM and 1 pM for detecting pre-clinical model HOTAIR lncRNA samples (%RSD <= 5%, for n = 3) and was highly specific, showing clear distinction between HOTAIR lncRNA targets and non-specific miR-891 and miR-486 (100 nM) (%RSD <= 5%, for n = 3). The method was tested using ovarian cancer-specific cell lines (SKOV3 and OVCAR3) and mesothelial cell line (MeT-5A)-derived lncRNAs. The analytical performance of our method was validated using RT-qPCR. Finally, the method was tested using clinical samples from ovarian cancer patients and the resulting electrochemical responses show a clear distinction between the ovarian carcinoma and benign samples.
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页数:13
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