The pros and cons of nucleic acid-amplified immunoassays-a comparative study on the quantitation of prostate-specific antigen with and without rolling circle amplification.

IF 3.8 2区 化学 Q1 BIOCHEMICAL RESEARCH METHODS Analytical and Bioanalytical Chemistry Pub Date : 2024-12-01 Epub Date: 2024-06-07 DOI:10.1007/s00216-024-05357-y
Mariia Dekaliuk, Zdeněk Farka, Niko Hildebrandt
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Abstract

Integrating isothermal nucleic acid amplification strategies into immunoassays can significantly decrease analytical limits of detection (LODs). On the other hand, an amplification step adds time, complication, reagents, and costs to the assay format. To evaluate the pros and cons in the context of heterogeneous multistep immunoassays, we quantified prostate-specific antigen (PSA) with and without rolling circle amplification (RCA). In addition, we compared time-gated (TG) with continuous-wave (CW) photoluminescence (PL) detection using a terbium complex and a fluorescein dye, respectively. For both direct (non-amplified) and amplified assays, TG PL detection provided circa four- to eightfold lower LODs, illustrating the importance of autofluorescence background suppression even for multi-wash assay formats. Amplified assays required an approximately 2.4 h longer assay time but led to almost 100-fold lower LODs down to 1.3 pg/mL of PSA. Implementation of TG-FRET (using a Tb-Cy5.5 donor-acceptor pair) into the RCA immunoassay resulted in a slightly higher LOD (3.0 pg/mL), but the ratiometric detection format provided important benefits, such as higher reproducibility, lower standard deviations, and multiplexing capability. Overall, our direct comparison demonstrated the importance of biological background suppression even in heterogeneous assays and the potential of using isothermal RCA for strongly decreasing analytical LODs, making such assays viable alternatives to conventional enzyme-linked immunosorbent assays (ELISAs).

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核酸扩增免疫测定的利与弊--关于使用和不使用滚动圈扩增法定量检测前列腺特异性抗原的比较研究。
将等温核酸扩增策略整合到免疫测定中可显著降低分析检测限(LOD)。另一方面,扩增步骤会增加检测形式的时间、复杂性、试剂和成本。为了评估异构多步免疫测定的利弊,我们对前列腺特异性抗原(PSA)进行了定量分析,包括有无滚动圈扩增(RCA)。此外,我们还比较了分别使用铽复合物和荧光素染料的时间门控(TG)和连续波(CW)光致发光(PL)检测法。对于直接(非扩增)和扩增检测,时间门控光致发光检测的检出限(LOD)大约低四倍到八倍,这说明了自发荧光背景抑制的重要性,即使对于多次洗涤的检测形式也是如此。扩增检测需要延长约 2.4 小时的检测时间,但可将 LOD 值降低近 100 倍,最低可达 1.3 pg/mL PSA。在 RCA 免疫测定中采用 TG-FRET(使用 Tb-Cy5.5 供体-受体对)会导致稍高的 LOD(3.0 pg/mL),但比率计量检测格式具有重要的优点,如更高的重现性、更低的标准偏差和复用能力。总之,我们的直接比较表明了生物背景抑制的重要性,即使是在异质检测中也是如此,而且等温 RCA 有可能大大降低分析 LOD,使这种检测成为传统酶联免疫吸附检测(ELISA)的可行替代品。
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来源期刊
CiteScore
8.00
自引率
4.70%
发文量
638
审稿时长
2.1 months
期刊介绍: Analytical and Bioanalytical Chemistry’s mission is the rapid publication of excellent and high-impact research articles on fundamental and applied topics of analytical and bioanalytical measurement science. Its scope is broad, and ranges from novel measurement platforms and their characterization to multidisciplinary approaches that effectively address important scientific problems. The Editors encourage submissions presenting innovative analytical research in concept, instrumentation, methods, and/or applications, including: mass spectrometry, spectroscopy, and electroanalysis; advanced separations; analytical strategies in “-omics” and imaging, bioanalysis, and sampling; miniaturized devices, medical diagnostics, sensors; analytical characterization of nano- and biomaterials; chemometrics and advanced data analysis.
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