Literature DB >> 16053288

Displacement enzyme linked aptamer assay.

Eva Baldrich1, Josep Lluis Acero, Gunter Reekmans, Wim Laureyn, Ciara K O'Sullivan.   

Abstract

Immense effort has been placed on the realization of immunoassays exploiting displacement of a suboptimum target, due to the ease of use and applicability to immunochromatographic strips and immunosensors. Most of the efforts reported to date focus on the use of a suboptimal target that is displaceable by the target toward which the antibody has higher affinity. Limited success has been achieved due to difficulty in obtaining suboptimal targets to which the antibody has enough affinity to bind while at the same time having lower levels of affinity in comparison to the target to facilitate displacement. Aptamers are synthetic oligonucleotides specifically selected to bind a certain target. Thanks to their high affinity and sensitivity, aptamers appear as alternative candidates to antibodies for analytical devices and several enzyme-linked aptamer assays and aptasensors have been reported. Aptamers, in contrast to antibodies, require the formation of a three-dimensional structure for target binding and can thus be anticipated to have a much higher affinity for binding its target rather than a modified form of the target (e.g., enzyme-labeled target). This phenomenon can be exploited for the development of a displacement assay, using enzyme-labeled target as a suboptimal displaceable molecule. Here, we report the first demonstration of the exploitation of an aptamer in an extremely rapid and highly sensitive displacement assay. Surface plasmon resonance studies demonstrated the thrombin-binding aptamer to have a lower affinity for enzyme-labeled thrombin than unmodified thrombin, with respective K(D) of 1.1 x 10(-8) and 2.9 x 10(-9) M. The assay is extremely rapid, requiring only 10 min for completion, and exhibits a detection limit lower than that obtainable with competitive enzyme-linked aptamer assays and comparable to that of hybrid aptamer-antibody assays. Optimal storage conditions for precoated microtiter plates (consisting of coated aptamer and captured labeled target) were elucidated, and the results demonstrated their amenability to long-term storage, facilitating commercially viable displacement enzyme-linked aptamer assays that simply require sample addition, with a total assay time, including color development, of 30 min.

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Year:  2005        PMID: 16053288     DOI: 10.1021/ac0502450

Source DB:  PubMed          Journal:  Anal Chem        ISSN: 0003-2700            Impact factor:   6.986


  6 in total

Review 1.  Functional nucleic acid sensors.

Authors:  Juewen Liu; Zehui Cao; Yi Lu
Journal:  Chem Rev       Date:  2009-05       Impact factor: 60.622

Review 2.  Aptamers and the next generation of diagnostic reagents.

Authors:  Varatharasa Thiviyanathan; David G Gorenstein
Journal:  Proteomics Clin Appl       Date:  2012-12       Impact factor: 3.494

3.  Cotinine-conjugated aptamer/anti-cotinine antibody complexes as a novel affinity unit for use in biological assays.

Authors:  Sunyoung Park; Dobin Hwang; Junho Chung
Journal:  Exp Mol Med       Date:  2012-09-30       Impact factor: 8.718

4.  DNAzyme Catalyzed Tyramide Depositing Reaction for In Situ Imaging of Protein Status on the Cell Surface.

Authors:  Lulu Xu; Shengchun Liu; Tiantian Yang; Yifan Shen; Yuhong Zhang; Lizhen Huang; Lutan Zhang; Shijia Ding; Fangzhou Song; Wei Cheng
Journal:  Theranostics       Date:  2019-03-16       Impact factor: 11.556

Review 5.  Electrochemical Aptasensors: Current Status and Future Perspectives.

Authors:  Ragaa Abd-Ellatief; Maha Ragaa Abd-Ellatief
Journal:  Diagnostics (Basel)       Date:  2021-01-11

Review 6.  Luminescent Aptamer-Based Bioassays for Sensitive Detection of Food Allergens.

Authors:  Donato Calabria; Martina Zangheri; Seyedeh Rojin Shariati Pour; Ilaria Trozzi; Andrea Pace; Elisa Lazzarini; Maria Maddalena Calabretta; Mara Mirasoli; Massimo Guardigli
Journal:  Biosensors (Basel)       Date:  2022-08-15
  6 in total

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