Development of ELISA and Lateral Flow Immunoassays for Ochratoxins (OTA and OTB) Detection Based on Monoclonal Antibody

Fadlalla, Mohamed Hassan; Ling, Sumei; Wang, Rongzhi; Li, Xiulan; Yuan, Jun; Xiao, Shiwei; Wang, Ke; Tang, Shuqin; Elsir, Hoyda; Wang, Shihua

doi:10.3389/fcimb.2020.00080

Cited by 37 publications

(25 citation statements)

References 47 publications

(57 reference statements)

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“…Colloidal gold nanoparticles (AuNPs) could easily be observed to conjugate with the antibody. The immunochromatographic strip test, based on colloidal gold nanoparticles, was successfully applied in the detection [ 21 ]. A schematic diagram of the immunochromatographic strip test is shown in Figure 2 , to explain the working mechanism.…”

Section: Resultsmentioning

confidence: 99%

Development of Immunochromatographic Strip for Detection of αB-VxXXIVA-Conotoxin Based on 5E4 Monoclonal Antibody

Tang

Liu

Chen

et al. 2022

Toxins

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Given the application of αB-VxXXIVA-conotoxin (αB-CTX) in analgesics and cancer chemotherapeutics, and its threat to humans, it is urgent to develop a rapid, effective and accurate method for the analysis and detection of αB-CTX in real shellfish and medicine drug samples. In the present study, two different immunochromatographic strips were established for αB-CTX detection, based on the monoclonal antibody 5E4 against αB-CTX, and the visual limits of detection (vLOD) for the colloidal gold nanoparticles-based strip (AuNPs-based strip) and nanoflowers-based strip (AuNFs-based strip) were 4 μg/mL and 1.5 μg/mL, respectively. The developed AuNPs-/AuNFs-based strips have good specificity and accuracy, and the detection results were analyzed in less than 10 min, without using an instrument. In view of the excellent repeatability and usability, the established methods could be applied to detect and analyze the content of αB-CTX in real samples.

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Section: Resultsmentioning

confidence: 99%

Development of Immunochromatographic Strip for Detection of αB-VxXXIVA-Conotoxin Based on 5E4 Monoclonal Antibody

Tang

Liu

Chen

et al. 2022

Toxins

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“…Moreover, complicated and tedious operation steps, high requirement of samples and detection practicability seriously limits their application in the detection of αB-CTX in real samples [ 19 ]. In contrast, immunoassays with high sensitivity, accuracy and adaptability have been widely used to detect the targets (toxins, pathogenic molecules and heavy metals) in different samples [ 20 , 21 , 22 ]. In the previous study, we developed ELISA and colloidal test strips based on monoclonal antibodies (mAb) against ω-CTX to detect ω-CTX MVIIA residue in Conus samples [ 5 ].…”

Section: Introductionmentioning

confidence: 99%

Detection of αB-Conotoxin VxXXIVA (αB-CTX) by ic-ELISA Based on an Epitope-Specific Monoclonal Antibody

Tang

Liu

Gao

et al. 2022

Toxins

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In view of the toxicological hazard and important applications in analgesics and cancer chemotherapeutics of αB-CTX, it is urgent to develop an accurate, effective and feasible immunoassay for the determination and analysis of αB-CTX in real samples. In this study, MBP-αB-CTX4 tandem fusion protein was used as an immunogen to elicit a strong immune response, and a hybridoma cell 5E4 secreting IgG2b against αB-CTX was successfully screened by hybridoma technology. The affinity of the purified 5E4 monoclonal antibody (mAb) was 1.02 × 108 L/mol, which showed high affinity and specificity to αB-CTX. Epitope 1 of αB-CTX is the major binding region for 5E4 mAb recongnization, and two amino acid residues (14L and 15F) in αB-CTX were critical sites for the interaction between αB-CTX and 5E4 mAb. Indirect competitive ELISA (ic-ELISA) based on 5E4 mAb was developed to detect and analyze αB-CTX in real samples, and the linear range of ic-ELISA to αB-CTX was 117–3798 ng/mL, with a limit of detection (LOD) of 81 ng/mL. All the above results indicated that the developed ic-ELISA had high accuracy and repeatability, and it could be applied for αB-CTX detection and drug analysis in real samples.

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“…This principle provides quick and easy-to-obtain assay results and determines the practical demand for LFIA tests [18]. Many studies have successfully used GNFs as antibody carriers and detectable markers for LFIA using decreased LODs, usually from 4 to 10 times compared to LFIAs using common GNSs [19][20][21][22][23]. However, most of these works were limited by the consideration of a single GNF preparation without substantiating the nanoparticle size and shape requirements and the grounded choice of a method for their synthesis.…”

Section: Introductionmentioning

confidence: 99%

Comparative Assessment of Different Gold Nanoflowers as Labels for Lateral Flow Immunosensors

Taranova

Byzova

Придворова

et al. 2021

Sensors

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Many studies have found that gold nanoparticles with branched surfaces (nanoflowers) are markers for immunosensors that provide higher sensitivity gains than the commonly used spherical gold nanoparticles. Although the analytical characteristics of nanoparticle-using systems vary significantly depending on their size and shape, the question of choosing the best gold nanoflowers remains open. This work presents a comparative study of a panel of 33 preparations of gold nanoflowers formed by varying several parameters: the size of spherical nanoparticles-nuclei, the concentrations of nuclei, and tetrachloroauric acid during growth. The sizes of the resulting particles, their sorption capacity under antibody immobilization, mobility along membranes for lateral flow assays, and the effects of these parameters on the limits of detection of lateral flow immunoassay are characterized. The optimality of preparations obtained by growing a 0.2% v/v solution of nuclei with a diameter of 10 or 20 nm with tetrachloroauric acid at a concentration of 0.12 mM was shown. With their use, lateral flow immune tests were developed to determine markers of acute myocardial infarction—fatty acids binding protein and troponins I and T. The use of gold nanoflowers obtained under the proposed protocols led to significant gains in the limits of detection—3 to 10 times under visual detection and over 100 times under instrumental detection—compared to spherical gold nanoparticles. The significant increase under instrumental detection is due to the label’s low nonspecific binding.

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Development of ELISA and Lateral Flow Immunoassays for Ochratoxins (OTA and OTB) Detection Based on Monoclonal Antibody

Cited by 37 publications

References 47 publications

Development of Immunochromatographic Strip for Detection of αB-VxXXIVA-Conotoxin Based on 5E4 Monoclonal Antibody

Development of Immunochromatographic Strip for Detection of αB-VxXXIVA-Conotoxin Based on 5E4 Monoclonal Antibody

Detection of αB-Conotoxin VxXXIVA (αB-CTX) by ic-ELISA Based on an Epitope-Specific Monoclonal Antibody

Comparative Assessment of Different Gold Nanoflowers as Labels for Lateral Flow Immunosensors

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