Silver and gold enhancement methods for lateral flow immunoassays

Rodríguez, Myriam Oliveira; Covián, Lucía Blanco; Garcı́a, Agustı́n Costa; Blanco‐López, M. Carmen

doi:10.1016/j.talanta.2015.10.068

Cited by 119 publications

(88 citation statements)

References 28 publications

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“…Anfossi et al [133] and Panferov et al [134,135] considered the possibilities of silver enhancement (restoration of the silver salt on the surface of a gold nanoparticle with an increase in its size) in LFIA. In a study by Rodriguez et al [136], the optimal regimes of silver and gold enhancements were determined to enhance the signal from the gold nanoparticles. Enzymatic amplification using alkaline phosphatase was studied by Panferov et al [137] for LFIA of potato virus X and by Kim et al [138] for LFIA of C-reactive protein.…”

Section: Proper Response For Lfiamentioning

confidence: 99%

Ways to Reach Lower Detection Limits of Lateral Flow Immunoassays

Zherdev¹,

Dzantiev²

2018

Rapid Test - Advances in Design, Format and Diagnostic Applications

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This chapter considers factors influencing sensitivity of lateral flow immunoassay and modern developments that are focused on reaching lower detection limits. The existing variety of proposed approaches is classified in accordance with the "big five rules" for these assays, including proper sample, receptor, interaction, response, and output. The solutions for rapid extraction of target analytes and preventing negative influence of extractants are considered. Role to antibodies affinity and specificity is characterized. Potential of alternate bioreceptor molecules is discussed. Immunoreactants' compositions, concentrations, and locations on the test strip are characterized as factors determining assay parameters. The existing variety of labels is compared in terms of their optical and alternate registration. Tools to modulate a sequence of analytical reactions and to form aggregates of the detected labels are considered. The discussed approaches are illustrated through developments of test strips for detection of mycotoxins, veterinary drugs, and other analytes.The overall design of the immunochromatographic test strip is shown in Figure 1. It is a composite of several membranes of different structures and porosities, fixed on a support. The bundling of the test strip can vary, so it makes sense to consider its design based on what analytical tasks are being performed on its different sites.A. Typically, the lower portion of the test strip contains a sample pad. It ensures the absorption of sample components, in which the presence of the target analyte is checked.B. The following is a section with immunoreagents that are washed out during the analysis and move upward along with the components of the sample. As a rule, a conjugate pad forms this zone. It contains a conjugate of antibodies against the target analyte with a nanodispersed label-particles of colored latex, colloidal gold, and so on.The next two sections are located on the main working membrane of the test strip. C.First, there is a zone along which the movement of the absorbed components of the sample and the washed immunoreagents continues. During this movement, immune reactions occur, and specific intermolecular complexes are formed. D.Next, a mixture of reacted and unreacted molecules enters the binding area with immobilized immunoreagents. Depending on whether the target analyte was present in the sample and in what amount, binding of labeled immune complexes occurs in certain areas (in the traditional case, with the formation of narrow colored lines). Usually, additional reagents are located here to control the functionality of the test system. E. The upper part of the test strip with the final pad, usually structurally similar to the sample pad, ensures the further movement of the reaction mixture under the action of capillary forces and the washing of unreacted components from the underlying areas. These processes allow the label's binding to be evaluated correctly.Membrane components of the test strip are fixed on a plastic support and partia...

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Section: Proper Response For Lfiamentioning

confidence: 99%

Ways to Reach Lower Detection Limits of Lateral Flow Immunoassays

Zherdev¹,

Dzantiev²

2018

Rapid Test - Advances in Design, Format and Diagnostic Applications

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“…In lateral flow tests, nitrocellulose membrane act as stationary phase, and aptamer, antibody or antigen are immobilized in the capture area. To visualize the interactions in capture area, different labels have been used including liposome, colloidal carbon, colloidal gold, fluorescent probes, quantum dots, phosphors, bioluminescent markers, enzyme labels, paramagnetic particles and latex particles (Takanashi, Okame et al 2008;Blazkova, Koets et al 2009;Quesada-González and Merkoçi 2015;Qi, Huang et al 2016;Rodríguez, Covián et al 2016;Zhao, Wang et al 2016), each of which has particular characteristic and their usage is dependent on the analyzed samples (Tse 2009). …”

Section: Labels For Immunochromatographic Assaysmentioning

confidence: 99%

“…Also, colloidal gold in unconjugated forms and conjugated forms can be easily found from a variety of commercial sources (Tse 2009). Besides, several investigations have been reported on the potential benefits of using different labels, for example, fluorescent dyes, liposomes encapsulating visible or fluorescent dyes, quantum dots, magnetic nanoparticles, and silver-gold nanoparticles (Goryacheva, Lenain et al 2013;Byzova, Smirnova et al 2014;Zhang, Huang et al 2015;Rodríguez, Covián et al 2016;Wu, Yuan et al 2016) A study using fluorescent immunoliposome as a label has been described by Khreich et al (Khreich, Lamourette et al 2008) for detection of Staphylococcus aureus enterotoxin B (SEB) in water and juice.…”

Section: Labels For Immunochromatographic Assaysmentioning

confidence: 99%

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Lateral flow based immunobiosensors for detection of food contaminants

Raeisossadati

Danesh

Borna³

et al. 2016

Biosensors and Bioelectronics

142

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“…The silver enhancement is based on the reduction of silver ions on the surface of gold nanoparticles (GNP), and provides a significant increase of initial GNP-caused coloration. This approach was previously used successfully in other LFIAs (Byzova, Zherdev, Sveshnikov, Sadykhov, & Dzantiev, 2015;Drygin et al, 2012;Gupta, Huda, Kilpatrick, & Velev, 2007;Panferov et al, 2016;Rodriguez, Covian, Garcia, & Blanco-Lopez, 2016), but it has not been combined with PLRV immunodetection. Because the possibility of nonspecific background coloration is indicated as an important risk factor in silver enhancement, this assay procedure was modified to limit this process.…”

Section: Introductionmentioning

confidence: 99%

Silver-enhanced lateral flow immunoassay for highly-sensitive detection of potato leafroll virus

Panferov

Safenkova

Byzova

et al. 2017

Food and Agricultural Immunology

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Rapid non-laboratory screening of plants for pathogenic viruses crucially influences crop yields in modern agricultural technologies. The aim of this study was to develop a highly-sensitive lateral flow immunoassay (LFIA) for rapid detection of potato leafroll virus (PLRV), an infectious agent of one of the most widespread potato diseases. The proposed LFIA combines the formation of sandwich immune complexes with gold nanoparticles (GNP) as labels and silver enhancement. The enhancement stage was realized using mixture of silver lactate and hydroquinone and subsequent addition of chloride-containing buffer to stop silver reduction. LFIA with silver enhancement was 15 times more sensitive (detection limit 0.2 ng/mL; 15 min) compared with conventional LFIA (detection limit 3 ng/mL; 10 min). The enhanced LFIA detected PLRV in leaves' extracts of infected potato in dilutions higher than enzyme-linked immunosorbent assay.

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Silver and gold enhancement methods for lateral flow immunoassays

Cited by 119 publications

References 28 publications

Ways to Reach Lower Detection Limits of Lateral Flow Immunoassays

Ways to Reach Lower Detection Limits of Lateral Flow Immunoassays

Lateral flow based immunobiosensors for detection of food contaminants

Silver-enhanced lateral flow immunoassay for highly-sensitive detection of potato leafroll virus

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