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Saliva as a source of anti-Toxoplasma gondii IgG for enzyme immunoassay in human samples
B.F.C. Sampaio, M.S. Macre, L.R. Meireles, H.F. Andrade Clinical Microbiology and Infection Volume 20, Issue 1, Pages O72-O74 (January 2014) DOI: / Copyright © 2014 European Society of Clinical Infectious Diseases Terms and Conditions
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FIG. 1 Dot-ELISA results for anti-T. gondii IgG detection in human saliva. (a) Results of the volunteers’ paired saliva and serum samples tested in quadruplicate. Dots contain T. gondii soluble antigen. Upper lanes, 1/200 serum; lower lane, 1 × reconstituted saliva. Arrows indicate specific IgG-positive samples. (b) Double dot design: upper dot was adsorbed with Staphylococcal IgG-binding protein A and lower dot was adsorbed with T. gondii soluble antigen and reacted with 1 × reconstituted saliva from the volunteers used in A. (c) Dot design as described in B using samples from university graduation students, as described in the Methods section. SPA, protein A dots; TGA, T. gondii soluble antigen dots. Clinical Microbiology and Infection , O72-O74DOI: ( / ) Copyright © 2014 European Society of Clinical Infectious Diseases Terms and Conditions
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FIG. 2 Protein A IgG capture ELISA assay of 100 samples of human saliva using T. gondii biotinylated antigen and revealed using OPD or TMB. Dot-ELISA positive (+) = closed symbols; Dot-ELISA negative (—) = open symbols; TMB (circles) and OPD (squares). The γ-axis was divided at the threshold of the 95% confidence interval cut-off of the negative samples. The mean and the SEM for each sample are shown. Clinical Microbiology and Infection , O72-O74DOI: ( / ) Copyright © 2014 European Society of Clinical Infectious Diseases Terms and Conditions
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