| Literature DB >> 29266845 |
Omid Taghavian1, Aarti Jain1, Chester J Joyner2, Sunny Ketchum3, Rie Nakajima1, Algis Jasinskas1, Li Liang1, Rich Fong4, Christopher King4, Bryan Greenhouse5, Maxwell Murphy5, Jason Bailey6, Mary R Galinski2,6, John W Barnwell7, Christopher V Plowe8, D Huw Davies1, Philip L Felgner1.
Abstract
The development of vaccines against malaria and serodiagnostic tests for detecting recent exposure requires tools for antigen discovery and suitable animal models. The protein microarray is a high-throughput, sample sparing technique, with applications in infectious disease research, clinical diagnostics, epidemiology, and vaccine development. We recently demonstrated Qdot-based indirect immunofluorescence together with portable optical imager ArrayCAM using single isotype detection could replicate data using the conventional laser confocal scanner system. We developed a multiplexing protocol for simultaneous detection of IgG, IgA, and IgM and compared samples from a controlled human malaria infection model with those from controlled malaria infections of Aotus nancymaae, a widely used non-human primate model of human malaria. IgG profiles showed the highest concordance in number of reactive antigens; thus, of the 139 antigens recognized by human IgG antibody, 111 were also recognized by Aotus monkeys. Interestingly, IgA profiles were largely non-overlapping. Finally, on the path toward wider deployment of the portable platform, we show excellent correlations between array data obtained in five independent laboratories around the United States using the multiplexing protocol (R2 : 0.60-0.92). This study supports the use of this platform for wider deployment, particularly in endemic areas where such a tool will have the greatest impact on global human health.Entities:
Keywords: antibody isotype; malaria; multiplex; protein microarray; quantum dots
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Year: 2018 PMID: 29266845 PMCID: PMC6637747 DOI: 10.1002/pmic.201700277
Source DB: PubMed Journal: Proteomics ISSN: 1615-9853 Impact factor: 3.984