![]() ![]() ![]() In this antigen detection system, antibodies conjugated by the chimera were used in ELISA-like procedure to detect immobilized bovine serum albumin (BSA) on plate, and then the DNA was amplified by PCR. published an application of the fusion product and termed it immuno-polymerase chain reaction (immuno-PCR) 2. The idea of Immuno-PCR started from Sano and Canter’s work on a chimera of streptavidin and IgG binding domain which provide a bridge between the antibody and biotinylated DNA oligos in the early 1990s 1. Overall, these results show that the immuno-PCR method results in rapid detection of multiple EV markers from small sample volumes in a single tube. We further described the development of a micro-size exclusion chromatography method, where we were able to detect EV surface proteins with as little as 10 μL of human serum when combined with immuno-PCR. This approach was also successfully applied to similar protocol using cell and serum samples. Using this method, we demonstrate that multiple EV surface proteins can be profiled simultaneously with high sensitivity and specificity. Here, we present a new immuno-PCR method that takes advantage of commercially available TotalSeq antibodies containing DNA conjugated oligos to identify immobilized protein analysts using real-time qPCR. One of the challenges in the study of EVs and there utility as diagnostic biomarkers is the amount of EVs needed for traditional protein analysis methods. Over the past decade, EVs have become a new emerging source for cancer diagnostics. EVs encapsulate proteins, RNAs and metabolites from its origin cell and play important roles in intercellular communication events. Extracellular vesicles (EVs) are small nanometer-sized membrane sacs secreted into biological fluids by all cells.
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