首页> 外文期刊>Journal of Virological Methods >Reproducibility of antigen-immobilized enzyme-linked immunosorbent assay (ELISA) and sandwich ELISA for quantitative detection of NNV particles
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Reproducibility of antigen-immobilized enzyme-linked immunosorbent assay (ELISA) and sandwich ELISA for quantitative detection of NNV particles

机译:抗原固定化酶联免疫吸附测定(ELISA)和夹心ELISA的再现性,用于定量检测NNV颗粒

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Nervous necrosis virus (NNV) is a fish virus belonging to family Nodaviridae. In this study, we prepared partially aggregated and monometric NNV particles to determine reproducibility of two different enzyme-linked immunosorbent assays (ELISAs): antigen-immobilized ELISA and sandwich ELISA. Passing ratios of purified NNV particles through ultrafilters with molecular weight cut off (MWCO) of 10(5), 3 x 10(5) and 10(6) were 0%, 35.2% and 80.3%, respectively, suggesting that purified NNV particles were partially aggregated whereas those in filtrates with MWCO of 3 x 10(5) could be monometric. Both NNV particles were subjected to ELISAs. Reduction ratios of ELISA values by 2-fold dilution of antigens were 50% in sandwich ELISA regardless of aggregation state of NNV particles. In contrast, those in antigen-immobilized ELISA were 42% (partially aggregated NNV) to 43% (monometric NNV), which were lower than the theoretical value (50%). This could be due to changes in aggregation state of NNV particles during dry-immobilization. Sandwich ELISA has excellent reproducibility from five times of experiments, in comparison with antigen-immobilized ELISA. Furthermore, available range of regression lines (R-2 > 0.99) in sandwich ELISA was wider than that in antigen-immobilized ELISA. These results revealed that sandwich ELISA had better quantitativeness, reproducibility and available range of ELISA values than antigen-immobilized ELISA.
机译:神经坏死病毒(NNV)是属于家族诺韦伐的鱼类病毒。在这项研究中,我们制备了部分聚集的和测量NNV颗粒以确定两种不同酶联免疫吸附测定的再现性(ELISA):抗原固定的ELISA和夹心ELISA。通过分子量切断(MWCO)为10(5),3×10(5)和10(6)(6)分别为0%,35.2%和80.3%的超过滤器通过纯化的NNV颗粒的通过,表明纯化的NNV颗粒部分汇集,而MWCO为3×10(5)的滤液中可以是单次的。对ELISAS进行NNV颗粒。无论NNV颗粒的聚集状态如何,在夹心ELISA中,ELISA值2倍稀释剂的减少比例为50%。相反,抗原 - 固定的ELISA中的那些是42%(部分聚集的NNV)至43%(单数值NNV),其低于理论值(50%)。这可能是由于干固化期间NNV颗粒聚集状态的变化。与抗原固定的ELISA相比,夹心ELISA具有优异的五次实验再现性。此外,夹心ELISA中的可用的回归线(R-2> 0.99)宽于抗原固定的ELISA。这些结果表明,Sandwich ELISA具有比抗原固定的ELISA更好的数量,可重复性和可用的ELISA值范围。

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