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Polyelectrolyte Multilayers-Modified Polystyrene Plate Improves Conventional Immunoassay: Full Covering of the Blocking Reagent

机译:聚电解质多层改性的聚苯乙烯板改进了常规的免疫测定:完全覆盖了封闭剂

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In this study, we fabricated polyelectrolyte multilayers (PEMs) on a polystyrene (PS) plate by a simple and novel alternate drop coating process (Acta Biomaterialia 2008, 4, 1255-1262), leading to the construction of a functional platform for improving conventional enzyme-linked immunosorbent assay (ELISA) systems. Poly(diallyldim-ethylammonium chloride) (PDDA) and poly(sodium 4-sty-renesulfonate) (PSS) were used as cationic and anionic polyelectrolytes, and then positively or negatively charged surfaces were obtained on the PEMs. The PDDA/PSS PEMs on the PS plate had the following favorable characteristics. On the positive PEMs, the coverage of the blocking reagent (ovalbumin from egg white: OVA) was over 100percent by electrostatic interaction between the protein and PEMs, hence, nonspecific adsorption from the secondary antibody was efficiently suppressed. Moreover, the positive PEMs showed higher sensitivity on the ELISA than the negative PEMs, including the PS plate. Regularly oscillating behavior for sensitivity (specific signal-to-noise ratio) was observed on 1-10-step assemblies. The calibration curves for antigen detection on the positive PEMs had wide range of concentration from 0.002 to 5 (mu)g/mL, and largest change in signal as compared with the negative PEMs and the PS plate. In summary, we discovered that positive PEMs possessed excellent performance for ELISA systems, and PEMs could easily improve the immunoassay with a convenient process and diverse substrates.
机译:在这项研究中,我们通过简单新颖的交替滴涂工艺在聚苯乙烯(PS)板上制造了聚电解质多层(PEM)(Acta Biomaterialia 2008,4,1255-1262),从而构建了用于改善常规功能的功能平台酶联免疫吸附测定(ELISA)系统。聚(二烯丙基亚乙基-乙基氯化铵)(PDDA)和聚(4-苯乙烯基磺酸钠)(PSS)被用作阳离子和阴离子聚电解质,然后在PEM上获得带正电或带负电的表面。 PS板上的PDDA / PSS PEM具有以下有利特性。在阳性PEM上,封闭剂(来自蛋清的卵白蛋白:OVA)通过蛋白质与PEM之间的静电相互作用覆盖率超过100%,因此,可有效抑制二抗的非特异性吸附。此外,阳性PEM在ELISA上的灵敏度高于阴性PEM(包括PS板)。在1步到10步的组件上观察到灵敏度(特定信噪比)的规则振荡行为。与阴性PEM和PS板相比,在阳性PEM上进行抗原检测的校准曲线的浓度范围从0.002到5μg/ mL,信号变化最大。总而言之,我们发现阳性PEM对ELISA系统具有出色的性能,并且PEM可以通过方便的过程和多种底物轻松改进免疫测定。

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