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开发并鉴定一种用于定量检测登革热病毒补体结合抗体的多重分析方法。

Development and Characterization of a Multiplex Assay to Quantify Complement-Fixing Antibodies against Dengue Virus.

机构信息

Takeda Vaccines, Inc., 40 Landsdowne Street, Cambridge, MA 02139, USA.

出版信息

Int J Mol Sci. 2021 Nov 5;22(21):12004. doi: 10.3390/ijms222112004.

Abstract

Antibodies capable of activating the complement system (CS) when bound with antigen are referred to as "complement-fixing antibodies" and are involved in protection against . A complement-fixing antibody test has been used in the past to measure the ability of dengue virus (DENV)-specific serum antibodies to activate the CS. As originally developed, the test is time-consuming, cumbersome, and has limited sensitivity for DENV diagnosis. Here, we developed and characterized a novel multiplex anti-DENV complement-fixing assay based on the Luminex platform to quantitate serum antibodies against all four serotypes (DENV1-4) that activate the CS based on their ability to fix the complement component 1q (C1q). The assay demonstrated good reproducibility and showed equivalent performance to a DENV microneutralization assay that has been used to determine DENV serostatus. In non-human primates, antibodies produced in response to primary DENV1-4 infection induced C1q fixation on homologous and heterologous serotypes. Inter-serotype cross-reactivity was associated with homology of the envelope protein. Interestingly, the antibodies produced following vaccination against Zika virus fixed C1q on DENV. The anti-DENV complement fixing antibody assay represents an alternative approach to determine the quality of functional antibodies produced following DENV natural infection or vaccination and a biomarker for dengue serostatus, while providing insights about immunological cross-reactivity among different .

摘要

当与抗原结合时能够激活补体系统 (CS) 的抗体被称为“补体固定抗体”,并参与针对 的保护。过去曾使用补体固定抗体试验来测量登革热病毒 (DENV)-特异性血清抗体激活 CS 的能力。最初开发的该试验耗时、繁琐,并且对 DENV 诊断的灵敏度有限。在这里,我们开发并表征了一种基于 Luminex 平台的新型多重抗 DENV 补体固定测定法,用于根据其固定补体成分 1q (C1q) 的能力来定量针对所有四个血清型 (DENV1-4) 的血清抗体。该测定法表现出良好的重现性,并且与用于确定 DENV 血清状态的 DENV 微量中和测定法具有等效性能。在非人类灵长类动物中,针对原发性 DENV1-4 感染产生的抗体诱导 C1q 固定在同源和异源血清型上。血清型间交叉反应性与包膜蛋白的同源性相关。有趣的是,针对寨卡病毒接种产生的抗体固定了 DENV 上的 C1q。抗 DENV 补体固定抗体测定法代表了一种替代方法,可以确定 DENV 自然感染或接种疫苗后产生的功能性抗体的质量,并且是登革热血清状态的生物标志物,同时提供了关于不同 之间免疫交叉反应性的见解。

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