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一种使用量子点和侧向流动试纸条检测小反刍兽疫病毒血清抗体的新型免疫测定法。

A new immunoassay of serum antibodies against Peste des petits ruminants virus using quantum dots and a lateral-flow test strip.

作者信息

Cheng Si, Sun Jie, Yang Junxing, Lv Jianqiang, Wu Feng, Lin Yanxing, Liao Lishan, Ye Yiyou, Cao Chenfu, Fang Liurong, Hua Qunyi

机构信息

Division of Animal Infectious Diseases, State Key Laboratory of Agricultural Microbiology, College of Veterinary Medicine, Huazhong Agricultural University, Wuhan, Hubei, 430070, China.

Shenzhen Entry-Exit Inspection and Quarantine Bureau of the People's Republic of China (SZCIQ), Shenzhen, Guangdong, 518045, China.

出版信息

Anal Bioanal Chem. 2017 Jan;409(1):133-141. doi: 10.1007/s00216-016-9972-3. Epub 2016 Oct 25.

DOI:10.1007/s00216-016-9972-3
PMID:27783124
Abstract

A fast and ultrasensitive test-strip system combining quantum dots (QDs) with a lateral-flow immunoassay strip (LFIAS) was established for detection of Peste des petits ruminants virus (PPRV) antibody. The highly luminescent water-soluble carboxyl-functionalized QDs were used as the signal output and were conjugated to streptococcal protein G (SPG), which was capable of binding to immunoglobulin G (IgG) from many species through an amide bond to capture the target PPRV IgGs. The PPRV N protein, which was immobilized on the detection zone of the test strip, was expressed by transfecting recombinant Bacmid-PPRV-N with Lipofect into Sf9 insect cells. When exposed to PPRV IgG, QD-SPG bound to PPRV N protein, resulting in the formation of a complex that subsequently produced a bright fluorescent band in response to 365 nm ultraviolet excitation. Sensitivity evaluation showed that the QD-LFIAS limit of detection (LOD) for PPRV antibody was superior to competitive enzyme-linked immunosorbent assay (c-ELISA) and the immunochromatographic strip. No cross reaction was observed when the positive sera of bluetongue virus, canine distemper virus, goat pox virus, and foot-and-mouth disease virus were tested. Further evaluation using field samples indicated that the diagnostic specificity and sensitivity of the QD-LFIAS was 99.47 and 97.67 %, respectively, with excellent agreement between QD-LFIAS and c-ELISA. The simple analysis step and objective results that can be obtained within 15 min indicate that this new method shows great promise for rapid, sensitive detection of PPRV IgG for onsite, point-of-care diagnosis and post vaccination evaluation (PVE). Graphical Abstract Ultrasensitive fluorescent QD immunochromotography in combination with recombinant PPRV N protein could be used to detect PPRV antibody in serum.

摘要

建立了一种将量子点(QDs)与侧向流动免疫分析试纸条(LFIAS)相结合的快速超灵敏检测系统,用于检测小反刍兽疫病毒(PPRV)抗体。高发光水溶性羧基功能化量子点用作信号输出,并与链球菌蛋白G(SPG)偶联,SPG能够通过酰胺键与多种物种的免疫球蛋白G(IgG)结合,以捕获目标PPRV IgG。固定在试纸条检测区的PPRV N蛋白是通过用脂质体转染重组杆粒-PPRV-N到Sf9昆虫细胞中表达的。当暴露于PPRV IgG时,QD-SPG与PPRV N蛋白结合,形成复合物,随后在365 nm紫外线激发下产生明亮的荧光带。灵敏度评估表明,QD-LFIAS对PPRV抗体的检测限优于竞争酶联免疫吸附测定(c-ELISA)和免疫层析试纸条。检测蓝舌病病毒、犬瘟热病毒、山羊痘病毒和口蹄疫病毒的阳性血清时未观察到交叉反应。使用现场样本的进一步评估表明,QD-LFIAS的诊断特异性和灵敏度分别为99.47%和97.67%,QD-LFIAS与c-ELISA之间具有极好的一致性。简单的分析步骤和15分钟内可获得客观结果表明,这种新方法在现场即时诊断和疫苗接种后评估(PVE)中快速、灵敏检测PPRV IgG方面显示出巨大潜力。图形摘要 超灵敏荧光QD免疫层析结合重组PPRV N蛋白可用于检测血清中的PPRV抗体。

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