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一种用于检测抗猪瘟E2和E抗体的双免疫层析试纸条的研制。

Development of a dual immunochromatographic test strip to detect E2 and E antibodies against classical swine fever.

作者信息

Huynh Loc Tan, Sohn Eun-Ju, Park Youngmin, Kim Juhun, Shimoda Tomohiko, Hiono Takahiro, Isoda Norikazu, Hong Sung-Hee, Lee Ha-Na, Sakoda Yoshihiro

机构信息

Laboratory of Microbiology, Department of Disease Control, Faculty of Veterinary Medicine, Hokkaido University, Sapporo, Hokkaido, Japan.

Faculty of Veterinary Medicine, College of Agriculture, Can Tho University, Can Tho, Vietnam.

出版信息

Front Microbiol. 2024 Apr 11;15:1383976. doi: 10.3389/fmicb.2024.1383976. eCollection 2024.

Abstract

BACKGROUND

It is essential to consider a practical antibody test to successfully implement marker vaccines and validate vaccination efficacy against classical swine fever virus (CSFV). The test should include a serological antibody assay, combined with a tool for differentiating infected from vaccinated animals (DIVA). The immunochromatographic test strip (ICS) has been exclusively designed for detecting CSFV E2 antibodies while lacking in detecting E antibodies, which can be employed and satisfy DIVA strategy. This study developed a novel ICS for detecting CSFV E2/E dual-antibody. The effectiveness of ICS in evaluating the DIVA capability of two novel chimeric pestivirus vaccine candidates was assessed.

METHODS

Recombinant E2 or E protein was transiently expressed in the plant using . ICS was subsequently assembled, and goat anti-rabbit IgG and recombinant CSFV E2 or E protein were plated onto the nitrocellulose membrane as control and test lines, respectively. The sensitivity and specificity of ICS were evaluated using sera with different neutralizing antibody titers or positive for antibodies against CSFV and other pestiviruses. The coincidence rates for detecting E2 and E antibodies between ICS and commercial enzyme-linked immunosorbent assay (ELISA) kits were also computed. ICS performance for DIVA capability was evaluated using sera from pigs vaccinated with conventional vaccine or chimeric vaccine candidates.

RESULTS

E2 and E proteins were successfully expressed in -produced recombinant proteins. ICS demonstrated high sensitivity in identifying CSFV E2 and E antibodies, even at the low neutralizing antibody titers. No cross-reactivity with antibodies from other pestiviruses was confirmed using ICS. There were high agreement rates of 93.0 and 96.5% between ICS and two commercial ELISA kits for E2 antibody testing. ICS also achieved strong coincidence rates of 92.9 and 89.3% with two ELISA kits for E antibody detection. ICS confirmed the absence of CSFV E-specific antibodies in sera from pigs vaccinated with chimeric vaccine candidates.

CONCLUSION

E2 and E proteins derived from the plant showed great potential and can be used to engineer a CSFV E2/E dual-antibody ICS. The ICS was also highly sensitive and specific for detecting CSFV E2 and E antibodies. Significantly, ICS can fulfill the DIVA concept by incorporating chimeric vaccine candidates.

摘要

背景

要成功实施标记疫苗并验证针对经典猪瘟病毒(CSFV)的疫苗效力,考虑一种实用的抗体检测方法至关重要。该检测应包括血清学抗体检测,并结合一种区分感染动物和接种动物(DIVA)的工具。免疫层析试纸条(ICS)专门设计用于检测CSFV E2抗体,但缺乏检测E抗体的能力,而E抗体可用于满足DIVA策略。本研究开发了一种用于检测CSFV E2/E双抗体的新型ICS。评估了ICS在评估两种新型嵌合瘟病毒疫苗候选物的DIVA能力方面的有效性。

方法

使用[具体方法]在植物中瞬时表达重组E2或E蛋白。随后组装ICS,并将山羊抗兔IgG和重组CSFV E2或E蛋白分别铺在硝酸纤维素膜上作为对照线和检测线。使用具有不同中和抗体效价或对CSFV和其他瘟病毒抗体呈阳性的血清评估ICS的敏感性和特异性。还计算了ICS与商业酶联免疫吸附测定(ELISA)试剂盒在检测E2和E抗体方面的符合率。使用接种传统疫苗或嵌合疫苗候选物的猪的血清评估ICS的DIVA能力性能。

结果

E2和E蛋白在[具体植物]产生的重组蛋白中成功表达。ICS在识别CSFV E2和E抗体方面表现出高敏感性,即使在低中和抗体效价时也是如此。使用ICS未确认与其他瘟病毒抗体的交叉反应性。在检测E2抗体方面,ICS与两种商业ELISA试剂盒之间的一致性率分别为93.0%和96.5%。在检测E抗体方面,ICS与两种ELISA试剂盒的一致性率也分别达到92.9%和89.3%。ICS证实接种嵌合疫苗候选物的猪血清中不存在CSFV E特异性抗体。

结论

源自植物的E2和E蛋白显示出巨大潜力,可用于构建CSFV E2/E双抗体ICS。ICS在检测CSFV E2和E抗体方面也具有高敏感性和特异性。重要的是,ICS通过纳入嵌合疫苗候选物可以实现DIVA概念。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/86d8/11043574/ec57e22edd95/fmicb-15-1383976-g001.jpg

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