基于免疫分析的rom28蛋白作为布鲁氏菌种鉴定候选蛋白的评价。

IF 2.4 4区 医学 Q3 MICROBIOLOGY
Richa Hans, Duraipandian Thavaselvam
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引用次数: 0

摘要

介绍。布鲁氏菌病是一种重要的细菌性人畜共患病,在发展中国家重新成为一个严重的公共卫生问题。两种主要的布鲁氏菌,即梅利氏菌和流产布鲁氏菌,在人类中引起复发性易感染。因此,在疾病负担低的地区,需要快速准确的诊断,以便进行疾病的早期控制和预防。本研究评价了夹心酶联免疫吸附试验(S-ELISA)免疫测定全细胞(WC)和重组外膜蛋白(rOmp28)衍生的IgG多克隆抗体在布鲁氏菌敏感检测中的应用前景。基于免疫测定的WC检测重要亚临床基质中布鲁氏菌的下限。方法学。采用Ni-NTA凝胶亲和层析纯化重组rOmp28,并利用BALB/c小鼠和新西兰白兔制备了针对布鲁氏菌不同抗原(Ags)的IgG多克隆抗体(pAbs)。采用棋盘夹心ELISA法和P/N比(“P”阳性检测样品与“N”阴性对照的光密度)对研究进行评价和优化。采用Western blot方法对pab进行了鉴定,并在不同基质中加入了布氏菌WC Ag。采用WC ag来源的兔IgG(捕获抗体浓度为10µg ml-1)和rom28来源的小鼠IgG(检测抗体浓度为100µg ml-1)建立双抗体S-ELISA,检测范围为102 ~ 108个细胞ml-1,检测限为102个细胞ml-1。wc2pab检测蜜蜂B. melitensis 16M和B. abortus S99的P/N比值分别为0.6和0.9,而wc2pab检测蜜蜂B. melitensis 16M和abortus S99的P/N比值为1.1。在免疫印迹分析中,WC Ag来源的兔IgG的P/N比为4.4,而针对布鲁氏菌细胞包膜(CE)、rom28和对rom28 Ag高亲和力的超声抗原(SA)来源的兔IgG的P/N比为4.2>4.1>2.4。在P/N分别为11.8和6.3的情况下,rommp28来源的小鼠IgG检测出两种布鲁氏菌。经验证,S-ELISA可检测人全血和血清样品中的布鲁氏菌WCs,与其他相关细菌无交叉反应。开发的S-ELISA对不同临床和非临床疾病表现基质的布鲁氏菌的早期检测具有特异性和敏感性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Immunoassay-based evaluation of rOmp28 protein as a candidate for the identification of Brucella species.

Introduction. Brucellosis is an important bacterial zoonosis, re-emerging as a serious public health concern in developing countries. Two major species, Brucella melitensis and Brucella abortus, cause recurrent facile infection in human. Therefore, rapid and accurate diagnosis for early disease control and prevention is needed in areas with low disease burden.Hypothesis. This study evaluated the sandwich enzyme-linked immunosorbent assay (ELISA) (S-ELISA) immunoassay for potential use of whole-cell (WC) and recombinant outer-membrane protein (rOmp28)-derived IgG polyclonals in sensitive detection of Brucella.Aim. Immunoassay-based WC detection of Brucella species in important sub-clinical matrices at lower limits of detection.Methodology. We purified recombinant rOmp28 with Ni-NTA gel affinity chromatography and produced IgG polyclonal antibodies (pAbs) using BALB/c mice and New Zealand white female rabbits against different antigens (Ags) of Brucella. Checkerboard sandwich ELISA and P/N ratio (optical density of 'P' positive test sample to 'N' negative control) were used for evaluation and optimization of the study. The pAbs were characterized using Western blot analysis and different matrices were spiked with WC Ag of Brucella.Results. Double-antibody S-ELISA was developed using WC Ag-derived rabbit IgG (capture antibody at 10 µg ml-1) and rOmp28-derived mice IgG (detection antibody at 100 µg ml-1) with a detection range of 102 to 108 cells ml-1 and a limit of detection at 102 cells ml-1. A P/N ratio of 1.1 was obtained with WC pAbs as compared to 0.6 and 0.9 ratios with rOmp28-derived pAbs for detecting B. melitensis 16M and B. abortus S99, respectively. An increased P/N ratio of 4.4 was obtained with WC Ag-derived rabbit IgG as compared to 4.2>4.1>2.4 ratios obtained with rabbit IgGs derived against cell envelope (CE), rOmp28 and sonicated antigen (SA) of Brucella with high affinity for rOmp28 Ag analysed on immunoblots. The rOmp28-derived mice IgG revealed two Brucella species at P/N ratios of 11.8 and 6.3, respectively. Upon validation, S-ELISA detected Brucella WCs in human whole blood and sera samples with no cross-reactivity to other related bacteria.Conclusion. The developed S-ELISA is specific and sensitive in early detection of Brucella from different matrices of clinical and non-clinical disease presentation.

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来源期刊
Journal of medical microbiology
Journal of medical microbiology 医学-微生物学
CiteScore
5.50
自引率
3.30%
发文量
143
审稿时长
4.5 months
期刊介绍: Journal of Medical Microbiology provides comprehensive coverage of medical, dental and veterinary microbiology, and infectious diseases. We welcome everything from laboratory research to clinical trials, including bacteriology, virology, mycology and parasitology. We publish articles under the following subject categories: Antimicrobial resistance; Clinical microbiology; Disease, diagnosis and diagnostics; Medical mycology; Molecular and microbial epidemiology; Microbiome and microbial ecology in health; One Health; Pathogenesis, virulence and host response; Prevention, therapy and therapeutics
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