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开发一种间接酶联免疫吸附测定法,用于检测新西兰澳大利亚刷尾负鼠(帚尾袋貂)存档血清中针对摇摆负鼠病病毒的抗体。

Development of an indirect ELISA for detection of antibody to wobbly possum disease virus in archival sera of Australian brushtail possums (Trichosurus vulpecula) in New Zealand.

作者信息

Giles J C, Johnson W, Jones G, Heuer C, Dunowska M

机构信息

a School of Veterinary Science, Massey University , Palmerston North , New Zealand.

b Department of Statistics , University of California , Irvine , CA 92617 , USA.

出版信息

N Z Vet J. 2018 Jul;66(4):186-193. doi: 10.1080/00480169.2018.1465483. Epub 2018 May 6.

Abstract

AIMS

To develop an indirect ELISA based on recombinant nucleocapsid (rN) protein of wobbly possum disease (WPD) virus for investigation of the presence of WPD virus in Australian brushtail possums (Trichosurus vulpecula) in New Zealand.

METHODS

Pre- and post-infection sera (n=15 and 16, respectively) obtained from a previous experimental challenge study were used for ELISA development. Sera were characterised as positive or negative for antibody to WPD virus based on western-blot using WPD virus rN protein as antigen. An additional 215 archival serum samples, collected between 2000-2016 from five different regions of New Zealand, were also tested using the ELISA. Bayesian modelling of corrected optical density at 450 nm (OD) results from the ELISA was used to obtain estimates of receiver operating characteristic (ROC) curves to establish cut-off values for the ELISA, and to estimate the prevalence of antibody to WPD virus.

RESULTS

Western blot analysis showed 5/14 (36%) pre-infection sera and 11/11 (100%) post-infection sera from experimentally infected possums were positive for antibodies to WPD virus. Bayesian estimates of the ROC curves established cut-off values of OD≥0.41 for samples positive, and OD<0.28 for samples negative for antibody to WPD virus, for sera diluted 1:100 for the ELISA. Based on the model, the estimated proportion of samples with antibodies to WPD virus was 0.30 (95% probability interval=0.196-0.418). Of the 230 archival serum samples tested using the ELISA, 48 (20.9%) were positive for antibody to WPD virus, 155 (67.4%) were negative and 27 (11.7%) equivocal, using the established cut-off values. The proportion of samples positive for WPD virus antibody differed between geographical regions (p<0.001).

CONCLUSION

The results suggested that WPD virus or a related virus has circulated among possums in New Zealand with differences in the proportion of antibody-positive samples from different geographical regions. Antibodies to WPD virus did not seem to protect possums from disease following experimental infection, as one third of possums from the previous challenge study showed evidence of pre-existing antibody at the time of challenge. These results provide further support for existence of different pathotypes of WPD virus, but the exact determinants of protection against WPD and epidemiology of infection in various regions of New Zealand remain to be established.

CLINICAL RELEVANCE

Availability of the indirect ELISA for detection of WPD virus antibody will facilitate prospective epidemiological investigation of WPD virus circulation in wild possum populations in New Zealand.

摘要

目的

开发一种基于颤抖负鼠病(WPD)病毒重组核衣壳(rN)蛋白的间接酶联免疫吸附测定(ELISA),以检测新西兰澳大利亚刷尾负鼠(帚尾袋貂)中WPD病毒的存在情况。

方法

从先前的实验性攻毒研究中获得的感染前和感染后血清(分别为n = 15和16)用于ELISA开发。基于以WPD病毒rN蛋白作为抗原的蛋白质印迹法,将血清鉴定为WPD病毒抗体阳性或阴性。还使用ELISA对2000年至2016年期间从新西兰五个不同地区收集的另外215份存档血清样本进行了检测。对ELISA在450nm处校正光密度(OD)结果进行贝叶斯建模,以获得受试者操作特征(ROC)曲线估计值,从而确定ELISA的临界值,并估计WPD病毒抗体的流行率。

结果

蛋白质印迹分析显示,来自实验感染负鼠的5/14(36%)份感染前血清和11/11(100%)份感染后血清WPD病毒抗体呈阳性。ROC曲线的贝叶斯估计确定,对于ELISA中稀释1:100的血清,OD≥0.41的样本为WPD病毒抗体阳性,OD<0.28的样本为阴性。基于该模型,估计有WPD病毒抗体的样本比例为0.30(95%概率区间 = 0.196 - 0.418)。在使用ELISA检测的230份存档血清样本中,根据既定临界值,48份(20.9%)WPD病毒抗体呈阳性,155份(67.4%)呈阴性,27份(11.7%)结果不明确。不同地理区域WPD病毒抗体阳性样本的比例存在差异(p<0.001)。

结论

结果表明,WPD病毒或相关病毒在新西兰负鼠中传播,不同地理区域抗体阳性样本的比例存在差异。在实验感染后,WPD病毒抗体似乎不能保护负鼠免受疾病侵害,因为先前攻毒研究中的三分之一负鼠在攻毒时显示有预先存在抗体的证据。这些结果进一步支持了WPD病毒不同致病型的存在,但针对WPD的保护的确切决定因素以及新西兰各地区感染的流行病学情况仍有待确定。

临床意义

可用于检测WPD病毒抗体的间接ELISA将有助于对新西兰野生负鼠种群中WPD病毒传播进行前瞻性流行病学调查。

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