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委内瑞拉马脑炎血清学诊断检测方法的评估

Assessment of assays for the serodiagnosis of Venezuelan equine encephalitis.

作者信息

Coates D M, Makh S R, Jones N, Lloyd G

机构信息

Division of Pathology, Service Centre for Applied Microbiology and Research, Salisbury, Wiltshire, U.K.

出版信息

J Infect. 1992 Nov;25(3):279-89. doi: 10.1016/0163-4453(92)91559-t.

Abstract

An enzyme-linked immunosorbent assay (ELISA), an immunofluorescence assay (IFA), a plaque-reduction neutralization (PRN) assay and an immunoblot assay, all by means of an antigen prepared from the attenuated Venezuelan equine encephalitis (VEE) vaccine strain of virus, were compared with the conventional haemagglutination-inhibition (HAI) assay for the serodiagnosis of VEE. The HAI assay, which includes the use of wild type virus antigen, was less sensitive than the other assays when known-positive samples of serum from an epidemic of VEE were tested. The superior sensitivity of the IgG ELISA was confirmed by assaying both VEE epidemic samples and a bank of samples from VEE vaccinees. Samples with antibody specific for other Alphaviruses, however, cross reacted weakly in this assay. The PRN, immunoblot and HAI assays, although less sensitive than the ELISA, proved more specific. Experimental infection of guinea-pigs demonstrated the value of the IgM ELISA in the early detection of VEE virus infection. Immunoglobulin M was first found at 4 days post-inoculation (p.i.) during the viraemic phase of infection. Immunoglobulin G was detected by ELISA, PRN assay and IFA at 6 days p.i. Immunoblot and HAI assays, however, did not give positive results until 10 days p.i. The results support the diagnostic use of ELISA for detecting VEE virus-specific IgM and IgG, and the use of the specific PRN assay for confirming the diagnosis.

摘要

采用从委内瑞拉马脑炎(VEE)病毒减毒疫苗株制备的抗原,对酶联免疫吸附测定(ELISA)、免疫荧光测定(IFA)、蚀斑减少中和(PRN)测定和免疫印迹测定进行了比较,并与传统的血凝抑制(HAI)测定法用于VEE的血清学诊断。当检测VEE流行时已知阳性血清样本时,包括使用野生型病毒抗原的HAI测定法比其他测定法敏感性低。通过检测VEE流行样本和一组VEE疫苗接种者的样本,证实了IgG ELISA的较高敏感性。然而,对其他甲病毒具有特异性抗体的样本在该测定中会发生弱交叉反应。PRN测定、免疫印迹测定和HAI测定虽然比ELISA敏感性低,但证明更具特异性。豚鼠的实验性感染证明了IgM ELISA在早期检测VEE病毒感染中的价值。在感染的病毒血症期,接种后4天首次发现免疫球蛋白M。接种后6天通过ELISA、PRN测定和IFA检测到免疫球蛋白G。然而,免疫印迹测定和HAI测定直到接种后10天才得出阳性结果。这些结果支持使用ELISA检测VEE病毒特异性IgM和IgG,并使用特异性PRN测定来确诊。

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