Use of Recombinant BP26 Protein in Serological Diagnosis of Brucella melitensis Infection in Sheep

A. Cloeckaert, Sylvie Baucheron, N. Vizcaı́no, M. Zygmunt
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引用次数: 62

Abstract

ABSTRACT Previously a Brucella protein named CP28, BP26, or Omp28 has been identified as an immunodominant antigen in infected cattle, sheep, goats, and humans. In the present study we evaluated antibody responses of infected and B. melitensisRev.1-vaccinated sheep to the BP26 protein using purified recombinant BP26 protein produced in Escherichia coli in an indirect enzyme-linked immunosorbent assay (I-ELISA). The specificity of the I-ELISA determined with sera from healthy sheep (n = 106) was 93%. The sensitivity of the I-ELISA assessed with sera from naturally infected and suspected sheep found positive in the current conventional diagnostic tests was as follows: 100% for bacteriologically and serologically positive sheep (n = 50), 88% for bacteriologically negative but serologically and delayed-type hypersensitivity-positive sheep (n = 50), and 84% for bacteriologically and serologically negative but delayed-type hypersensitivity-positive sheep (n = 19). However, the absorbance values observed did not reach those observed in an I-ELISA using purified O-polysaccharide (O-PS) as an antigen. In sheep experimentally infected with B. melitensis H38 the antibody response to BP26 was delayed and much weaker than that to O-PS. Nevertheless, the BP26 protein appears to be a good diagnostic antigen to be used in confirmatory tests and for serological differentiation between infected and B. melitensis Rev.1-vaccinated sheep. Weak antibody responses to BP26 in some of the latter sheep suggest that aB. melitensis Rev.1 bp26 gene deletion mutant should be constructed to ensure this differentiation.
重组BP26蛋白在绵羊布氏菌感染血清学诊断中的应用
以前,一种名为CP28、BP26或Omp28的布鲁氏菌蛋白已被确定为感染牛、绵羊、山羊和人的免疫优势抗原。在本研究中,我们评估了被感染的B. melitensisRev的抗体反应。通过间接酶联免疫吸附试验(I-ELISA),用大肠杆菌生产的纯化重组BP26蛋白接种了1只羊的BP26蛋白。用健康绵羊(n = 106)血清检测I-ELISA的特异性为93%。对目前常规诊断试验中自然感染和疑似感染羊的血清进行I-ELISA评估的敏感性如下:细菌学和血清学阳性羊(n = 50)为100%,细菌学阴性但血清学和延迟型超敏反应阳性羊(n = 50)为88%,细菌学和血清学阴性但延迟型超敏反应阳性羊(n = 19)为84%。然而,观察到的吸光度值没有达到用纯化的o -多糖(O-PS)作为抗原的I-ELISA所观察到的吸光度值。绵羊实验感染羊羊H38后,抗体对BP26的反应延迟,且比对O-PS的反应弱得多。尽管如此,BP26蛋白似乎是一种良好的诊断抗原,可用于确诊试验和感染绵羊与接种了rev .1的绵羊之间的血清学区分。对BP26的弱抗体反应表明,应该构建aB. melitensis Rev.1 BP26基因缺失突变体来确保这种分化。
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