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Cloning of a Truncated Babesia equi Gene Encoding an 82-Kilodalton Protein and Its Potential Use in an Enzyme-Linked Immunosorbent Assay

机译:截短的Bassia equi基因编码82-Kilodalton蛋白的克隆及其在酶联免疫吸附测定中的潜在用途

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摘要

To isolate Babesia equi genes encoding immunodominant proteins, a cDNA expression library prepared from B. equi mRNA was immunoscreened with B. equi-infected horse serum. Eighteen positive cDNA clones were obtained, and the clone that showed the strongest immunoreactivity, designated Be82, was further characterized. The Be82 gene consisted of 1,953 bp and contained a partial open reading frame lacking the 5′-terminal sequence. As shown by Western blot analyses, immune sera from mice intraperitoneally injected with the Be82 gene product recognized the 82- and 52-kDa proteins of B. equi but not those of Babesia caballi. The glutathione S-transferase fusion protein expressed in Escherichia coli that was purified and used as the antigen in the enzyme-linked immunosorbent assay reacted specifically with B. equi-infected horse sera. These results suggest that the Be82 gene product is a potential diagnostic antigen candidate in the detection of B. equi infection in horses that will be useful both in the performance of epidemiological studies and in the granting of quarantine passes.
机译:为了分离编码免疫优势蛋白的巴贝斯马(Babesia equi)基因,用马氏杆菌感染的马血清免疫筛选由马氏杆菌mRNA制备的cDNA表达文库。获得了18个阳性cDNA克隆,并进一步鉴定了显示出最强免疫反应性的克隆Be82。 Be82基因由1,953 bp组成,并包含缺少5'端序列的部分开放阅读框。如Western印迹分析所示,腹膜内注射Be82基因产物的小鼠的免疫血清识别马来酸双歧杆菌的82-和52-kDa蛋白,但不能识别巴贝斯贝氏杆菌的。在大肠杆菌中表达的谷胱甘肽S-转移酶融合蛋白经过纯化,并在酶联免疫吸附测定中用作抗原,与马来酸支原体感染的马血清特异性反应。这些结果表明,Be82基因产物是检测马匹中的B. equi感染的潜在诊断抗原候选物,将在进行流行病学研究和授予检疫通行证中有用。

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