AhpC、AhpD和禽分枝杆菌14千道尔顿分泌抗原。在酶联免疫吸附试验中区分副结核和牛结核

I. Olsen, M. Tryland, H. Wiker, L. Reitan
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引用次数: 49

摘要

自然感染禽分枝杆菌亚种的牛血清。对56例副结核患者(n = 56)、自然感染(n = 4)和实验感染(n = 8)的牛分枝杆菌患者进行了副结核抗原抗体检测。建立了一种酶联免疫吸附法(ELISA)。鸟结核无性系种群。禽分枝杆菌亚种的超免疫抗血清上副结核抗原。以去除交叉反应的抗原。这种吸收抗原ELISA法识别出66%的副结核动物(56只中的37只),而患有自然发生的牛结核病(TB)的动物中没有可检测到的抗体。然而,实验牛结核动物在ELISA中也有应答。在一种商业化的酶联免疫吸附试验中也发现了类似的结果,表明这两种试验都不能区分副结核病和牛结核病。进一步检测血清对纯化AhpC和AhpD的抗体活性,这两种蛋白是由m组成表达的。鸟结核无性系种群。副结核菌病,并抵抗来自他们的培养滤液中分泌的14kda蛋白。鸟结核复杂。在48例副结核病牛中,分别有27%(13例)、15%(7例)和27%(13例)的AhpC、AhpD和14-kDa抗原抗体水平升高。48只动物中有17只(35%)的elisa阳性。患有牛结核病的动物中没有检测到针对任何纯化蛋白的抗体,尽管它们的交叉反应抗体水平很高。这些结果表明,在ELISA中需要纯化的特异性抗原来区分副结核和牛结核。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
AhpC, AhpD, and a Secreted 14-Kilodalton Antigen fromMycobacterium avium subsp.paratuberculosis Distinguish between Paratuberculosis and Bovine Tuberculosis in an Enzyme-Linked Immunosorbent Assay
ABSTRACT Sera from cattle naturally infected with Mycobacterium avium subsp. paratuberculosis(n = 56) and naturally (n = 4) and experimentally (n = 8) infected withMycobacterium bovis were tested for the presence of antibodies against paratuberculosis antigens. An enzyme-linked immunosorbent assay (ELISA) was established based on absorption ofM. avium subsp. paratuberculosis antigens on a hyperimmune antiserum against M. avium subsp.avium proteins in order to remove cross-reacting antigens. This absorbed-antigen ELISA recognized 66% of animals with paratuberculosis (37 of 56), while none of the animals with naturally occurring bovine tuberculosis (TB) had detectable antibodies. However, the animals with experimental bovine TB also responded in this ELISA. Similar results were found in a commercial ELISA, showing that neither of these tests was able to distinguish between paratuberculosis and bovine TB. The sera were further tested for antibody activities against purified AhpC and AhpD, which are proteins constitutively expressed byM. avium subsp. paratuberculosis, and against a secreted 14-kDa protein present in culture filtrates from theM. avium complex. Elevated antibody levels to AhpC, AhpD, and the 14-kDa antigen were found in 27% (13 of 48), 15% (7 of 48), and 27% (13 of 48), respectively, of the cattle with paratuberculosis. Together these ELISAs were positive with 35% (17 of 48) of the animals. None of the animals with bovine TB had detectable antibodies against any of the purified proteins despite their high levels of cross-reacting antibodies. These results show that purified specific antigens are needed to differentiate between paratuberculosis and bovine TB in ELISA.
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