Recombinant proteins are a suggested alternative for the diagnosis of toxocariasis. The current Escherichia coli recombinant protein overexpression system usually produces insoluble products. As an alternative, yeast such as Pichia pastoris have secretory mechanisms, which could diminish the cost and time for production. This study aimed to produce recombinant proteins in Pichia pastoris and verify their sensibility and specificity in an indirect ELISA assay. Two sequences (rTES-30 and rTES-120) of Toxocara canis excretory-secretory antigens were cloned in a pPICZαB vector and expressed in P. pastoris KM71H. Sera samples collected from human adults infected by Toxocara spp. were tested by indirect ELISA using rTES-30 and rTES-120 as antigens. Recombinant proteins were detected at 72 hours after induction, in the supernatant, as pure bands between 60~70 kDa with hyperglycosylation. Regarding diagnosis potential, recombinant antigens had high specificity (95.6%); however, sensitivity was 55.6% for rTES-30 and 68.9% for rTES-120. Further deglycosylation of the P. pastoris antigens did not seem to affect ELISA performance (p0.05). The low sensitivity in the serodiagnosis diminished any advantage that P. pastoris expression could have. Therefore, we do not recommend P. pastoris recombinant TES production as an alternative for the diagnosis of toxocariasis.
展开▼
机译:重组蛋白是诊断毒性病毒的建议选择。目前的大肠杆菌重组蛋白过表达系统通常产生不溶性产物。作为替代方案,酵母如匹氏牧场等酵母具有分泌机制,可以减少生产成本和时间。本研究旨在在Pichia Pastoris中产生重组蛋白质,并在间接ELISA测定中验证它们的敏感性和特异性。在PPICZαB载体中克隆了毒素甘露油排泄分泌抗原的两个序列(RTES-30和RTES-120),并在P. Pastoris km71h中表达。从受毒素SPP感染的人类成年人收集的血清样本。通过TRES-30和RTES-120作为抗原的间接ELISA测试。在诱导后72小时在上清液后72小时检测重组蛋白,如60〜70kDa的纯条带,高糖基化。关于诊断潜力,重组抗原具有高特异性(95.6%);然而,对于rtes-30和68.9%的敏感性为55.6%,对于rtes-120。 P. Pastoris抗原的进一步脱糖基化似乎似乎不会影响ELISA性能(P> 0.05)。血清诊断的低灵敏度降低了P.牧场表达可能具有的任何优点。因此,我们不推荐P. Pastoris重组TES作为诊断毒性病毒的替代品。
展开▼
