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Establishment of Stably Transfected Cells Constitutively Expressing the Full-Length and Truncated Antigenic Proteins of Two Genetically Distinct Mink Astroviruses

机译:构建表达两种遗传性水貂星状病毒的全长和截短的抗原蛋白的稳定转染细胞的建立

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摘要

Astroviruses are becoming a growing concern in veterinary and public health. To date there are no registered vaccines against astrovirus-induced disease, mostly due to the difficulty to cultivate astroviruses to high titer for vaccine development using conventional techniques. As means to circumvent this drawback, we have developed stably transfected mink fetal cells and BHK21 cells constitutively expressing the full-length and truncated capsid proteins of two distinct genotypes of mink astrovirus. Protein expression in these stably transfected cells was demonstrated by strong signals as evaluated by in-situ PLA and IFA, and confirmed by Western blotting. The recombinant full-length and truncated proteins induced a high level of antibodies in mink, evaluated by ELISA, demonstrating their immunogenicity. In a challenge experiment in mink, a reduction in presentation clinical signs and virus shedding was observed in mink kits born from immunized females. The gene integration and protein expression were sustained through cell passage, showing that the used approach is robust and reliable for expression of functional capsid proteins for vaccine and diagnostic applications.
机译:在兽医和公共卫生中,星状病毒正变得日益受到关注。迄今为止,还没有针对星状病毒引起的疾病的注册疫苗,这主要是由于难以使用常规技术将星状病毒培养到高滴度来开发疫苗。作为规避此缺陷的手段,我们开发了稳定转染的水貂胎儿细胞和BHK21细胞,组成型表达了两种不同基因型的水貂星状病毒的全长和截短的衣壳蛋白。通过原位PLA和IFA评估的强信号证明了这些稳定转染的细胞中的蛋白质表达,并通过Western印迹证实了这一点。重组全长和截短蛋白通过ELISA评估,在貂皮中诱导了高水平的抗体,证明了它们的免疫原性。在貂皮的挑战实验中,在从免疫雌性出生的貂皮试剂盒中观察到临床症状和病毒脱落的减少。基因整合和蛋白质表达通过细胞传代得以维持,这表明所使用的方法对于用于疫苗和诊断应用的功能性衣壳蛋白的表达是可靠且可靠的。

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