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Production of a Recombinant Major Inner Capsid Protein for Serological Detection of Epizootic Hemorrhagic Disease Virus

机译:重组主要内衣壳蛋白的生产用于血清学检测流行性出血病病毒

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摘要

Constructs of the major core protein, designated VP7, from epizootic hemorrhagic disease virus (EHDV) type 1 were made by amino- or carboxyl-terminal fusion of a six-histidine residue tag to the VP7-1 gene. The resulting fusion proteins were produced in a baculovirus expression system and purified by a rapid, one-step procedure using nickel-nitrilotriacetic acid technology. A high level of VP7-1 protein expression was detected with the N-terminal six-histidine tag fusion construct and was comparable to the level of expression observed with an untagged VP7-1 Bam construct. In contrast, the inclusion of a six-histidine tag at the C terminus adversely affected protein expression. The antigenicity of the N-terminal six-histidine tag EHDV VP7-1 product was identical to that observed with the native virus antigen and untagged EHDV VP7-1 recombinant protein, as determined by reactivity with EHDV specific antibodies in an enzyme-linked immunosorbent assay (ELISA) and Western blot. The high production and purity levels that can be attained for the N-terminal six-histidine tag VP7-1 protein and its reactivity with EHDV-specific sera in a competitive ELISA make it a suitable assay reagent.
机译:通过将六个组氨酸残基标签的氨基端或羧基端融合到VP7-1基因上,制成了1型流行性出血性疾病病毒(EHDV)的主要核心蛋白,命名为VP7。所得的融合蛋白在杆状病毒表达系统中产生,并使用镍-三三乙酸镍技术通过快速的一步步骤进行纯化。 N末端的六组氨酸标签融合构建体检测到高水平的VP7-1蛋白表达,与未标记的VP7-1 Bam构建体观察到的表达水平相当。相反,在C末端包含一个六组氨酸标签会对蛋白质表达产生不利影响。 N端六组氨酸标签EHDV VP7-1产物的抗原性与天然病毒抗原和未标记的EHDV VP7-1重组蛋白的抗原性相同,这是通过与EHDV特异性抗体在酶联免疫吸附测定中的反应性确定的(ELISA)和蛋白质印迹。 N末端六组氨酸标签VP7-1蛋白可获得高产量和纯度,并且在竞争性ELISA中与EHDV特异性血清具有反应性,因此使其成为合适的测定试剂。

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