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Two antiviral proteins from tobacco: purification and characterization by monoclonal antibodies to human beta-interferon.

机译:来自烟草的两种抗病毒蛋白:通过针对人β-干扰素的单克隆抗体进行纯化和鉴定。

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摘要

Polyclonal antibodies to human beta-interferon reacted specifically with two plant proteins (gp22 and gp35) by Western blot analysis of crude protein extracts from tobacco leaves infected with tobacco mosaic virus. Immunoaffinity chromatography of these extracts on a column of immobilized monoclonal antibodies to human beta-interferon and then reversed-phase HPLC yielded gp22 and gp35 in a pure state. Both proteins reacted with the Schiff reagent and concanavalin A (indicating their glycoprotein nature) and exhibited antiviral activity (inhibiting tobacco mosaic virus replication in tobacco-leaf discs at concentrations of ng/ml). Each protein was cleaved by cyanogen bromide and the resultant peptides, separated by HPLC, were sequenced as far as the Edman degradation allowed, giving a total of 61 amino acid residues for gp22 and 105 residues for gp35, which represent 30-50% of their expected length. Computer analyses of the sequenced segments revealed no significant homology to human beta-interferon, each other, or any other recorded sequence.
机译:通过对被烟草花叶病毒感染的烟叶中的粗蛋白提取物进行蛋白质印迹分析,针对人β-干扰素的多克隆抗体与两种植物蛋白(gp22和gp35)发生特异性反应。在固定的抗人β-干扰素单克隆抗体柱上对这些提取物进行免疫亲和层析,然后进行反相HPLC,得到纯净状态的gp22和gp35。两种蛋白质均与Schiff试剂和伴刀豆球蛋白A反应(表明其糖蛋白性质),并表现出抗病毒活性(以ng / ml的浓度抑制烟草叶盘中的烟草花叶病毒复制)。每种蛋白质均被溴化氰裂解,并在允许的埃德曼降解条件下对通过HPLC分离的肽进行测序,得到gp22共有61个氨基酸残基,gp35共有105个氨基酸残基,占其30%至50%预期的长度。对测序片段的计算机分析表明与人β-干扰素,彼此或任何其他记录的序列均无显着同源性。

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