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在脑心肌炎病毒感染的HeLa细胞中合成的病毒特异性蛋白。

Virus-specific proteins synthesized in encephalomyocarditis virus-infected HeLa cells.

作者信息

Butterworth B E, Hall L, Stoltzfus C M, Rueckert R R

出版信息

Proc Natl Acad Sci U S A. 1971 Dec;68(12):3083-7. doi: 10.1073/pnas.68.12.3083.

Abstract

The in vivo synthesis of encephalomyocarditis-specific proteins was studied by labeling the viral proteins with radioactive amino acids under conditions where host-protein synthesis was almost completely inhibited. To assure recovery of all proteins, intact cells were lysed in hot 1% sodium dodecyl sulfate. These lysates were analyzed by quantitative high-resolution electrophoresis on sodium dodecyl sulfate-polyacrylamide gels. This technique allowed the detection and estimation of the molecular weight of 15 virus-specific polypeptides: A, 100,000; B, 90,000; C, 84,000; D, 75,000, D1, 65,000; E, 56,000; epsilon, 40,000; F, 38,000; alpha, 34,000; beta, 30,000; gamma, 23,000; G, 16,000; H, 12,000; I, 11,000; and delta, 9,000. Pulse-chase experiments, in conjunction with cyanogen bromide and tryptic mapping of the isolated polypeptides, indicate that at least three primary gene products (A,F,C), with a cumulative weight of about 220,000, are generated during translation of the RNA genome. Chains A and C then undergo post-translational cleavages, while F remains uncleaved. The proteins generated by the cleavage of A include all of the capsid chains (alpha, beta, gamma, delta, epsilon). Those generated by the cleavage of C include D and E. The chains alpha, beta, gamma, delta, E, F, G, H, I, with a cumulative molecular weight of about 230,000, are stable and are produced in about equimolar amounts. A model for the synthesis of, and a cleavage sequence that accounts for, all of the viral polypeptides is proposed.

摘要

通过在宿主蛋白合成几乎完全被抑制的条件下用放射性氨基酸标记病毒蛋白,研究了脑心肌炎特异性蛋白的体内合成。为确保所有蛋白的回收,完整细胞在热的1%十二烷基硫酸钠中裂解。这些裂解物通过在十二烷基硫酸钠-聚丙烯酰胺凝胶上进行定量高分辨率电泳进行分析。该技术能够检测和估计15种病毒特异性多肽的分子量:A,100,000;B,90,000;C,84,000;D,75,000;D1,65,000;E,56,000;ε,40,000;F,38,000;α,34,000;β,30,000;γ,23,000;G,16,000;H,12,000;I,11,000;以及δ,9,000。脉冲追踪实验,结合对分离多肽的溴化氰和胰蛋白酶图谱分析,表明在RNA基因组翻译过程中产生了至少三种初级基因产物(A、F、C),其累积重量约为220,000。然后A链和C链经历翻译后切割,而F链保持未切割状态。A链切割产生的蛋白包括所有衣壳链(α、β、γ、δ、ε)。C链切割产生的蛋白包括D和E。α、β、γ、δ、E、F、G、H、I链,其累积分子量约为230,000,是稳定的,且以大约等摩尔量产生。提出了一个解释所有病毒多肽合成及切割序列的模型。

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