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多瘤病毒核蛋白复合物的分离与特性分析

Isolation and characterization of polyoma nucleoprotein complexes.

作者信息

Garcea R L, Benjamin T L

出版信息

Virology. 1983 Oct 15;130(1):65-75. doi: 10.1016/0042-6822(83)90118-6.

Abstract

A method for the isolation of polyoma nucleoprotein complexes has been developed using neuraminidase treatment of infected cell lysates. At least three distinct forms of polyoma virion intermediates were identified by their [3H]thymidine labeling kinetics and sedimentation coefficients: a rapidly labeled 95 S "replicating complex" which chases to a 75 S minichromosome and then to a 240 S virion structure. The general properties of these distinct intermediates were similar to those found for SV40. In contrast to SV40, however, a continuum of labeled polyoma viral DNA sedimented between 240 S and 95 S. These complexes were characterized by their release from cell debris with neuraminidase, precipitation with antivirion antibody, complete disruption in 1 M NaCl, and association with hemagglutinating (HA) activity. These intermediates may represent incremental capsid protein additions to the 75 S minichromosome, hypothesized in the current models for SV40 assembly. The ability to isolate a complete complement of polyoma subviral complexes provides a basis for studying the growth defect of polyoma host-range mutants, and the properties of neuraminidase release, hemagglutination, and specific immunoprecipitation suggest purification steps for further characterization of these virion assembly intermediates.

摘要

一种分离多瘤病毒核蛋白复合物的方法已经开发出来,该方法是对感染细胞裂解物进行神经氨酸酶处理。通过其[3H]胸腺嘧啶标记动力学和沉降系数鉴定出至少三种不同形式的多瘤病毒体中间体:一种快速标记的95S“复制复合物”,它追踪到一个75S的微型染色体,然后到一个240S的病毒体结构。这些不同中间体的一般特性与SV40的相似。然而,与SV40不同的是,在240S和95S之间沉降的标记多瘤病毒DNA是连续的。这些复合物的特征在于它们可通过神经氨酸酶从细胞碎片中释放出来,能用抗病毒体抗体沉淀,在1M NaCl中完全破坏,并与血凝(HA)活性相关。这些中间体可能代表了向75S微型染色体逐步添加衣壳蛋白,这是当前SV40组装模型中所假设的。分离完整的多瘤病毒亚病毒复合物的能力为研究多瘤病毒宿主范围突变体的生长缺陷提供了基础,并且神经氨酸酶释放、血凝和特异性免疫沉淀的特性为进一步表征这些病毒体组装中间体的纯化步骤提供了依据。

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