首页> 美国卫生研究院文献>Journal of Virology >Characterization of a DNA-protein complex and capsomere subunits derived from polyoma virus by treatment with ethyleneglycol-bis-NN-tetraacetic acid and dithiothreitol.
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Characterization of a DNA-protein complex and capsomere subunits derived from polyoma virus by treatment with ethyleneglycol-bis-NN-tetraacetic acid and dithiothreitol.

机译:通过用乙二醇-双-NN-四乙酸和二硫苏糖醇处理从多瘤病毒衍生的DNA-蛋白质复合物和帽体亚单位的表征。

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摘要

Treatment of polyoma virions with ethyleneglycol-bil-N,N'-tetraacetic acid (EGTA) and dithiothreitol (DTT) at pH 8.5 resulted in the dissociation of the virions into a DNA-protein complex and individual structural capsomere subunits. The sedimentation value of the DNA-protein complex in sucrose gradients was approximately 48S, and it had a density of 1.45 g/cm3 in equilibrium CsCl gradients. Alkaline sucrose analysis of the DNA within this DNA-protein complex demonstrated that approximately 75% of the DNA is component 1. The proteins associated with the DNA were dissociated by treatment with either NaCl or the anionic detergent Sarkosyl. VP1 and the histone proteins VP 4--7 were the major proteins associated with the DNA. Treatment of the DNA-protein complex with alkaline pH resulted in the specific removal of FP1. Electron microscopy of the 48S DNA-protein complex demonstrated that it is a very tightly coiled structure that is slightly larger than the intact virion. Treatment of the complex with either NaCl or with pH 10.5 buffer resulted in the loss of protein and subsequent loosening of the DNA-protein complex such that the DNA could be visualized. The capsomere subunits released as a result of the EGTA-DTT treatment sedimented as 18S, 12S, and 5S subunits in sucrose gradients. Electrophoretic analysis of the isolated capsomeres demonstrated that VP1, VP2, and VP3 were present in each species, although the ratios of the proteins varied. In addition to the structural proteins, histones VP 4--7 were found to be predominantly associated with the 5S capsomere subunit.
机译:用乙二醇-bil-N-N,N'-四乙酸(EGTA)和二硫苏糖醇(DTT)在pH 8.5下处理多瘤病毒粒子导致病毒粒子解离为DNA-蛋白质复合物和单个结构性帽泡亚基。 DNA-蛋白质复合物在蔗糖梯度中的沉降值约为48S,在平衡CsCl梯度中的密度为1.45 g / cm3。对该DNA-蛋白质复合物中DNA的碱性蔗糖分析表明,大约75%的DNA是组分1。与DNA相关的蛋白质通过用NaCl或阴离子去污剂Sarkosyl处理而解离。 VP1和组蛋白VP 4--7是与DNA相关的主要蛋白质。用碱性pH处理DNA-蛋白质复合物可导致FP1的特异性清除。 48S DNA-蛋白质复合物的电子显微镜显示,它是一个非常紧密的盘绕结构,比完整的病毒体稍大。用NaCl或pH 10.5缓冲液处理该复合物会导致蛋白质损失,随后使DNA-蛋白质复合物变松,从而可以看到DNA。由于EGTA-DTT处理而释放的衣壳状亚基以蔗糖梯度沉积为18S,12S和5S亚基。对分离的衣壳体的电泳分析表明,尽管蛋白质的比例不同,但每个物种中都存在VP1,VP2和VP3。除了结构蛋白外,还发现组蛋白VP 4--7主要与5S capsomere亚基相关。

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