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从仙台病毒中分离出的一种糖蛋白融合素的特性研究。

Characterization of a glycoprotein fusogen isolated from Sendai virus.

作者信息

Kruse C A, Wisnieski B J, Popják G

出版信息

Biochim Biophys Acta. 1984 Jan 24;797(1):40-50. doi: 10.1016/0304-4165(84)90380-5.

Abstract

After isolation from Sendai virus, the glycoproteins HN and F retained their ability to induce hemagglutination and both heterologous and homologous cell-cell fusion. Both methods for demonstrating cell fusion indicated that the isolated HN and F glycoproteins compared favorably with whole Sendai virus as a fusogen. Conditions affecting the degree of fusion were examined and optimized. Whole virus and isolated glycoprotein preparations were characterized by electron microscopy and by SDS-polyacrylamide gel electrophoresis. Lipid analysis of the glycoprotein preparations by thin layer chromatography and gas chromatography/mass spectrometry indicated that they were partially lipid-depleted during the isolation protocol and the ratio of cholesterol to phospholipid was higher than in the whole virus. A complete fatty acid analysis was performed on lipid extracts from whole virus and from glycoprotein preparations. Detergent was removed from the glycoproteins by dialysis and by incubation with Amberlite XAD-2 resin. The detergent content of the glycoprotein preparations was monitored by gas chromatography and with [3H]Triton X-100. Both methods showed that virtually all (greater than or equal to 99.8%) of the originally added detergent was removed. Electron microscopy of the negatively-stained HN and F preparations showed primarily spherical particles 120 +/- 20 A in diameter (range 80-250 A). Since no organization reminiscent of envelopes could be demonstrated, we conclude that the fusogenic activity of Sendai virus resides in the glycoproteins per se rather than in bilayer integrated lipid-protein complexes.

摘要

从仙台病毒中分离出来后,糖蛋白HN和F保留了其诱导血凝以及异源和同源细胞 - 细胞融合的能力。两种证明细胞融合的方法均表明,分离出的HN和F糖蛋白作为融合剂与完整的仙台病毒相比毫不逊色。研究并优化了影响融合程度的条件。通过电子显微镜和SDS - 聚丙烯酰胺凝胶电泳对完整病毒和分离出的糖蛋白制剂进行了表征。通过薄层色谱法以及气相色谱/质谱法对糖蛋白制剂进行脂质分析表明,在分离过程中它们部分脂质缺失,且胆固醇与磷脂的比例高于完整病毒。对完整病毒和糖蛋白制剂的脂质提取物进行了完整的脂肪酸分析。通过透析以及与Amberlite XAD - 2树脂孵育从糖蛋白中去除去污剂。通过气相色谱法以及使用[3H] Triton X - 100监测糖蛋白制剂的去污剂含量。两种方法均表明几乎所有(大于或等于99.8%)最初添加的去污剂都被去除了。对经负染的HN和F制剂进行电子显微镜观察,主要显示直径为120±20 Å(范围80 - 250 Å)的球形颗粒。由于未发现类似包膜的结构,我们得出结论,仙台病毒的融合活性存在于糖蛋白本身而非双层整合的脂蛋白复合物中。

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