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猫杯状病毒与培养细胞的早期相互作用。

Early interaction of feline calicivirus with cells in culture.

作者信息

Kreutz L C, Seal B S, Mengeling W L

机构信息

Virology Swine Research Unit, National Animal Disease Center, USDA, Ames, Iowa.

出版信息

Arch Virol. 1994;136(1-2):19-34. doi: 10.1007/BF01538814.

Abstract

The kinetics and biochemical properties of feline calicivirus (FCV) attachment to Crandell-Reese feline kidney cells were determined. Maximum binding was observed at pH 6.5. Cells in suspension at 4 degrees C bound virus more efficiently than cells in monolayers at 4 degrees C or 37 degrees C. High initial binding rate was observed in monolayers or cells in suspension and proceeded to a maximum at 90 min, although half maximal binding was observed as early as 15 min. Binding was specific and competitively blocked by serotypically homologous or heterologous FCV as well as by San Miguel sea lion virus. Treatment of cells with proteases increased FCV binding, whereas phospholipase had no effect on virus attachment. Conversely, cells treated with neuraminidase followed by O-glycanase treatment showed a decreased binding ability. Cells of feline origin bound FCV very efficiently, and non-permissive cells showed a poor binding ability. Following transfection of viral RNA, infectious virus could be recovered from all non-permissive cells, except from Madin-Darby canine kidney cells. These results suggest that FCV binds to a receptor in which carbohydrates may be an important component and that FCV replication in non-permissive cells is primarily restricted by the absence of appropriate receptors on the cell surface.

摘要

测定了猫杯状病毒(FCV)与克兰德尔-里斯猫肾细胞结合的动力学和生化特性。在pH 6.5时观察到最大结合。4℃悬浮培养的细胞比4℃或37℃单层培养的细胞更有效地结合病毒。在单层或悬浮培养的细胞中观察到较高的初始结合率,在90分钟时达到最大值,尽管早在15分钟时就观察到半数最大结合。结合具有特异性,可被血清型同源或异源的FCV以及圣米格尔海狮病毒竞争性阻断。用蛋白酶处理细胞可增加FCV结合,而磷脂酶对病毒附着无影响。相反,先用神经氨酸酶处理细胞,再用O-聚糖酶处理,细胞的结合能力降低。猫源细胞非常有效地结合FCV,而不允许病毒复制的细胞结合能力较差。转染病毒RNA后,除了马-达二氏犬肾细胞外,所有不允许病毒复制的细胞都能回收感染性病毒。这些结果表明,FCV与一种受体结合,其中碳水化合物可能是重要组成部分,并且FCV在不允许病毒复制的细胞中的复制主要受细胞表面缺乏适当受体的限制。

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