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荧光细胞计数作为呼吸道合胞病毒的一种检测方法。

Fluorescent cell counting as an assay method for respiratory syncytial virus.

作者信息

Schieble J H, Kase A, Lennette E H

出版信息

J Virol. 1967 Jun;1(3):494-9. doi: 10.1128/JVI.1.3.494-499.1967.

Abstract

The fluorescent cell-counting technique was applied to the enumeration of cell-infecting units of respiratory syncytial (RS) virus in human fetal diploid (HFD) cover-slip cell cultures; it was a sensitive, precise, and rapid assay method. Approximately 2 hr was required for maximal adsorption of RS virus to HFD cell monolayers. However, about 15% of the infectious virus in the inoculum remained unadsorbed; this percentage was not significantly reduced even when the adsorption period was extended to 5 hr. A linear relationship between virus concentration and the number of fluorescent cells existed over a range of 1.2 log(10) units. Variation of the mean of replicate determinations in a single experiment was approximately 7.5%. The distribution of single infected HFD cells on cover-slip cell cultures corresponded with the calculated frequencies of the Poisson distribution. The Chi square test for the extent of fit was calculated for several experiments, and the value of P was never less than 0.5. The addition of immune serum after virus adsorption effectively inhibited the development of detectable levels of viral antigen in secondarily infected cells.

摘要

荧光细胞计数技术被应用于在人类胎儿二倍体(HFD)盖玻片细胞培养物中对呼吸道合胞(RS)病毒的细胞感染单位进行计数;这是一种灵敏、精确且快速的检测方法。RS病毒吸附到HFD细胞单层上达到最大吸附量大约需要2小时。然而,接种物中约15%的感染性病毒仍未被吸附;即使将吸附时间延长至5小时,这一百分比也没有显著降低。在1.2个对数(10)单位的范围内,病毒浓度与荧光细胞数量之间存在线性关系。在单个实验中,重复测定的平均值的变异约为7.5%。盖玻片细胞培养物上单个感染的HFD细胞的分布与泊松分布的计算频率相符。对多个实验计算了拟合程度的卡方检验,P值从未小于0.5。病毒吸附后添加免疫血清可有效抑制二次感染细胞中可检测水平的病毒抗原的产生。

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