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马疱疹病毒体内外感染马单核细胞后细胞内病毒感染中心测定及感染性病毒滴度测定

Infectious center assay of intracellular virus and infective virus titer for equine mononuclear cells infected in vivo and in vitro with equine herpesviruses.

作者信息

Dutta S K, Myrup A C

出版信息

Can J Comp Med. 1983 Jan;47(1):64-9.

Abstract

A novel, simple method of infectious center assay was developed to detect and quantitate the intracellular existence of equine herpesvirus 1 and equine herpesvirus 2 in peripheral blood mononuclear cells infected in vivo and in vitro with the viruses by cocultivation of these cells with a permissive equine cell culture. The infectious center titers were correlated with the infectious virus titers. In vivo equine herpesvirus 1-infected mononuclear cells obtained from ponies experimentally infected with the virus and equine herpesvirus 2-infected mononuclear cells obtained from selected naturally infected ponies with the virus gave by infectious center assay a mean value of 67 infectious center/2 x 10(6) cells as a peak titer on day 4 postinfection and 26 infectious center/2 x 10(6) cells for equine herpesvirus 1 and equine herpesvirus 2 respectively. The mononuclear cells, in both cases, did not contain detectable infectious virus, but the infectious virus was detected from the respective cells when they were cultured in the presence of mitogen. The equine herpesvirus 1 infected mononuclear cells in culture gave a mean count of 8.05 x 10(2) infectious center/2 x 10(6) cells/mL and contained 1.08 x 10(4) plague assay/mL of infectious virus. Similarly the equine herpesvirus 2 infected mononuclear cells in culture gave a mean count of 7.1 x 10(1) infectious center/2 x 10(6) cells/mL and contained <10(1) tissue culture infective dose(50)/mL of infectious virus. Mononuclear cells infected in vitro with equine herpesvirus 1 gave a mean count of 9.3 x 10(4) infectious center/2 x 10(6) cells/mL and contained 5.75 x 10(3) plaque assay/mL of infectius virus. Culturing these cells in the presence of mitogen gave a mean count of 5.5 x 10(3) infectious center/2 x 10(6) cells/mL and contained 9 x 10(3) plague assay/mL of infectious virus. A correlation between infectious center assay and infectious virus assay is discussed.

摘要

开发了一种新颖、简单的感染中心测定方法,通过将外周血单核细胞与允许性马细胞培养物共培养,来检测和定量体内和体外感染马疱疹病毒1和马疱疹病毒2的外周血单核细胞内的病毒存在情况。感染中心滴度与感染性病毒滴度相关。通过感染中心测定,从实验感染该病毒的小马获得的体内感染马疱疹病毒1的单核细胞以及从选定的自然感染该病毒的小马获得的感染马疱疹病毒2的单核细胞,在感染后第4天的峰值滴度分别为平均67个感染中心/2×10⁶个细胞,马疱疹病毒1和马疱疹病毒2分别为26个感染中心/2×10⁶个细胞。在这两种情况下,单核细胞均未检测到可检测到的感染性病毒,但当它们在有丝分裂原存在的情况下培养时,可从相应细胞中检测到感染性病毒。培养中的感染马疱疹病毒1的单核细胞平均计数为8.05×10²个感染中心/2×10⁶个细胞/毫升,含有1.08×10⁴个蚀斑测定/毫升的感染性病毒。同样,培养中的感染马疱疹病毒2的单核细胞平均计数为7.1×10¹个感染中心/2×10⁶个细胞/毫升,含有<10¹个组织培养感染剂量(50)/毫升的感染性病毒。体外感染马疱疹病毒1的单核细胞平均计数为9.3×10⁴个感染中心/2×10⁶个细胞/毫升,含有5.75×10³个蚀斑测定/毫升的感染性病毒。在有丝分裂原存在的情况下培养这些细胞,平均计数为5.5×10³个感染中心/2×10⁶个细胞/毫升,含有9×10³个蚀斑测定/毫升的感染性病毒。讨论了感染中心测定与感染性病毒测定之间的相关性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e1e5/1235886/59243b9bd8e6/compmed00009-0068-a.jpg

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