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人红系骨髓细胞在体外被B19细小病毒有效感染。

Productive infection by B19 parvovirus of human erythroid bone marrow cells in vitro.

作者信息

Ozawa K, Kurtzman G, Young N

出版信息

Blood. 1987 Aug;70(2):384-91.

PMID:3038211
Abstract

B19 parvovirus, the cause of fifth disease and transient aplastic crisis, has been successfully propagated in suspension cultures of human erythroid bone marrow cells obtained from patients with sickle cell disease and stimulated by erythropoietin. B19 inoculation in vitro resulted in a marked decline in identifiable erythroid cells over seven to nine days of incubation. Characteristic giant early erythroid cells were seen on Wright's-Giemsa stain of infected cultures. By in situ hybridization, 30% to 40% of erythroblasts were infected at 48 hours; a similar proportion of cells showed B19 capsid protein by immunofluorescence. B19 DNA was present in erythroblasts but not in the leukocyte fraction of bone marrow. B19 replication, as determined by Southern analysis, and B19 encapsidation, as determined by sensitivity of isolated cell fractions to DNase I, were restricted to the nuclei. B19 DNA was detectable in the nuclei from infected cultures beginning at 18 hours and in the supernatant at 32 hours; B19 genome copy number was estimated at about 25,000 to 30,000/infected cell at 48 hours. Recovery of virus depended on the multiplicity of infection (moi); at low moi, approximately 200x input virus was recovered from total cultures and 50x from the culture supernatants. Virus released into the supernatant was as infectious or more infectious than virus obtained from sera of infected patients. Human erythroid bone marrow culture represents a safe in vitro system for the elucidation of the cellular and molecular biology of the pathogenic B19 parvovirus.

摘要

B19细小病毒是传染性红斑和暂时性再生障碍危象的病原体,已在从镰状细胞病患者获取并经促红细胞生成素刺激的人红系骨髓细胞悬浮培养物中成功繁殖。体外接种B19后,在七至九天的培养期内可识别的红系细胞显著减少。在感染培养物的瑞氏-吉姆萨染色中可见特征性的巨大早期红系细胞。通过原位杂交,48小时时30%至40%的成红细胞被感染;通过免疫荧光,类似比例的细胞显示有B19衣壳蛋白。B19 DNA存在于成红细胞中,但不存在于骨髓的白细胞部分。通过Southern分析确定的B19复制以及通过分离细胞组分对DNase I的敏感性确定的B19衣壳化均局限于细胞核。从18小时开始在感染培养物的细胞核中可检测到B19 DNA,32小时时在上清液中可检测到;在48小时时,估计每个感染细胞的B19基因组拷贝数约为25,000至30,000。病毒的回收取决于感染复数(moi);在低moi时,从总培养物中回收的病毒约为输入病毒的200倍,从培养上清液中回收的病毒约为输入病毒的50倍。释放到上清液中的病毒与从感染患者血清中获得的病毒具有相同或更高的传染性。人红系骨髓培养代表了一种用于阐明致病性B19细小病毒细胞和分子生物学的安全体外系统。

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