Menna J H, Collins A R, Flanagan T D
Infect Immun. 1975 Jan;11(1):152-8. doi: 10.1128/iai.11.1.152-158.1975.
The parameters of a persistent-state measles virus infection in BGM/MV cells were examined. The BGM/MV cell line was established by cocultivation of measles virus-infected primary C3H mouse brain cells with a stable line of African green monkey kidney cells (BGM). Initially, a morphologically mixed population of cells existed:BGM-like (epithelioid) and fibroblasts. Gradually the fibroblasts were replaced by BGM-like cells, resulting in a morphologically homogeneous population. Measles cytopathic effect was noted 2 days after initiation of this culture and persisted for approximately 290 days. The time of disappearance of viral cytopathic effect corresponded to the time at which morphological homogeneity was reached. Low titers of infectious measles virus were detected in the BGM/MV culture up to 20 days postseeding; thereafter none was observed. After 440 days in culture, 100% of BGM/MV cells demonstrated intractyoplasmic measles antigen by immunofluorescence. Nuclear fluorescence was never observed. Electron microscopy revealed the presence of measles virus mucleocapsid within the almost completely filling the cytoplasm of BGM/MV cells. The plasma membrane of these cells appeared normal; no maturing or budding particles were observed. Measles virus hemagglutinin was not detected in either clarified cell lysates or in supernatant culture fluids. Cell membrane alteration by measles virus was detected in less than 1% of these cells by hemadsorption and by membrane immunofluorescence. The hemadsorption activity of the cells could be enhanced (30 to 70%) by treatment with actinomycin D or enucleation with cytochalasin B; these treatments, however, were unsuccessful in inducing detectable levels of measles hemagglutinin. Treatment of BGM/MV cells with 5-bromo-2'-deoxyuridine (BUdR) at 5 to 50 mug/ml and cytosine arabinoside at 1 to 50 mug/ml failed to enhance hemadsorption activity. Doses of 5-bromo-2'-deoxyuridine ranging from 5 to 200 mug/ml and of actinomycin D ranging from 0.1 to 10 mug/ml were ineffective in inducing the synthesis of infectious virus. Various physical methods of induction of infectious virus was also unsuccessful.
对BGM/MV细胞中持续状态麻疹病毒感染的参数进行了研究。BGM/MV细胞系是通过将感染麻疹病毒的原代C3H小鼠脑细胞与稳定的非洲绿猴肾细胞系(BGM)共培养而建立的。最初,存在形态学上混合的细胞群体:BGM样(上皮样)细胞和成纤维细胞。逐渐地,成纤维细胞被BGM样细胞取代,形成形态学上均一的细胞群体。在该培养开始2天后观察到麻疹细胞病变效应,并持续约290天。病毒细胞病变效应消失的时间与达到形态学均一性的时间一致。在接种后20天内,在BGM/MV培养物中检测到低滴度的感染性麻疹病毒;此后未观察到。培养440天后,100%的BGM/MV细胞通过免疫荧光显示胞浆内麻疹抗原。从未观察到核荧光。电子显微镜显示在几乎完全充满BGM/MV细胞胞浆的内部存在麻疹病毒核衣壳。这些细胞的质膜看起来正常;未观察到成熟或出芽颗粒。在澄清的细胞裂解物或上清培养液中均未检测到麻疹病毒血凝素。通过血细胞吸附和膜免疫荧光,在不到1%的这些细胞中检测到麻疹病毒引起的细胞膜改变。用放线菌素D处理或用细胞松弛素B去核可增强细胞的血细胞吸附活性(30%至70%);然而,这些处理未能诱导出可检测水平的麻疹血凝素。用5至50μg/ml的5-溴-2'-脱氧尿苷(BUdR)和1至50μg/ml的阿糖胞苷处理BGM/MV细胞未能增强血细胞吸附活性。5至200μg/ml的5-溴-2'-脱氧尿苷剂量和0.1至10μg/ml的放线菌素D剂量在诱导感染性病毒合成方面无效。各种诱导感染性病毒的物理方法也未成功。
