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猿猴病毒40转化细胞的克隆系自发产生病毒以及突变猿猴病毒40株的脱氧核糖核酸超感染的影响。

Spontaneous virus production by clonal lines of siminan virus 40-transformed cells and effects of superinfection by deoxyribonucleic acid from mutant simian virus 40 strains.

作者信息

Dubbs D R, Kit S

出版信息

J Virol. 1971 Oct;8(4):430-6. doi: 10.1128/JVI.8.4.430-436.1971.

Abstract

Small amounts of infectious simian virus 40 (SV40) were recovered from parental cultures of SV40-transformed human embryonic lung (WI38 Va13A) cells, from 12 primary clones, from 17 secondary clones, and from 18 tertiary clones. The cloning experiments demonstrated that the capacity for spontaneous virus production is a hereditary property of WI38 Va13A cells. Infectious virus was not recovered from every clone at every passage. Repeated trials at different passage levels were necessary to detect virus production. Approximately one in 10(5) to 10(6) of the cells of the clonal lines initiated plaque formation when plated on the CV-1 line of African green monkey kidney cells. No increase in infectious center formation was observed after the clonal lines were treated with bromodeoxyuridine, iododeoxyuridine, or mitomycin C or after heterokaryon formation of treated cells with CV-1 cells. The clonal lines of WI38 Va13A cells were susceptible to superinfection by SV40 deoxyribonucleic acid (DNA). To determine whether only those cells which spontaneously produced virus supported the replication of superinfecting SV40 DNA, cultures were infected with DNA from a plaque morphology mutant and a temperature-sensitive mutant of SV40. After infection by SV40 DNA, approximately 100 to 4,400 times more transformed cells formed infectious centers than were spontaneously producing virus. To determine whether the resident SV40 genome or the superinfecting SV40 genome was replicating, infectious centers produced by SV40 DNA-infected WI38 Va13A cells on CV-1 monolayers were picked and the progeny virus was analyzed. Only the superinfecting SV40 was recovered from the infectious centers, indicating that in the majority of superinfected cells the resident SV40 was not induced to replicate.

摘要

从猴空泡病毒40(SV40)转化的人胚肺(WI38 Va13A)细胞的亲代培养物、12个一级克隆、17个二级克隆和18个三级克隆中回收了少量感染性SV40。克隆实验表明,自发产生病毒的能力是WI38 Va13A细胞的一种遗传特性。并非每次传代时每个克隆都能回收感染性病毒。需要在不同传代水平进行重复试验以检测病毒产生情况。当克隆系的细胞接种在非洲绿猴肾细胞的CV - 1系上时,约每10⁵至10⁶个细胞中有一个启动蚀斑形成。在用溴脱氧尿苷、碘脱氧尿苷或丝裂霉素C处理克隆系后,或在用处理过的细胞与CV - 1细胞形成异核体后,未观察到感染中心形成增加。WI38 Va13A细胞的克隆系对SV40脱氧核糖核酸(DNA)的超感染敏感。为了确定是否只有那些自发产生病毒的细胞支持超感染的SV40 DNA的复制,用SV40的蚀斑形态突变体和温度敏感突变体的DNA感染培养物。用SV40 DNA感染后,形成感染中心的转化细胞比自发产生病毒的细胞多约100至4400倍。为了确定是驻留的SV40基因组还是超感染的SV40基因组在复制,挑选了由SV40 DNA感染的WI38 Va13A细胞在CV - 1单层上产生的感染中心,并分析子代病毒。从感染中心仅回收了超感染的SV40,这表明在大多数超感染细胞中,驻留的SV40未被诱导复制。

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