Establishment of a line of human fetal glial cells that supports JC virus multiplication.
- 1 February 1985
- journal article
- research article
- Published by Proceedings of the National Academy of Sciences in Proceedings of the National Academy of Sciences
- Vol. 82 (4) , 1257-1261
- https://doi.org/10.1073/pnas.82.4.1257
Abstract
Primary cultures of human fetal brain cells were transfected with plasmid DNA pMK16, containing an origin-defective mutant of simian virus 40 (SV40). Several weeks after DNA treatment, proliferation of glial cells was evident in the culture, allowing passage of the cells at low split ratios. Initially, only 10% of the cells demonstrated nuclear fluorescence staining using a hamster tumor antibody to the SV40 T protein. By the sixth passage, however, 100% of the cells reacted positively to the same antibody. During these early passages, the cells designated SVG began growing very rapidly and acquired a homogeneous morphology. Cell division required only low serum concentrations, was not contact-inhibited, and remained anchorage dependent. These characteristics of the SVG cells have been stable through 25 passages or approximately equal to 80 cell generations. The SV40 T protein is continuously produced in the cells and can direct the replication of DNA inserts in the pSV2 vector, determined by in situ hybridization using biotin-labeled DNA probes, which contains the SV40 replication origin. More importantly, SVG cells support the multiplication of the human papovavirus JCV at levels comparable to primary cultures of human fetal glial cells, producing infectious virus as early as 1 week after viral adsorption. Their brain-cell derivation has been established as astroglial, based on their reactivity with a monoclonal antibody to glial fibrillary acid protein and lack of activity with an anti-galactocerebroside antibody, which identifies oligodendroglial cells. The SVG cells represent a unique line of continuous rapidly growing human fetal astroglial cells that synthesizes a replication-proficient SV40 T protein. Their susceptibility to JC virus (JCV) infection obviates a host restriction barrier that limited JCV studies to primary cultures of human fetal brain and thus should allow for more detailed molecular studies of human brain cells and JCV that infects them.This publication has 29 references indexed in Scilit:
- SV40-transformed simian cells support the replication of early SV40 mutantsCell, 1981
- Origin-defective Mutants of SV40Published by Cold Spring Harbor Laboratory ,1980
- Human brain in tissue culture. III. PML‐SV40‐induced transformation of brain cells and establishment of permanent linesJournal of Comparative Neurology, 1975
- A new technique for the assay of infectivity of human adenovirus 5 DNAVirology, 1973
- Nature of Col E 1 plasmid replication in Escherichia coli in the presence of the chloramphenicol.1972
- CULTIVATION OF PAPOVA-LIKE VIRUS FROM HUMAN BRAIN WITH PROGRESSIVE MULTIFOCAL LEUCOENCEPHALOPATHYThe Lancet, 1971
- A dye-buoyant-density method for the detection and isolation of closed circular duplex DNA: the closed circular DNA in HeLa cells.Proceedings of the National Academy of Sciences, 1967
- Transformation of Astrocytes and Destruction of Spongioblasts Induced by a Simian Tumor Virus (SV40) in Cultures of Human Fetal Neuroglia*†‡Journal of Neuropathology and Experimental Neurology, 1967
- Propagation of human fetal spongioblasts and astrocytes in dispersed cell culturesExperimental Cell Research, 1965
- PROGRESSIVE MULTIFOCAL LEUKO-ENCEPHALOPATHYBrain, 1958