Quantitative transformation of primate cells by PARA (defective SV40)-adenovirus type 7

## Abstract PARA (defective SV40) was transcapsidated from adenovirus type 7 to the highly oncogenic Huie strain of adenovirus type 12. This transfer of PARA to adenovirus 12 was found to hasten the appearance of SV40‐type tumors in hamsters inoculated as newborns; the tumors induced by the PARA‐ad

## Abstract A preparation of adenovirus 4, containing infectious SV40 genetic material enclosed within adenovirus coats (Ad. 4‐SV40 hybrid), induced both transformation of newborn hamster kidney cells in vitro and tumors in neonatally inoculated hamsters. Injection of transformed cells into an irra

## Abstract Untransformed, non‐tumorigenic mouse cells respond to cytochalasin B (CB) with limited nuclear division. BALB/c mouse embryo fibroblasts (MEF) and both BALB/c 3T3 and Swiss 3T3 cells become binucleated in the presence of CB and cells with three or more nuclei are very rare or undetectab

## Abstract Amplification of SV40 genes in SV40‐transformed Chinese hamster embryo cells (CO631) by chemical carcinogens as well as by herpes simplex virus infection can be inhibited by infection with the defective parvovirus, AAV‐5. This is shown by __in situ__ hybridization with SV40 DNA of AAV‐5

Co-culturing with origin-defective SV40 DNAinjected transformants, we succeeded in activating the limited growth potential of late-phase-II fibroblasts from patients with Werner's syndrome (WS cells). Residual life spans of three WS cell lines increased 2.3-5.6 fold. Co-culture with normal IMR-90 ce