Abrahams P J, Mulder C, Van De Voorde A, Warnaar S O, van der Eb A J
J Virol. 1975 Oct;16(4):818-23. doi: 10.1128/JVI.16.4.818-823.1975.
Linear simian virus 40 (SV40) DNA molecules of genome length and DNA fragments smaller than genome length when prepared with restriction endonucleases and tested for transforming activity on primary cultures of baby rat kidney cells. The linear molecules of genome length (prepared with endonucleases R-EcoRI, R-BamHI, and R-HpaII or R-HapII), a 74% fragment (EcoRI/HpaII or HapII-A), and a 59% fragment (BamHI/HapII-A) could all transform rat kidney cells with the same efficiency as circular SV40 DNA. All transformed lines tested contained the SV40-specific T-antigen in 90 to 100% of the cells, which was taken as evidence that the transformation was SV40 specific. The DNA fragments with transforming activity contained the entire early region of SV40 DNA. Endo R-HpaI, which introduced one break in the early region, apparently inactivated the transforming capacity of SV40 DNA, since no transformation was observed with any of the three HpaI fragments tested. Attempts were made to rescue infectious virus from some of the transformed lines by fusion with permissive BSC-1 cells. Infectious virus was only recovered from the cells transformed by circular form I DNA. No infectious virus could be isolated from any of the other types of transformed cells.
用限制性内切酶制备的基因组长度的线性猿猴病毒40(SV40)DNA分子以及小于基因组长度的DNA片段,在原代新生大鼠肾细胞培养物上检测其转化活性。基因组长度的线性分子(用内切酶R-EcoRI、R-BamHI和R-HpaII或R-HapII制备)、一个74%的片段(EcoRI/HpaII或HapII-A)和一个59%的片段(BamHI/HapII-A)都能以与环状SV40 DNA相同的效率转化大鼠肾细胞。所有测试的转化细胞系在90%至100%的细胞中含有SV40特异性T抗原,这被视为转化是SV40特异性的证据。具有转化活性的DNA片段包含SV40 DNA的整个早期区域。内切酶R-HpaI在早期区域引入了一个切口,显然使SV40 DNA的转化能力失活,因为在所测试的三个HpaI片段中均未观察到转化。尝试通过与允许性BSC-1细胞融合从一些转化细胞系中拯救感染性病毒。仅从由环状I型DNA转化的细胞中回收了感染性病毒。从任何其他类型的转化细胞中均未分离出感染性病毒。
