Khoury G, May E
J Virol. 1977 Jul;23(1):167-76. doi: 10.1128/JVI.23.1.167-176.1977.
Virus-specific RNA synthesized in monkey cells after infection by both wild-type simian virus 40 (SV40) and the early SV40 temperature-sensitive mutant tsA58 has been analyzed. The fraction of SV40-specific RNA increased throughout infection with either wild-type SV40 or with tsA58 in direct proportion to the accumulation of progeny DNA molecules, suggesting their role in the late transcriptional process. Cytoplasmic fractions from cells infected at various temperatures (31.5 to 41 degrees C) by wild-type virus and harvested 48 h later contained 4 to 8% virus-specific RNA, of which 5 to 10% was early SV40 RNA. In contrast, though 5 to 8% of the cytoplasmic RNA from tsA 58-infected cells incubated at 31.5 to 37 degrees C for 48 h was virus specific, the percentage of early virus-specific RNA ranged from 25 to 80% as the incubation temperature increased. In tsA58-infected cultures incubated for 48 h at 41 degrees C (a temperature at which essentially no tsA 58 DNA synthesis occurred), only 0.4% of the cytoplasmic RNA was virus specific, but at least 90% of this RNA was early. In experiments where cells were inoculated at 32 degrees C and shifted at 48 h postinfection to 40 degrees C for various times, the percentage of virus-specific pulse-labeled RNA varied from 3.5 to 10.0%. Of the virus-specific RNA, early SV40 RNA ranged from 14 to 65% in tsA 58-infected cultures. Analogous studies with Sarkosyl-extracted viral transcription complexes to incorporate label into nascent (unprocessed) viral RNA yielded essentially identical results. This finding strongly suggests that the overproduction of early SV40 RNA occurs at the level of synthesis. While cytosine arabinoside effectively terminated most viral DNA replication in wild-type-infected cells, the ratio of early to late viral RNA remained less than 1:9. These results demonstrate that: (1) the amount of virus-specific RNA synthesized depends directly on the amount of viral DNA available for use as templates; once viral DNA replication has occurred, presumably providing progeny SV40 DNA molecules for templates, the level of transcription remains high; (ii) termination of viral DNA replication does not terminate late SV40 transcription; (iii) early SV40 RNA is overproduced by tsA 58 at all temperatures, but especially at higher temperatures; and (iv) overproduction of early SV40 RNA appears to be correlated with defectiveness of the tsA mutant T-antigen. These results suggest that T-antigen may regulate its own production either by repressing the synthesis of early viral RNA or by stimulating the synthesis of late SV40 RNA or both.
对野生型猿猴病毒40(SV40)和早期SV40温度敏感突变体tsA58感染后在猴细胞中合成的病毒特异性RNA进行了分析。在野生型SV40或tsA58感染的整个过程中,SV40特异性RNA的比例与子代DNA分子的积累成正比增加,表明它们在晚期转录过程中发挥作用。在不同温度(31.5至41摄氏度)下被野生型病毒感染并在48小时后收获的细胞的细胞质部分含有4%至8%的病毒特异性RNA,其中5%至10%是早期SV40 RNA。相比之下,虽然在31.5至37摄氏度下孵育48小时的tsA 58感染细胞的细胞质RNA中有5%至8%是病毒特异性的,但随着孵育温度的升高,早期病毒特异性RNA的百分比范围为25%至80%。在41摄氏度(基本上没有tsA 58 DNA合成发生的温度)下孵育48小时的tsA58感染培养物中,只有0.4%的细胞质RNA是病毒特异性的,但至少90%的这种RNA是早期的。在细胞于32摄氏度接种并在感染后48小时转移至40摄氏度不同时间的实验中,病毒特异性脉冲标记RNA的百分比从3.5%至10.0%不等。在tsA 58感染的培养物中,病毒特异性RNA中的早期SV40 RNA范围为14%至65%。用十二烷基肌氨酸钠提取的病毒转录复合物进行类似研究,将标记掺入新生(未加工)病毒RNA中,得到了基本相同的结果。这一发现强烈表明,早期SV40 RNA的过量产生发生在合成水平。虽然阿糖胞苷有效地终止了野生型感染细胞中的大多数病毒DNA复制,但早期与晚期病毒RNA的比例仍小于l:9。这些结果表明:(1)合成的病毒特异性RNA的量直接取决于可作为模板使用的病毒DNA的量;一旦发生病毒DNA复制,大概为子代SV40 DNA分子提供了模板,转录水平就会保持较高;(ii)病毒DNA复制的终止不会终止晚期SV40转录;(iii)tsA 58在所有温度下,尤其是在较高温度下,都会过量产生早期SV40 RNA;(iv)早期SV40 RNA的过量产生似乎与tsA突变体T抗原的缺陷有关。这些结果表明,T抗原可能通过抑制早期病毒RNA的合成或刺激晚期SV40 RNA的合成或两者兼而有之来调节其自身的产生。
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