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猿猴病毒40在允许细胞和非允许细胞中的基因表达调控机制。

Regulatory mechanism of simian virus 40 gene expression in permissive and in nonpermissive cells.

作者信息

Graessmann A, Graessmann M, Mueller C

出版信息

J Virol. 1976 Mar;17(3):854-8. doi: 10.1128/JVI.17.3.854-858.1976.

Abstract

Primary or continuous lines of mouse cells (3T3) are nonpermissive for simian virus 40 (SV40). Abortively infected cells synthesize tumor antigen (T antigen but not viral DNA and virus capsid protein (V antigen). V antigen, however, was obtained when SV40 DNA was injected into 3T3 cells. This late gene expression also appears to be correlated with the quantity of injected DNA molecules per 3T3 cell. T antigen formation can be detected after microinjection of only 1 to 2 DNA molecules, but the intensity of intranuclear T antigen fluorescence is significantly brighter with injection of higher concentrations of viral DNA. In permissive cells (TC7), early and late SV40 gene expression is directly related to the number of injected molecules. Microinjection of 1DNA molecule induced T and V antigen formation with the same efficiency as microinjection of 2,000 to 4,000 molecules. The question of weather late SV40 gene expression is directly related to the quantity of an early virus-specific product was approached by microinjection of early SV40 complementary RNA together with small amounts of viral DNA. V antigen was obtained in a high proportion of recipient 3T3 cells at conditions where microinjection of viral DNA alone induced T but not V antigen synthesis.

摘要

小鼠细胞系(3T3)的原代细胞或连续传代细胞对猴病毒40(SV40)不敏感。被感染但未产生完整子代病毒的细胞合成肿瘤抗原(T抗原),但不合成病毒DNA和病毒衣壳蛋白(V抗原)。然而,当将SV40 DNA注入3T3细胞时,可获得V抗原。这种晚期基因表达似乎也与每个3T3细胞中注入的DNA分子数量相关。仅显微注射1至2个DNA分子后即可检测到T抗原的形成,但注入较高浓度的病毒DNA时,核内T抗原荧光强度明显更强。在敏感细胞(TC7)中,SV40的早期和晚期基因表达与注入分子的数量直接相关。显微注射1个DNA分子诱导T抗原和V抗原形成的效率与显微注射2000至4000个分子相同。通过将早期SV40互补RNA与少量病毒DNA一起显微注射,探讨了SV40晚期基因表达是否与早期病毒特异性产物的量直接相关的问题。在单独显微注射病毒DNA仅诱导T抗原而非V抗原合成的条件下,在很大比例的受体3T3细胞中获得了V抗原。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1ca7/515485/3486a29e88d9/jvirol00219-0195-a.jpg

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