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聚肌苷酸×聚胞苷酸诱导的人成纤维细胞干扰素mRNA稳定性的调节:干扰素mRNA的选择性失活以及在干扰素产生关闭过程中2',5'-寡聚腺苷酸合成酶激活未参与其中。

Regulation of the stability of poly(I)xpoly(C)-induced human fibroblast interferon mRNA: selective inactivation of interferon mRNA and lack of involvement of 2',5'-oligo(A) synthetase activation during the shutoff of interferon production.

作者信息

Sehgal P B, Gupta S L

出版信息

Proc Natl Acad Sci U S A. 1980 Jun;77(6):3489-93. doi: 10.1073/pnas.77.6.3489.

Abstract

The inactivation of interferon mRNA during the shutoff phase of interferon production in poly(I)xpoly(C)-induced human fibroblast cultures is selective. We have determined that the shutoff of interferon production, which takes place from 3 to 8 hr after the beginning of induction, is not associated with an appreciable declined in the rate of bulk cellular protein synthesis or of cellular protein secretion. While the amount of translatable interferon mRNA declined markedly during the shutoff phase, the level of translatable bulk cellular mRNA and the stability of [3H]uridine-labeled mRNA were unaffected. Superinduction with actinomycin D selectively stabilized interferon mRNA with no apparent effect on the stability of bulk cellular mRNA. Furthermore, an activation of the 2',5'-oligo(A) synthetase/endonuclease system does not appear to be involved in the shutoff phenomenon. Uninduced FS-4 cells contained a low basal level of 2'5'-oligo(A) synthetase activity, which was unchanged in poly(I)xpoly(C)-induced cells during the shutoff phase. Treatment of FS-4 cells with interferon for 16-18 hr prior to induction increased the enzyme activity by approximately 200-fold. However, this did not inhibit interferon production after induction with poly(I)xpoly(C) alone or after superinduction with cycloheximide or actinomycin D or both. Furthermore, the rates of decay of interferon production were comparable in cells with either a basal or an increased level of 2',5'-oligo(A) synthetase. Thus a 200-fold increase in 2',5'-oligo(A) synthetase level did not affect either the stability of interferon mRNA or the efficacy of interferon superinduction by metabolic inhibitors.

摘要

在聚肌苷酸-聚胞苷酸(poly(I)xpoly(C))诱导的人成纤维细胞培养物中,干扰素产生的关闭阶段干扰素mRNA的失活具有选择性。我们已经确定,在诱导开始后3至8小时发生的干扰素产生的关闭,与总体细胞蛋白质合成速率或细胞蛋白质分泌速率的明显下降无关。虽然在关闭阶段可翻译的干扰素mRNA量显著下降,但可翻译的总体细胞mRNA水平和[3H]尿苷标记的mRNA稳定性未受影响。用放线菌素D进行超诱导可选择性地稳定干扰素mRNA,而对总体细胞mRNA的稳定性没有明显影响。此外,2',5'-寡聚腺苷酸合成酶/核酸内切酶系统的激活似乎与关闭现象无关。未诱导的FS-4细胞含有低基础水平的2',5'-寡聚腺苷酸合成酶活性,在聚肌苷酸-聚胞苷酸诱导的细胞的关闭阶段该活性未发生变化。在诱导前用干扰素处理FS-4细胞16至18小时,可使该酶活性增加约200倍。然而,这并不抑制单独用聚肌苷酸-聚胞苷酸诱导后或用环己酰亚胺或放线菌素D或两者进行超诱导后的干扰素产生。此外,在2',5'-寡聚腺苷酸合成酶水平为基础水平或升高水平的细胞中,干扰素产生的衰减速率相当。因此,2',5'-寡聚腺苷酸合成酶水平增加200倍既不影响干扰素mRNA的稳定性,也不影响代谢抑制剂对干扰素的超诱导效果。

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