首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Interferon messenger RNA content of human fibroblasts during induction shutoff and superinduction of interferon production
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Interferon messenger RNA content of human fibroblasts during induction shutoff and superinduction of interferon production

机译:诱导关闭和超诱导干扰素产生过程中人成纤维细胞的干扰素信使RNA含量

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摘要

Translation of injected mRNA in oocytes of Xenopus laevis has been used as a highly sensitive and quantitative assay for interferon mRNA. Injection into oocytes of polyadenylylated RNA extracted from poly(I)·poly(C)-induced human diploid fibroblasts (FS-4) leads to the synthesis of biologically active human fibroblast interferon over a period of 24-32 hr. There is a linear relationship between the amount of mRNA injected and the interferon yield obtained over a range of 1-20 ng of injected RNA. Injection of 40-80 ng of mRNA into each of 15 oocytes, homogenized in 0.3 ml of incubation medium, gave a titer of 128-256 interferon reference units/ml of homogenate.FS-4 cells at the peak of interferon production—i.e., approximately 2.5 hr after the beginning of induction with poly(I)·poly(C)—gave mRNA that yielded 24-48 interferon reference units/ml in the oocyte assay (30 ng of RNA injected per oocyte). An equivalent amount of mRNA from FS-4 cells in the shutoff phase, approximately 6 hr after induction, gave ≤4 interferon reference units/ml. In contrast, mRNA extracted from FS-4 cells that had been induced and maintained in the presence of 40 μM 5,6-dichloro-1-β-D-ribofuranosylbenzimidazole for 6 hr produced 64-128 interferon reference units/ml. Polyadenylylated RNA obtained from uninduced FS-4 cells did not lead to detectable interferon synthesis (<4 interferon reference units/ml). These data provide a direct verification of the hypothesis that the shutoff of interferon production in FS-4 cells involves a regulatory event leading to the posttranscriptional inactivation or degradation of interferon mRNA. Because the inactivating mechanism is sensitive to inhibition by 5,6-dichloro-1-β-D-ribofuranosylbenzimidazole, a selective inhibitor of nuclear heterogeneous RNA and mRNA synthesis, it is likely that synthesis of an RNA molecule is necessary for the shutoff of interferon production.
机译:非洲爪蟾卵母细胞中注射的mRNA的翻译已用作干扰素mRNA的高度灵敏和定量测定。注射到卵母细胞中的聚腺苷酸化的RNA提取从poly(I)·poly(C)诱导的人类二倍体成纤维细胞(FS-4)中提取,可以在24-32 hr的时间内合成具有生物活性的人类成纤维细胞干扰素。在1-20 ng注射RNA范围内,注射的mRNA量与获得的干扰素产量之间存在线性关系。在15 ml卵母细胞中分别注入40-80 ng mRNA,并在0.3 ml培养液中匀浆,得到的滴度为128-256干扰素参考单位/ ml匀浆。在干扰素产生高峰时,FS-4细胞即在开始用多聚(I)·多聚(C)诱导大约2.5小时后,产生卵母细胞测定中产生24-48干扰素参考单位/ ml的mRNA(每个卵母细胞注射30 ng RNA)。诱导后约6小时,在封闭期,来自FS-4细胞的等量mRNA给出≤4干扰素参考单位/ ml。相反,从已被诱导并维持在40μM5,6-二氯-1-β-D-呋喃呋喃糖基苯并咪唑存在下6小时的FS-4细胞中提取的mRNA产生64-128干扰素参考单位/毫升。从未诱导的FS-4细胞获得的聚腺苷酸化RNA不会导致可检测到的干扰素合成(<4干扰素参考单位/ ml)。这些数据直接证实了以下假设:FS-4细胞中干扰素生产的关闭涉及导致转录后失活或干扰素mRNA降解的调节事件。由于失活机制对5,6-dichloro-1-β-D-核呋喃糖基苯并咪唑(一种核异质RNA和mRNA合成的选择性抑制剂)的抑制敏感,因此可能需要合成RNA分子来阻断干扰素。生产。

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