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放线菌素D处理后一些小核仁核糖核蛋白的去定位以耗尽早期前体核糖体RNA。

Delocalization of some small nucleolar RNPs after actinomycin D treatment to deplete early pre-rRNAs.

作者信息

Rivera-León R, Gerbi S A

机构信息

Brown University, Division of Biology and Medicine, Department of Molecular Biology, Cell Biology and Biochemistry, Providence, RI 02912, USA.

出版信息

Chromosoma. 1997 Jun;105(7-8):506-14. doi: 10.1007/BF02510487.

Abstract

Retention of some components within the nucleolus correlates with the presence of rRNA precursors found early in the rRNA processing pathway. Specifically, after most 40S, 38S and 36S pre-rRNAs have been depleted by incubation of Xenopus kidney cells in 0.05 microg/ml actinomycin D for 4 h, only 69% U3 small nucleolar RNA (snoRNA), 68% U14 snoRNA and 72% fibrillarin are retained in the nucleolus as compared with control cells. These nucleolar components are important for processing steps in the pathway that gives rise to 18S rRNA. In contrast, U8 snoRNA, which is used for 5.8S and 28S rRNA production, is fully retained in the nucleolus after actinomycin D treatment. Therefore, U8 snoRNA is in a different category than U3 and U14 snoRNA and fibrillarin. It is proposed that U3 and U14 snoRNA and fibrillarin, but not U8 snoRNA, bind to the external transcribed spacer or internal transcribed spacer 1, and when these binding sites are lost after actinomycin D treatment some of these components cannot be retained in the nucleolus. Other binding sites may also exist, which would explain why only some and not all of these components are lost from the nucleolus.

摘要

核仁中某些成分的保留与核糖体RNA加工途径早期发现的核糖体RNA前体的存在相关。具体而言,将非洲爪蟾肾细胞在0.05微克/毫升放线菌素D中孵育4小时后,大多数40S、38S和36S前核糖体RNA被消耗,与对照细胞相比,核仁中仅保留69%的U3小核仁RNA(snoRNA)、68%的U14 snoRNA和72%的纤维蛋白原。这些核仁成分对于产生18S核糖体RNA的途径中的加工步骤很重要。相比之下,用于产生5.8S和28S核糖体RNA的U8 snoRNA在放线菌素D处理后完全保留在核仁中。因此,U8 snoRNA与U3、U14 snoRNA和纤维蛋白原属于不同类别。有人提出,U3和U14 snoRNA以及纤维蛋白原而非U8 snoRNA与外部转录间隔区或内部转录间隔区1结合,并且在放线菌素D处理后这些结合位点丧失时,其中一些成分无法保留在核仁中。也可能存在其他结合位点,这可以解释为什么只有部分而非所有这些成分从核仁中丢失。

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