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雏鸡输卵管中的雌激素撤退。使用汞化前体对分离细胞核中合成的RNA进行表征。

Estrogen withdrawal in chick oviduct. Characterization of RNA synthesized in isolated nuclei using a mercurated precursor.

作者信息

Mizuno S, Tallman N A, Cox R F

出版信息

Biochim Biophys Acta. 1978 Aug 23;520(1):184-202. doi: 10.1016/0005-2787(78)90019-9.

Abstract
  1. As a prerequisite for analyzing the effect of estrogen on transcription in chick oviduct, we describe suitable methods for the synthesis (under conditions restricting reinitiation), and isolation of RNA transcripts from oviduct nuclei in vitro, utilizing mercurated UTP (Hg-UTP) as an RNA precursor and chromatography on sulphydryl-Sepharose (SH-Sepharose) to recover mercurated RNA (Hg-RNA). The techniques described include treatment of Hg-RNA with p-hydroxymercuribenzoate, to improve the efficiency of binding to SH-Sepharose, and elution of Hg-RNA from SH-Sepharose after treatment with 60% formamide at 90 degrees C, to eliminate contamination by aggregated nucleic acid. 2. RNA synthesized by endogenous form B RNA polymerase (using either UTP or Hg-UTP as precursor) was recovered in nuclear lysates in the form of 30--85-S heterogeneous RNA . protein complexes, and after removal of protein, was 10--12 S in size. 3. The nature of RNA transcripts synthesized in vitro was examined by hybridization. More than 90% of the RNA was complementary to "unique" DNA sequences, and 50--60% of the hybridized RNA could be competed with homologous, steady-state nuclear RNA, indicating a significant degree with homologous, steady-state nuclear RNA, indicating a significant degree of homology between in vitro transcripts and in vivo RNA. The level of homology was similar whether RNA synthesis was performed in low salt, or in high salt in the presence of heparin. Possible reasons for only partial competition in these experiments are discussed. 4. Withdrawal of estrogen from chicks leads to a 50% reduction in endogenous RNA polymerase activities in nuclei within 48 h. Similar levels of competition with Hg-RNA transcripts for "unique" DNA were obtained using oviduct nuclear RNAs isolated before or after estrogen withdrawal, and even with liver nuclear RNA. Thus, in oviduct, those sequences present in primary transcripts, and analyzed under our experimental conditions, are present in different hormonal states and also in other chick tissues.
摘要
  1. 作为分析雌激素对鸡输卵管转录作用的前提条件,我们描述了合适的方法,即在限制重新起始的条件下合成,并从输卵管细胞核中体外分离RNA转录本,利用汞化UTP(Hg-UTP)作为RNA前体,并通过巯基琼脂糖凝胶(SH-琼脂糖凝胶)色谱法回收汞化RNA(Hg-RNA)。所述技术包括用对羟基汞苯甲酸处理Hg-RNA,以提高与SH-琼脂糖凝胶结合的效率,以及在90℃用60%甲酰胺处理后从SH-琼脂糖凝胶上洗脱Hg-RNA,以消除聚集核酸的污染。2. 由内源性B型RNA聚合酶合成的RNA(使用UTP或Hg-UTP作为前体)以30 - 85-S异质RNA·蛋白质复合物的形式在核裂解物中回收,去除蛋白质后,大小为10 - 12 S。3. 通过杂交检查体外合成的RNA转录本的性质。超过90%的RNA与“独特”DNA序列互补,50 - 60%的杂交RNA可被同源的稳态核RNA竞争,这表明体外转录本与体内RNA之间存在显著程度的同源性。无论RNA合成是在低盐条件下进行,还是在肝素存在的高盐条件下进行,同源性水平相似。讨论了这些实验中仅部分竞争的可能原因。4. 从雏鸡中撤除雌激素会导致48小时内核中内源性RNA聚合酶活性降低50%。使用在撤除雌激素之前或之后分离的输卵管核RNA,甚至使用肝核RNA,获得了与Hg-RNA转录本对“独特”DNA的类似竞争水平。因此,在输卵管中,初级转录本中存在的那些序列,在我们的实验条件下进行分析时,存在于不同的激素状态以及其他鸡组织中。

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