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汞化核苷酸:用于研究分离细胞核中RNA合成与加工的新工具的评估

Mercurated nucleotides: assessment of a new tool to study RNA synthesis and processing in isolated nuclei.

作者信息

Schäfer K P

出版信息

Nucleic Acids Res. 1977 Dec;4(12):4465-79. doi: 10.1093/nar/4.12.4465.

Abstract

Mercurated pyrimidine nucleotides have been used to study RNA synthesis and processing in isolated nuclei from mouse L cells. 5-mercuridine triphosphate (5-Hg-UTP) or 5-Hg-CTP are accepted as substrates by the purified RNA polymerases (I+III) and (II) from mouse cells, respectively, as well as by the enzymes still bound to the nuclear chromatin. In nuclei, RNA synthesis in the presence of Hg-UTP is reduced to 60-70% of a control. 30-60% of RNA labeled in vitro with (3H)UTP in isolated nuclei is not retained on sulfhydryl sepharose columns. Sucrose gradient analysis reveals a size distribution of the non-bound RNA similar to non-mercurated control RNA. Hg-RNA is found in a single peak from 4-10S. Chase experiments indicate that this RNA is the original transcript. It is argued that Hg-nucleotides may cause premature chain termination. Methylation of RNA in vitro by S-adenosyl methionine ((3H)SAM) is reduced to 75% of controls in the presence of Hg-UTP. Only 6% of the methyl groups appear in Hg-RNA. Polyadenylation is reduced as well. 15% of poly(A) (+)RNA are found in control assays whereas only 1% of Hg-RNA carries a poly(A) end added in vitro. These results limit the use of mercurated nucleotides for studies of nuclear RNA synthesis and processing.

摘要

汞化嘧啶核苷酸已被用于研究从小鼠L细胞分离出的细胞核中的RNA合成和加工过程。5-汞尿苷三磷酸(5-Hg-UTP)或5-汞胞苷三磷酸(5-Hg-CTP)分别被小鼠细胞纯化的RNA聚合酶(I+III)和(II)以及仍与核染色质结合的酶接受为底物。在细胞核中,存在Hg-UTP时的RNA合成减少至对照的60-70%。在分离的细胞核中用(3H)UTP体外标记的RNA中,30-60%不能保留在巯基琼脂糖柱上。蔗糖梯度分析显示未结合RNA的大小分布与未汞化的对照RNA相似。Hg-RNA出现在4-10S的单峰中。追踪实验表明这种RNA是原始转录本。有人认为汞化核苷酸可能导致链过早终止。在存在Hg-UTP的情况下,S-腺苷甲硫氨酸((3H)SAM)体外对RNA的甲基化减少至对照的75%。只有6%的甲基出现在Hg-RNA中。聚腺苷酸化也减少。在对照试验中发现15%的聚(A)(+)RNA,而只有1%的Hg-RNA带有体外添加的聚(A)末端。这些结果限制了汞化核苷酸在核RNA合成和加工研究中的应用。

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