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分化的小鼠红白血病细胞中珠蛋白RNA的细胞质合成:RNA依赖性RNA聚合酶的可能参与。

Cytoplasmic synthesis of globin RNA in differentiated murine erythroleukemia cells: possible involvement of RNA-dependent RNA polymerase.

作者信息

Volloch V

出版信息

Proc Natl Acad Sci U S A. 1986 Mar;83(5):1208-12. doi: 10.1073/pnas.83.5.1208.

DOI:10.1073/pnas.83.5.1208
PMID:3456580
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC323044/
Abstract

Three lines of evidence indicate that RNA-dependent RNA synthesis occurs in mouse erythroleukemia cells. The first involves labeling studies with [3H]uridine and shows a greater initial labeling rate of globin RNA in the cytoplasm than in the nucleus. Labeled globin RNA found in the cytoplasm after a very short pulse with tritiated uridine is of the "mature" 9S size while labeled globin RNA in the nuclei is exclusively in the form of 15S precursor molecules, suggesting that cytoplasmic globin RNA is not of nuclear origin. A high concentration of actinomycin D has no effect on the initial rate of labeling of cytoplasmic globin RNA, supporting this conclusion. Other experiments showed that the labeling of cytoplasmic globin RNA does not involve end addition to preexisting globin RNA. The second line of evidence is the identification of globin RNA minus strand in the cytoplasm of differentiated murine erythroleukemia cells by hybridization with single-stranded DNA probes containing the strand of the same sense as globin mRNA. This material has the same electrophoretic mobility as globin RNA and hybridizes with probes containing only the 5' part or only the 3' part of the gene suggesting that it is a full size copy of globin RNA. Finally, in murine erythroleukemia cells an RNA-dependent RNA polymerase activity is detected by using poly(A) . oligo(U) as a template-primer combination. This activity increases significantly after induction, suggesting that it is differentiation specific.

摘要

三条证据表明,RNA依赖性RNA合成发生在小鼠红白血病细胞中。第一条涉及用[³H]尿苷进行的标记研究,结果显示,细胞质中珠蛋白RNA的初始标记率高于细胞核。用氚化尿苷进行极短时间脉冲后,在细胞质中发现的标记珠蛋白RNA为“成熟”的9S大小,而细胞核中的标记珠蛋白RNA仅以15S前体分子的形式存在,这表明细胞质中的珠蛋白RNA并非来自细胞核。高浓度放线菌素D对细胞质珠蛋白RNA的初始标记率没有影响,支持了这一结论。其他实验表明,细胞质珠蛋白RNA的标记不涉及在预先存在的珠蛋白RNA上进行末端添加。第二条证据是通过与包含与珠蛋白mRNA同意义链的单链DNA探针杂交,在分化的小鼠红白血病细胞的细胞质中鉴定出珠蛋白RNA负链。这种物质具有与珠蛋白RNA相同的电泳迁移率,并与仅包含基因5'部分或仅3'部分的探针杂交,这表明它是珠蛋白RNA的全长拷贝。最后,在小鼠红白血病细胞中,通过使用聚(A)·寡聚(U)作为模板-引物组合检测到RNA依赖性RNA聚合酶活性。诱导后,这种活性显著增加,表明它是分化特异性的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/21e8/323044/7e5deb340555/pnas00309-0050-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/21e8/323044/7e5deb340555/pnas00309-0050-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/21e8/323044/7e5deb340555/pnas00309-0050-a.jpg

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