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Abelson murine leukemia virus-transformed cells that lack p53 protein synthesis express aberrant p53 mRNA species.

机译:缺乏p53蛋白合成的Abelson鼠白血病病毒转化细胞表达异常的p53 mRNA种类。

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摘要

Cells of the Abelson murine leukemia virus-transformed line L12 that lack the p53 protein also lack polyadenylated mRNA capable of directing the synthesis of p53 in a cell-free system. Direct analysis of stable polyadenylated mRNA from a variety of cell lines shows that all p53 producers shared a common mRNA species (2.0 kilobases) which hybridized with a p53-specific cDNA probe. This species, which appears to be the mature, normal-sized p53 mRNA, was totally undetectable in L12 cells, which did not produce p53 in vivo. However, L12 cells contained two major p53-specific mRNA species of a substantially larger size (3.5 and 6.5 kilobases) than the p53-specific mRNA in the p53-producing cells. Genomic DNA analysis uncovered an apparent alteration in the 5' proximal part of only one p53 gene, which is unique to the L12 cell line. It is thus possible that the nonproducer phenotype of L12 cells is due at least in part to an alteration within a p53-specific DNA sequence. These findings define a system in which production of p53 appears to be efficiently regulated at the level of stable mRNA and which can be used to study the mechanisms controlling p53 expression in Abelson murine leukemia virus-transformed cells.
机译:缺乏p53蛋白的Abelson鼠白血病病毒转化L12系细胞也缺乏能够指导无细胞系统中p53合成的聚腺苷酸化mRNA。对各种细胞系中稳定的聚腺苷酸mRNA的直接分析表明,所有p53生产者都共享一个常见的mRNA种类(2.0千碱基),并与p53特异性cDNA探针杂交。该物种似乎是成熟的,正常大小的p53 mRNA,在L12细胞中完全无法检测到,而L12细胞在体内不产生p53。但是,L12细胞包含两个主要的p53特异性mRNA种类,其大小(分别为3.5和6.5千碱基)比产生p53的细胞中的p53特异性mRNA更大。基因组DNA分析发现只有一个p53基因的5'近端部分有明显的改变,这是L12细胞系独有的。因此,L12细胞的非生产者表型可能至少部分是由于p53特异性DNA序列内的改变所致。这些发现确定了一种系统,其中p53的产生似乎在稳定的mRNA水平上得到有效调节,并且可以用于研究在阿伯森鼠白血病病毒转化细胞中控制p53表达的机制。

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