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Size distribution of the urokinase mRNA decay intermediates in different tissues and cell lines

机译:尿激酶mRNA降解中间体在不同组织和细胞系中的大小分布

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Many genes, particularly those encoding the products participating in the regulation of transcription, replication and tissue remodeling, produce short-lived mRNA. It has been commonly accepted that once mRNA is disintegrated, the degradation process is so rapid that the decay intermediates cannot be detected. In the present study we verified this postulate and focused our attention on the quantification of the decay products of the urokinase-type plasminogen activator (uPA) mRNA that belongs to short-lived mRNAs. Using a previously described modified quantitative RT-PCR method, we have shown that intact uPA mRNA coexists in normal human tissues, Jurkat and 5637 cells with a great abundance of its degradation products. The uPA mRNA decay products were not detected in T24P cells. The content of intact uPA mRNA in normal tissues was as low as 5% of the total amount of its poly(A)~+ fraction. The size distribution of the mRNA decay products suggests that the mRNA is digested by exonucleases or/and non-specific endonuclease with cut sites evenly distributed along the mRNA chain. Different decay degrees were demonstrated for subpopulation of the uPA mRNA molecules with intact 3' and 5' ends.
机译:许多基因,特别是那些编码参与转录,复制和组织重塑调控的产物的基因,会产生短暂的mRNA。人们普遍接受的是,一旦mRNA分解,降解过程就会如此迅速,以至于无法检测到降解中间体。在本研究中,我们验证了这一假设,并将我们的注意力集中在了定量分析尿激酶型纤溶酶原激活物(uPA)mRNA的衰变产物上,该产物属于短暂的mRNA。使用先前描述的改进的定量RT-PCR方法,我们已经显示完整的uPA mRNA共存于正常人组织,Jurkat和5637细胞中,并且降解产物很多。在T24P细胞中未检测到uPA mRNA衰减产物。正常组织中完整的uPA mRNA的含量低至其poly(A)〜+部分总量的5%。 mRNA衰减产物的大小分布表明,mRNA被核酸外切酶或/和非特异性核酸内切酶消化,切割位点沿mRNA链均匀分布。对于具有完整的3'和5'末端的uPA mRNA分子的亚群,证明了不同的衰减度。

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