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Identification of mRNAs that are spliced but not exported to the cytoplasm in the absence of THOC5 in mouse embryo fibroblasts

机译:在没有THOC5的情况下鉴定小鼠胚胎成纤维细胞中剪接但未输出到细胞质的mRNA

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摘要

The TREX (transcription/export) complex has been conserved throughout evolution from yeast to man and is required for coupled transcription elongation and nuclear export of mRNAs. The TREX complex in mammals and Drosophila is composed of the THO subcomplex (THOC1, THOC2, THOC5, THOC6, and THOC7), THOC3, UAP56, and Aly/THOC4. In human and Drosophila, various studies have shown that THO is required for the export of heat shock mRNAs, but nothing is known about other mRNAs. Our previous study using conditional THOC5 (or FMIP) knockout mice revealed that the presence of THOC5 is critical in hematopoietic cells but not for terminally differentiated cells. In this study, we describe the establishment of a mouse embryo fibroblast cell line (MEF), THOC5 flox/flox. Four days after infection of MEF THOC5 flox/flox with adenovirus carrying Cre-recombinase gene (Ad-GFP-Cre), THOC5 is down-regulated >95% at the protein level, and cell growth is strongly suppressed. Transcriptome analysis using cytoplasmic RNA isolated from cells lacking functional THOC5 reveals that only 2.9% of all genes were down-regulated more than twofold. Although we examined these genes in fibroblasts, one-fifth of all down-regulated genes (including HoxB3 and polycomb CBX2) are known to play a key role in hematopoietic development. We further identified 10 genes that are spliced but not exported to the cytoplasm in the absence of THOC5. These mRNAs were copurified with THOC5. Furthermore, Hsp70 mRNA was exported in the absence of THOC5 at 37°C, but not under heat shock condition (42°C), suggesting that THOC5 may be required for mRNA export under stress and/or upon signaling-induced conditions.
机译:从酵母到人的整个进化过程中,TREX(转录/出口)复合物一直被保存下来,并且是转录转录延长和mRNA核输出所必需的。哺乳动物和果蝇中的TREX复合物由THO亚复合物(THOC1,THOC2,THOC5,THOC6和THOC7),THOC3,UAP56和Aly / THOC4组成。在人类和果蝇中,各种研究表明,THO是热休克mRNA的输出所必需的,但对其他mRNA却一无所知。我们以前的使用条件性THOC5(或FMIP)基因敲除小鼠的研究表明,THOC5的存在在造血细胞中至关重要,但对于终末分化细胞却不重要。在这项研究中,我们描述了小鼠胚胎成纤维细胞系(MEF)THOC5 flox / flox的建立。用携带Cre重组酶基因(Ad-GFP-Cre)的腺病毒感染MEF THOC5 flox / flox后四天,THOC5在蛋白质水平下调> 95%,并强烈抑制细胞生长。使用从缺乏功能性THOC5的细胞中分离出的胞质RNA进行转录组分析,发现只有2.9%的所有基因被下调了两倍以上。尽管我们在成纤维细胞中检查了这些基因,但已知所有下调基因的五分之一(包括HoxB3和polycomb CBX2)在造血发育中起关键作用。我们进一步确定了在没有THOC5的情况下有10个剪接但没有输出到细胞质的基因。这些mRNA与THOC5共纯化。此外,Hsp70 mRNA在不存在THOC5的情况下在37°C时输出,但在热休克条件下(42°C)则不是,这表明在压力和/或信号诱导条件下,mRNA输出可能需要THOC5。

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