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The human hnRNP-M proteins: structure and relation with early heat shock-induced splicing arrest and chromosome mapping.

机译:人类hnRNP-M蛋白:与早期热激诱导的剪接停止和染色体作图的结构及其关系。

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摘要

With anti-hnRNP monoclonal antibody 6D12 we previously showed in HeLa cells that as early as 10 min after the onset of a heat shock at 45 degrees C, a 72.5-74 kDa antigen doublet leaves the hnRNPs and strongly associates with the nuclear matrix, the effect being reversed after a 6 h recovery at 37 degrees C. cDNA cloning and sequencing enabled us to identify these antigens as hnRNP-M proteins and further to show that the correct sequence differs by an 11 amino acid stretch from the originally published sequence. We also show that monoclonal antibodies raised against synthetic hnRNP-M peptides can directly inhibit in vitro splicing. Furthermore, stressing cells at 45 degrees C for 10 min is sufficient to abolish the splicing capacity of subsequently prepared nuclear extracts which, interestingly, do not contain the hnRNP-M proteins any more. Taken together, our data suggest that these proteins are involved in splicing as well as in early stress-induced splicing arrest. Further in situ hybridization assays located the hnRNP-M encoding gene on human chromosome 19.
机译:我们先前使用抗hnRNP单克隆抗体6D12在HeLa细胞中显示,早在45摄氏度的热休克发作后10分钟,一个72.5-74 kDa的抗原双链体就离开了hnRNPs,并与核基质紧密结合。在37摄氏度恢复6小时后,这种作用被逆转。cDNA克隆和测序使我们能够将这些抗原鉴定为hnRNP-M蛋白,并进一步证明正确的序列与原始公开的序列相差11个氨基酸。我们还显示针对合成的hnRNP-M肽产生的单克隆抗体可以直接抑制体外剪接。此外,在45摄氏度下对细胞施加10分钟的压力足以消除随后制备的核提取物的剪接能力,有趣的是,核提取物不再包含hnRNP-M蛋白。综上所述,我们的数据表明这些蛋白质参与剪接以及早期的应力诱导的剪接阻滞。进一步的原位杂交测定将hnRNP-M编码基因定位在人类19号染色体上。

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