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Characterization of a naturally occurring truncated Dicer

机译:天然截短切块机的表征

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Dicer is central to small RNA silencing pathways, thus playing an important role in physiological and pathological states. Recently, a number of mutations in dicer gene have been identified in diverse types of cancer, implicating Dicer in oncogenic cooperation. Here we report on the properties of a rare splice variant of the human dicer gene, occurring in neuroblastoma cells, and not detectable in normal tissues. Due to the skipping of one exon, the alternatively spliced transcript encodes a putative truncated protein, t-Dicer, lacking the dsRNA-binding domain and bearing altered one of the two RNase III catalytic centers. The ability of the exon-depleted t-dicer transcript to be translated in vitro was first investigated by the expression of flagged t-Dicer in human cells. We found that t-dicer transcript could be translated in vitro, albeit not as efficiently as full-length dicer transcript. Then, the possible enzymatic activity of t-Dicer was analyzed by an in vitro dicing assay able to distinguish the enzymatic activity of the individual RNase III domains. We showed that t-Dicer preserved partial dicing activity. Overall, the results indicate that t-dicer transcript could produce a protein still able to bind the substrate and to cleave only one of the two pre-miRNA strands. Given the increasing number of mutations reported for dicer gene in tumours, our experimental approach could be useful to characterize the activity of these mutants, which may dictate changes in selected classes of small RNAs and/or lead to their aberrant maturation.
机译:切酶对小RNA沉默途径至关重要,因此在生理和病理状态中起着重要作用。最近,已在多种癌症中鉴定了dicer基因的许多突变,这暗示了Dicer参与致癌合作。在这里,我们报告人类切丁机基因的罕见剪接变体的属性,该变体发生在成神经细胞瘤细胞中,而在正常组织中则无法检测到。由于跳过了一个外显子,因此选择性剪接的转录本编码了一种假定的截短蛋白t-Dicer,它缺少dsRNA结合结构域,并且带有两个RNase III催化中心之一。首先通过标记的t-Dicer在人细胞中的表达来研究外显子耗尽的t-dicer转录本在体外翻译的能力。我们发现t-dicer转录本可以在体外翻译,尽管效率不如全长dicer转录本。然后,通过能够区分单个RNase III结构域的酶促活性的体外切割试验,分析了t-Dicer可能的酶促活性。我们表明,t-Dicer保留了部分切割活性。总体而言,结果表明t-dicer转录本可以产生仍能结合底物并仅切割两条pre-miRNA链之一的蛋白质。考虑到针对肿瘤中的切丁酶基因报道的突变数量不断增加,我们的实验方法可能有助于表征这些突变体的活性,这可能决定了所选小分子RNA类型的变化和/或导致其异常成熟。

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