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Characterization of the 5' region of the Leishmania infantum L0RIEN/MAT2 gene cluster and role of LORIEN flanking regions in post-transcriptional regulation

机译:婴儿利什曼原虫L0RIEN / MAT2基因簇5'区的表征和LORIEN侧翼区在转录后调控中的作用

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LORIEN (encoding a protein that contains a SP-RING/Miz zinc-finger motif present in a group of proteins involved in the Small Ubiquitin-related Modifier -SUMO- conjugation pathway) and MAT2 (encoding the methionine adenosyltransferase -MAT-) genes are arranged as two alternating copies in a head-to-tail configuration, with the LORIEN gene as the first copy of the cluster. The 5880 bp preceding the first LORIEN gene copy were compared to the same region of L. major, showing a 93% identity between them. Bioinformatic analysis of this region predicted the presence of a 747-bp ORF encoding a hypothetical protein of 248 amino acids. Transcription of this ORF was confirmed by run-on assays and RT-PCR. Expression of the LORIEN gene was tested in both the promastigote and amastigote stages. Transcription arrest evidenced that LORIEN mRNA stability was very similar in both stages of the parasite life cycle. Protein synthesis inhibition by cycloheximide led to an increase in the steady-state levels of LORIEN transcripts only during the promastigote stage, pointing out to the existence of different stage-dependent mechanisms operating on the post-transcriptional regulation of this gene. The role of the LORIEN untranslated regions (5'UTR and 3'UTR) in post-transcriptional regulation was analysed using the luciferase (luc) reporter gene. Results evidenced that the 5'UTR was responsible for a low reporter gene expression, whereas the intergenic region (IR) between LORIEN and MAT2 genes provided high luc levels. However, the 3'UTR seemed to lack regulatory elements. Basing on these results, a model of regulation for the LORIEN gene is proposed.
机译:LORIEN(编码包含SP-RING / Miz锌指基序的蛋白质存在于与泛素相关的小修饰子-SUMO-偶联途径的一组蛋白质中)和MAT2(编码甲硫氨酸腺苷基转移酶-MAT-)基因是以头尾相接的形式排列成两个交替的拷贝,LORIEN基因是簇的第一个拷贝。将第一个LORIEN基因拷贝之前的5880 bp与大麦芽孢杆菌的相同区域进行比较,显示它们之间的同源性为93%。该区域的生物信息学分析预测,存在一个747-bp的ORF,该ORF编码一个248个氨基酸的假设蛋白质。通过连续分析和RT-PCR证实了该ORF的转录。在前鞭毛体和鞭毛体两个阶段都测试了LORIEN基因的表达。转录逮捕证明,在寄生虫生命周期的两个阶段,LORIEN mRNA的稳定性都非常相似。仅在前鞭毛体阶段,环己酰亚胺对蛋白质合成的抑制作用会导致LORIEN转录本的稳态水平增加,这表明存在对该基因的转录后调控起作用的不同阶段依赖性机制。使用荧光素酶(luc)报告基因分析了LORIEN非翻译区(5'UTR和3'UTR)在转录后调控中的作用。结果证明5'UTR导致报告基因表达低,而LORIEN和MAT2基因之间的基因间区域(IR)提供了较高的luc水平。但是,3'UTR似乎缺乏调控成分。基于这些结果,提出了LORIEN基因的调控模型。

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