Abanades Daniel R, Ramírez Laura, Iborra Salvador, Soteriadou Ketty, González Victor M, Bonay Pedro, Alonso Carlos, Soto Manuel
Centro de Biología Molecular Severo Ochoa, Departamento de Biología Molecular, Universidad Autónoma de Madrid, CSIC-UAM, Nicolás Cabrera 1, 28049 Madrid, Spain.
BMC Mol Biol. 2009 May 21;10:48. doi: 10.1186/1471-2199-10-48.
Histone synthesis in Leishmania is tightly coupled to DNA replication by a post-transcriptional mechanism operating at the level of translation.
In this work we have analyzed the implication of the 5' and 3' untranslated regions (UTR) in the cell cycle regulated expression of the histone H2A in Leishmania infantum. For that purpose, L. infantum promastigotes were stably transfected with different plasmid constructs in which the CAT coding region used as a reporter was flanked by the 5' and 3' UTR regions of the different H2A genes. We report that in spite of their sequence differences, histone H2A 5' and 3' UTRs conferred a cell cycle dependent pattern of expression on the CAT reporter since de novo synthesis of CAT increased when parasites enter the S phase. Using one established L. infantum cell line we showed that CAT expression is controlled by the same regulatory events that control the endogenous histone gene expression. Thus, although we did not detect changes in the level of CAT mRNAs during cell cycle progression, a drastic change in the polysome profiles of CAT mRNAs was observed during the progression from G1 to S phase. In the S phase CAT mRNAs were on polyribosomal fractions, but in the G1 phase the association of CAT transcripts with ribosomes was impaired. Furthermore, it was determined that the addition of just the H2A 3' UTR to the CAT reporter gene is sufficient to achieve a similar pattern of post-transcriptional regulation indicating that this region contains the major regulatory sequences involved in the cell cycle dependent expression of the H2A genes. On the other hand, although CAT transcripts bearing the H2A 5' alone were translated both in the G1 and S phase, higher percentages of transcripts were detected on polyribosomes in the S phase correlating with an increase in the de novo synthesis of CAT. Thus, it can be concluded that this region also contributes, although to a minor extent than the 3' UTR, in the enhancement of translation in the S phase relative to the G1 phase.
Our findings indicate that both, the 5' and the 3' UTRs contain sequence elements that contribute to the cell cycle expression of L. infantum H2A. The 3' UTR region is essential for cell cycle dependent translation of the L. infantum H2A transcripts whereas the 5' UTR has a minor contribution in their S phase dependent translation.
利什曼原虫中的组蛋白合成通过一种在翻译水平起作用的转录后机制与DNA复制紧密偶联。
在本研究中,我们分析了5'和3'非翻译区(UTR)在婴儿利什曼原虫组蛋白H2A细胞周期调控表达中的作用。为此,用不同的质粒构建体稳定转染婴儿利什曼原虫前鞭毛体,其中用作报告基因的CAT编码区两侧是不同H2A基因的5'和3'UTR区。我们报告,尽管它们的序列不同,但组蛋白H2A的5'和3'UTR赋予了CAT报告基因细胞周期依赖性的表达模式,因为当寄生虫进入S期时,CAT的从头合成增加。使用一个已建立的婴儿利什曼原虫细胞系,我们表明CAT表达受控制内源性组蛋白基因表达的相同调控事件控制。因此,尽管我们在细胞周期进程中未检测到CAT mRNA水平的变化,但在从G1期到S期的进程中观察到CAT mRNA多核糖体图谱的剧烈变化。在S期,CAT mRNA存在于多核糖体组分上,但在G1期,CAT转录本与核糖体的结合受损。此外,已确定仅将H2A 3'UTR添加到CAT报告基因就足以实现类似的转录后调控模式,表明该区域包含参与H2A基因细胞周期依赖性表达的主要调控序列。另一方面,尽管仅携带H2A 5'的CAT转录本在G1期和S期均被翻译,但在S期多核糖体上检测到的转录本百分比更高,这与CAT的从头合成增加相关。因此,可以得出结论,该区域在相对于G1期增强S期的翻译中也有贡献,尽管程度比3'UTR小。
我们的研究结果表明,5'和3'UTR均包含有助于婴儿利什曼原虫H2A细胞周期表达的序列元件。3'UTR区域对于婴儿利什曼原虫H2A转录本的细胞周期依赖性翻译至关重要,而5'UTR在其S期依赖性翻译中的贡献较小。
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