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Regulation of translation by upstream translation initiation codons of surfactant protein Al splice variants

机译:用表面活性剂蛋白Al剪接变体的上游翻译引发密码子调节

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Surfactant protein A (SP-A), a molecule with roles in lung innate immunity and surfactant-related functions, is encoded by two genes in humans: SFTPA1 (SP-A1) and SFTPA2 (SP-A2). The mRNAs from these genes differ in their 5'-untranslated regions (5'-UTR) due to differential splicing. The 5'-UTR variant ACD' is exclusively found in transcripts of SP-A1, but not in those of SP-A2. Its unique exon C contains two upstream AUG codons (uAUGs) that may affect SP-A1 translation efficiency. The first uAUG (ul) is in frame with the primary start codon (p), but the second one (u2) is not. The purpose of this study was to assess the impact of uAUGs on SP-A1 expression. We employed RT-qPCR to determine the presence of exon C-containing SP-A1 transcripts in human RNA samples. We also used in vitro techniques including mutagenesis, reporter assays, and toeprinting analysis, as well as in silico analyses to determine the role of uAUGs. Exon C-containing mRNA is present in most human lung tissue samples and its expression can, under certain conditions, be regulated by factors such as dexamethasone or endotoxin. Mutating uAUGs resulted in increased luciferase activity. The mature protein size was not affected by the uAUGs, as shown by a combination of toeprint and in silico analysis for Kozak sequence, secondary structure, and signal peptide and in vitro translation in the presence of microsomes. In conclusion, alternative splicing may introduce uAUGs in SP-A1 transcripts, which in turn negatively affect SP-A1 translation, possibly affecting SP-A1/ SP-A2 ratio, with potential for clinical implication.
机译:表面活性剂蛋白A(SP-A),具有肺先天免疫和表面活性剂相关功能的作用的分子由人类中的两个基因编码:SFTPA1(SP-A1)和SFTPA2(SP-A2)。由于差异剪接,来自这些基因的MRNA在其5' - 未转换的区域(5'--UTR)中不同。 5'-UTR变体ACD'专用于SP-A1的转录物,但不在SP-A2的转录物中找到。其独特的外显子C包含两个可能影响SP-A1翻译效率的两个上游八个八个八卦密码子(UAUG)。第一个UAUG(UL)与主起始密码子(P)相框,但第二个(U2)不是。本研究的目的是评估UAUG对SP-A1表达的影响。我们使用RT-QPCR确定人RNA样品中含外显子的SP-A1转录物的存在。我们还使用体外技术,包括诱变,记者测定和泰式印刷分析,以及硅分析,以确定UAUG的作用。含外显子C的mRNA存在于大多数人肺组织样品中,其表达可以在某些条件下由诸如地塞米松或内毒素等因素进行调节。突变导致荧光素酶活性增加。成熟的蛋白质尺寸不受uAug的影响,如趾孔序列,二次结构和信号肽的组合和硅藻分析和在微粒体存在下的体外翻译中所示。总之,替代剪接可以在SP-A1转录物中引入uAug,其反过来呈负影响SP-A1平移,可能影响SP-A1 / SP-A2比率,具有临床意义的可能性。

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