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Functional characterization of alternatively spliced human SECISBP2 transcript variants

机译:选择性剪接的人类SECISBP2转录本变体的功能表征

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Synthesis of selenoproteins depends on decoding of the UGA stop codon as the amino acid selenocysteine (Sec). This process requires the presence of a Sec insertion sequence element (SECIS) in the 3'-untranslated region of selenoprotein mRNAs and its interaction with the SECIS binding protein 2 (SBP2). In humans, mutations in the SBP2-encoding gene Sec insertion sequence binding protein 2 (SECISBP2) that alter the amino acid sequence or cause splicing defects lead to abnormal thyroid hormone metabolism. Herein, we present the first in silico and in vivo functional characterization of alternative splicing of SECISBP2. We report a complex splicing pattern in the 5'-region of human SECISBP2, wherein at least eight splice variants encode five isoforms with varying N-terminal sequence. One of the isoforms, mtSBP2, contains a mitochondrial targeting sequence and localizes to mitochondria. Using a minigene-based in vivo splicing assay we characterized the splicing efficiency of several alternative transcripts, and show that the splicing event that creates mtSBP2 can be modulated by antisense oligonucleotides. Moreover, we show that full-length SBP2 and some alternatively spliced variants are subject to a coordinated transcriptional and translational regulation in response to ultraviolet type A irradiation-induced stress. Overall, our data broadens the functional scope of a housekeeping protein essential to selenium metabolism.
机译:硒蛋白的合成取决于作为氨基酸硒代半胱氨酸(Sec)的UGA终止密码子的解码。此过程需要在硒蛋白mRNA的3'-非翻译区中存在Sec插入序列元件(SECIS),并与SECIS结合蛋白2(SBP2)相互作用。在人类中,SBP2编码基因Sec插入序列结合蛋白2(SECISBP2)的突变会改变氨基酸序列或引起剪接缺陷,从而导致甲状腺激素代谢异常。在本文中,我们提出了SECISBP2选择性剪接的第一个计算机模拟和体内功能表征。我们报告了人类SECISBP2 5'区域中的复杂剪接模式,其中至少八个剪接变体编码具有变化的N端序列的五个同工型。异构体之一mtSBP2包含线粒体靶向序列,并定位于线粒体。使用基于小基因的体内剪接测定法,我们表征了几种替代转录物的剪接效率,并表明产生mtSBP2的剪接事件可被反义寡核苷酸调节。此外,我们表明全长SBP2和一些选择性剪接的变异体响应紫外线A型辐射诱导的胁迫而受到协调的转录和翻译调控。总体而言,我们的数据拓宽了硒代谢必不可少的管家蛋白的功能范围。

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