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首页> 外文期刊>Biochemical and Biophysical Research Communications >Experimental validation and complexity of miRNA-mRNA target interaction during zebrafish primitive erythropoiesis.
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Experimental validation and complexity of miRNA-mRNA target interaction during zebrafish primitive erythropoiesis.

机译:斑马鱼原始红细胞生成过程中miRNA-mRNA靶相互作用的实验验证和复杂性。

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MicroRNAs (miRNAs) are endogenous small non-protein coding RNAs that play important regulatory roles in animals and plants by binding to target transcripts for cleavage or translational repression. Despite increasing number of genes has been predicted to be miRNA targets by bioinformatics analysis and luciferase-based reporter assay in vitro (RA-In Vitro), few of them have been experimentally validated in physiological context. Using transient reporter assay in vivo (TRA-In Vivo), we identified hydroxymethylbilane synthase b (hmbsb) and Kruppel-like transcription factor d (klfd) as potential target gene for miR-451 and miR-144, respectively. Although hmbsb, miR-451, klfd and miR-144 are all co-expressed in the developing erythroid progenitors during zebrafish erythropoiesis, only klfd can be validated as a bona fide physiological target of miR-144 using a transgene-based physiological reporter assay in vivo (PRA-In Vivo). Thus, failure to verify hmbsb as miR-451 target in physiological context raises a crucial question as to how to determine bona fide target of miRNA. The results address the importance of using multiple approaches combined with Western blot analysis to validate the physiological target of a given miRNA.
机译:MicroRNA(miRNA)是内源性的非蛋白质小分子编码RNA,通过与靶标转录物结合以进行切割或翻译抑制,在动物和植物中起重要的调节作用。尽管通过生物信息学分析和体外基于萤光素酶的报告基因检测(RA-Introtro)预测了越来越多的基因成为miRNA靶标,但很少有人在生理方面进行了实验验证。使用体内瞬时报告基因检测(TRA-体内),我们分别确定了羟甲基胆碱合酶b(hmbsb)和Kruppel样转录因子d(klfd)作为miR-451和miR-144的潜在靶基因。尽管hmbsb,miR-451,klfd和miR-144在斑马鱼促红细胞生成过程中都在发育中的类红细胞祖细胞中共表达,但使用基于转基因的生理报告基因检测方法,只有klfd可以被确认为miR-144的真正生理靶标。 vivo(体内PRA)。因此,在生理背景下无法将hmbsb验证为miR-451靶标提出了一个至关重要的问题,即如何确定miRNA的真正靶标。结果解决了使用多种方法与Western blot分析相结合来验证给定miRNA的生理学指标的重要性。

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