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摘要:
Intron splicing in eukaryotic organisms requires the interactions of five snRNAs and numerous different proteins in the spliceosome. Although the molecular mechanism behind splicing has been well studied, relatively little is known about regulation of expression for these splicing factor proteins. One of these proteins is the evolutionarily-conserved Drosophila RNP-4F splicing assembly factor. This protein is transcribed from a single gene into two developmentally regulated mRNAs that differ in their 5’-UTR structure. In the longer isoform, known to be abundant in the developing fly central nervous system, a conserved retained intron which folds into a stem-loop has been implicated in expression control of the mRNA. Here, we describe construction and utilization of several new rnp-4f gene expression study vectors using a GFP reporter in the ΦC31 system. The results confirm our previous observation that presence of the regulatory stem-loop enhances RNP-4F protein expression. However, in that study, the enhancement factor protein was not identified. We show here that overexpression of the RNP-4F transgene compared to the control results in additional translation, as indicated by the GFP reporter in the fluorescent images. These results are interpreted to show that RNP-4F protein acts back on its own mRNA 5’-UTR regulatory region via a feedback pathway to enhance protein synthesis in the developing fly central nervous system. A model is proposed to explain the molecular mechanism behind rnp-4f gene expression control.
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篇名 Regulation of Expression for the RNP-4F Splicing Assembly Factor in the Fruit-Fly <i>Drosophila melanogaster</i>
来源期刊 动物科学期刊(英文) 学科 医学
关键词 rnp-4f GENE GENE Expression Control ΦC31 Transgenic VECTORS UAS-GAL4 System Fluorescence Microscopy
年,卷(期) 2015,(4) 所属期刊栏目
研究方向 页码范围 418-428
页数 11页 分类号 R73
字数 语种
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rnp-4f
GENE
GENE
Expression
Control
ΦC31
Transgenic
VECTORS
UAS-GAL4
System
Fluorescence
Microscopy
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动物科学期刊(英文)
季刊
2161-7597
武汉市江夏区汤逊湖北路38号光谷总部空间
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381
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