Trypanosomatid, fluorescence-based in vitro U-insertion/U-deletion RNA-editing (FIDE)

被引:1
|
作者
Leeder, Matthias [1 ]
Kruse, Elisabeth [1 ]
Goeringer, H. Ulrich [1 ]
机构
[1] Tech Univ Darmstadt, Mol Genet, Darmstadt, Germany
来源
BIO-PROTOCOL | 2021年 / 11卷 / 05期
关键词
RNA-editing; U-insertion/U-deletion editing; Editosome; Guide RNA; RNA-processing; Mitochondrial gene expression; African trypanosomes; Protozoan parasites; GUIDE RNA; MECHANISM; SEQUENCE; MODEL; GRNA;
D O I
10.21769/BioProtoc.3935
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Gene expression within the mitochondria of African trypanosomes and other protozoan organisms relies on a nucleotide-specific RNA-editing reaction. In the process exclusively uridine (U)-nucleotides are site-specifically inserted into and deleted from sequence-deficient primary transcripts to convert them into translatable mRNAs. The reaction is catalyzed by a 0.8 MDa multiprotein complex termed the editosome. Here we describe an improved in vitro test to quantitatively explore the catalytic activity of the editosome. The assay uses synthetic, fluorophore-derivatized oligoribonucleotides as editing substrates, which enable the automated electrophoretic separation of the reaction products by capillary electrophoresis (CE) coupled to laser-induced fluorescence (LIF) detection systems. The assay is robust, it requires only nanogram amounts of materials and by using multicapillary CE/LIF-instruments it can be executed in a highly parallel layout. Further improvements include the usage of phosphorothioate-modified and thus RNase-resistant substrate RNAs as well as multiplex-type fluorophore labeling strategies to monitor the U-insertion and U-deletion reaction simultaneously. The assay is useful for investigating the mechanism and enzymology of the editosome. However, it can also be executed in high-throughput to screen for RNA editing -specific inhibitors. [GRAPHICS]
引用
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页数:20
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