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Literature DB >> 23872059

BRIC-seq: a genome-wide approach for determining RNA stability in mammalian cells.

Naoto Imamachi¹, Hidenori Tani², Rena Mizutani¹, Katsutoshi Imamura³, Takuma Irie⁴, Yutaka Suzuki⁴, Nobuyoshi Akimitsu⁵.

Abstract

We recently developed a novel transcriptome analysis method, termed 5'-bromo-uridine (BrU) immunoprecipitation chase-deep sequencing analysis (BRIC-seq). BRIC-seq enables the determination of genome-wide RNA stability by chasing chronological decreases of BrU-labeled RNAs under physiologically undisturbed conditions. The RNA half-life of each transcript is calculated from the decreasing number of BrU-labeled RNA sequence tags measured by deep sequencing of BrU-labeled RNAs. Here, we describe a detailed protocol and provide tips for BRIC-seq, followed by computational analysis.

Entities: Chemical Gene Species

Keywords: Genome-wide technology; High-throughput sequencing; Massive sequencing analysis; RNA decay; RNA degradation; RNA stability

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Substances：

Year: 2013 PMID： 23872059 DOI： 10.1016/j.ymeth.2013.07.014

Source DB: PubMed Journal: Methods ISSN： 1046-2023 Impact factor: 3.608

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Cited

36 in total

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3. Investigation of RNA Synthesis Using 5-Bromouridine Labelling and Immunoprecipitation.

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5. Loss of the fragile X syndrome protein FMRP results in misregulation of nonsense-mediated mRNA decay.

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Review 8. RNA-binding proteins in neurodegeneration: Seq and you shall receive.

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9. Oncofetal protein IGF2BP3 facilitates the activity of proto-oncogene protein eIF4E through the destabilization of EIF4E-BP2 mRNA.

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