Literature DB >> 17592041

NRF IRES activity is mediated by RNA binding protein JKTBP1 and a 14-nt RNA element.

Marc René Reboll1, André Oumard, Aniko Carla Gazdag, Isabelle Renger, Birgit Ritter, Michael Schwarzer, Hansjoerg Hauser, Monika Wood, Michiyuki Yamada, Klaus Resch, Mahtab Nourbakhsh.   

Abstract

The mRNA of human NF-kappaB repressing factor (NRF) contains a long 5'-untranslated region (UTR) that directs ribosomes to the downstream start codon by a cap-independent mechanism. Comparison of the nucleotide (nt) sequences of human and mouse NRF mRNAs reveals a high degree of identity throughout a fragment of 150 nt proximal to the start codon. Here, we show that this region constitutes a minimal internal ribosome entry segment (IRES) module. Enzymatic RNA structure analysis reveals a secondary structure model of the NRF IRES module. Point mutation analysis of the module determines a short, 14-nt RNA element (nt 640-653) as a mediator of IRES function. Purification of IRES binding cellular proteins and subsequent ESI/MS/MS sequence analysis led to identification of the RNA-binding protein, JKTBP1. EMSA experiments show that JKTBP1 binds upstream to the 14-nt RNA element in the NRF IRES module (nt 579-639). Over-expression of JKTBP1 significantly enhances activity of the NRF IRES module in dicistronic constructs. Moreover, siRNA experiments demonstrate that down-regulation of endogenous JKTBP1 decreases NRF IRES activity and the level of endogenous NRF protein. The data of this study show that JKTBP1 and the 14-nt element act independently to mediate NRF IRES activity.

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Year:  2007        PMID: 17592041      PMCID: PMC1924892          DOI: 10.1261/rna.545407

Source DB:  PubMed          Journal:  RNA        ISSN: 1355-8382            Impact factor:   4.942


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