[No authors listed]
Despite studies that have investigated the interactions of double-stranded RNA-binding proteins like Staufen with RNA in vitro, how they achieve target specificity in vivo remains uncertain. We performed RNA co-immunoprecipitations followed by microarray analysis to identify Staufen-associated mRNAs in early Drosophila embryos. Analysis of the localization and functions of these transcripts revealed a number of potentially novel roles for Staufen. Using computational methods, we identified two sequence features that distinguish Staufen's target transcripts from non-targets. First, these Drosophila transcripts, as well as those human transcripts bound by human Staufen1 and 2, have 3' untranslated regions (UTRs) that are 3-4-fold longer than unbound transcripts. Second, the 3'UTRs of Staufen-bound transcripts are highly enriched for three types of secondary structures. These structures map with high precision to previously identified Staufen-binding regions in Drosophila bicoid and human ARF1 3'UTRs. Our results provide the first systematic genome-wide analysis showing how a double-stranded RNA-binding protein achieves target specificity.
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CR18854, CR32207, Dsp1, CG17724, CG18273, CG44774, CG32767, CG5966, CG10777, Traf6, 825-Oak, CG32212, CG32214, CG32267, oc, CG32756, Kdm4B, Imp, Flo2, Tob, sl, nonA, vfl, bves, cpb, Prx6005, FASN1, CG33932, CG14915, CG4788, aret, nub, CG31688, VhaAC45, dap, Spred, stau, Pepck, Ppa, CG43736, seq, MED14, Rap1, CG9977, vn, CG5830, CG12519, CG14100, Pka-R1, Pc, lost, Mms19, Vha26, bcd, osk, pros, l(3)neo38, flfl, put, kuk, nos, sqz, CG17270, orb, RpS27, Nf1, fus, spen, ps, Pp4-19C, VhaPPA1-1, vir, CR18166, CR14578
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