Identification and evolutionary analysis of a new Dapper1 variant generated by alternative splicing during vertebrate development

Alternative splicing is an important mechanism to expand protein diversity in eukaryotes. This process allows the production of different mRNAs from a single coding sequence and is frequentfy used by genes involved in development. Oapper 1 (Opr1) is an important rnodulator of Wnt signalling, working in several developmental processes, such as neural tissue specification, head morphogenesis, heart and eye development. While its interaction with Oishevelled is known to modulate Wnt signalling both in vivo and in vitre, the interaction wrth other molecules is required to mediate its multiple biological functions. Considering that Dpr1 has a modular structure that mediates its interaction with different partners through different structural domains, this molecule could greatly benefit from alternative splicing in order to combine different domains and consequently amplify its biological functions. In the present study we describe a new Opr1 isoform that was initially identified in the mouse transcriptome using bioinformatic tools. This isoform is 111 pb longer than the one encoded by the RefSeq mRNA for Opr1, here named O and E isoforms, respectively. The variant transcripts are generated through two distinct acceptor splice sites in exon 4. The segment exclusive of the O isoform is in frame and encodes 37 residues located in a variable region of Oprl exon 4, known to be necessary for the interaction with the transcriptional factor Tcf3. comparative analysis of the Opr1 locus among fish, frog, chicken, mouse and human revealed that in tetrapods two acceptor splice sites are conserved in the beginning of the exon 4, while in fish a single acceptor splice site is found. RT-PCR using species-specific primers confirmed the expression of the O and E isoforms in tetrapods while in fish only the O isoform was detected. In addition, we showed that the Opr1 isoforms are coexpressed throughout chicken development, suggesting that the relative concentration of these molecules may be important for their functionality. Finally, even though no evidence of positive selection was detected for the entire Dpr1 protein, exon 4 seems to be under more relaxed selective pressure than the other exons. These results are consistent with the notion that alternative splicing can act as a mechanism for opening accelerated paths of evolution by reducing negative selection pressure. (AU)