RNA primary and secondary motif discovery is an important step in the annotation and characterization of unknown interaction dynamics between RNAs and RNA-Binding Proteins, and several methods have been developed to meet the need of fast and efficient discovery of interaction motifs. Recent advances have increased the amount of data produced by experimental assays and there is no available method suitable for the analysis of all type of results. Here we present a simple workflow to help choosing the more appropriate method, depending on the starting situation, among the three algorithms that best cover the landscape of approaches. A detailed analysis is presented to highlight the need for different algorithms in different working settings. In conclusion, the proposed workflow depends on the nature of the starting data and on the availability of RNA annotations.
Keywords: CLIP-Seq; High-throughput assay; Motif discovery; RNA; RNA secondary structure.