Clustered regularly interspaced short palindromic repeats (CRISPR) and their associated CRISPR-associated sequence (CAS) proteins constitute a novel antiviral defence system that is widespread in prokaryotes. Repeats are separated by spacers, some of them homologous to sequences in mobile genetic elements. Although the whole process involved remains uncharacterized, it is known that new spacers are incorporated into CRISPR loci of the host during a phage challenge, conferring specific resistance against the virus. Moreover, it has been demonstrated that such interference is based on small RNAs carrying a spacer. These RNAs would guide the defence apparatus to foreign molecules carrying sequences that match the spacers. Despite this essential role, the spacer uptake mechanism has not been addressed. A first step forward came from the detection of motifs associated with spacer precursors (protospacers) of Streptococcus thermophilus, revealing a specific recognition of donor sequences in this species. Here we show that the conservation of proto-spacer adjacent motifs (PAMs) is a common theme for the most diverse CRISPR systems. The PAM sequence depends on the CRISPR-CAS variant, implying that there is a CRISPR-type-specific (motif-directed) choice of the spacers, which subsequently determines the interference target. PAMs also direct the orientation of spacers in the repeat arrays. Remarkably, observations based on such polarity argue against a recognition of the spacer precursors on transcript RNA molecules as a general rule.
INTRODUCTIONProkaryotes belonging to the most varied groups contain a peculiar type of repetitive DNA, recognized in 2000 as a family (Mojica et al., 2000), distinguished by the regular spacing of the recurrent motif, and consequently defined as short regularly spaced repeats (SRSR). A majority are partially palindromic, a feature that was later incorporated in the present denomination of CRISPR (clustered regularly interspaced short palindromic repeats), proposed by Jansen and co-workers in agreement with our group (Jansen et al., 2002). Repeat units are 24-47 bp long, and alternate with unique sequences (spacers) of similar size (27-72 bp). Despite considerable divergence, CRISPR can be classified based on sequence similarity (Kunin et al., 2007), defining 12 major groups (henceforth referred in the text as CRISPR-n, where n is the group identification number). Arrays of the same CRISPR are sometimes immediately followed by a conserved AT-rich sequence (Mojica et al., 2000) known as the leader (Jansen et al., 2002). In arrays with a degenerated terminal repeat, the leader is typically located on the opposite edge. Although their role remains undetermined, various reports suggest that leaders promote transcription towards the repeats (Brouns et al., 2008;Lillestøl et al., 2006;Mandin et al., 2007;Tang et al., 2002Tang et al., , 2005Willkomm et al., 2005). Also, the preferential incorporation of new spacers at the leaderproximal side of the array is consistent with a participation in the reco...
