Thus, these polymorphic pk1 and pk2 ank genes, located within a so-called WO prophage region of Wolbachia genome, are suggested to contribute to the CI phenotype. Consistent with this argument, expression of the pk2 gene occurred specifically in female mosquitoes [8, 22, 23]. Moreover, a premature stop codon was found in the pk2 gene of the Wolbachia strain (wAu) that
is unable to cause CI in D. simulans[21]. In this study, we aimed to determine whether the prophage pk1 and pk2 ankyrin genes were involved in the CI phenotype described in three Wolbachia-infected species of terrestrial isopods. We also investigated whether these genes were conserved and expressed in Wolbachia Selleck Selumetinib strains inducing feminization, the main Wolbachia phenotype described for this group of hosts [2]. From the genome of the feminizing wVulC Wolbachia strain that infects the isopod Armadillidium vulgare
(the genome completion is currently being done by our group in the Alpelisib concentration frame of the European Wolbachia project: EuWol), we annotated the pk1 and pk2 alleles among all ank genes identified from the wVulC contigs. We investigated the distribution, copy number and expression patterns of both genes in seven additional Wolbachia strains that induce either CI Cediranib (AZD2171) or feminization in isopods. We identified a large copy number variation of the pk1 and pk2 genes among Wolbachia strains, which is probably coupled to prophage evolution. Surprisingly, our results also revealed that expression of one pk2 allele (pk2b2) is only detected in feminizing Wolbachia strains and never in the three CI-inducing strains of isopods. Results Characterization
and distribution of pk1 and pk2 genes Six copies of the pk1 gene and three copies of the pk2 gene were identified in the contig assembly of the wVulC genome (Table 1). Each of the six putative prophage regions of the assembly contains one pk1 allele and three of these prophages also harbour one pk2 allele (Table 1). Two wVulC pk1 alleles (ANK46a/b and ANK60a/b) and one pk2 allele (ANK40a/b) were each found in two identical copies. These results were confirmed by Southern blotting (Additional file 1: Figure S1) and are consistent with the sequencing of PCR products (Table 1).