Table 4 shows the presence of genes encoding Hox orthologs in the genomes of Hymenolepis and Echinococcus spp., S. mansoni, polyopisthocotylean ‘monogeneans’, and the planarian S. mediterranea. From these representatives, it appears that flatworms have a core set of one anterior gene (Hox1/Lab) and three central
genes (Hox3, Hox4/Dfd, Lox4/Abd-A). CP-690550 solubility dmso In addition, both characteristic lophotrochozoan posterior Hox genes (Post-1/2) are found, although those were initially thought to be missing from flatworms (128,142). Planarians also show the presence of Hox5 orthologs and larger numbers of central and posterior paralogs than found in parasitic flatworms, although it must be noted that whereas some of the homeobox sequences (e.g. Hox1, Hox4/Dfd and Hox8/Abda) show high levels of similarity to cognates outside the group, other flatworm homeoboxes are divergent and difficult to classify. Nevertheless, compared with other major lophotrochozoan groups such as annelids and molluscs, both free-living and parasitic flatworms show reductions in the numbers of Hox gene classes, and this may relate to their lack of axial elaboration. Hymenolepis is also oddly missing Protein Tyrosine Kinase inhibitor an ortholog of the central Hox3 gene found in all other flatworms examined. In all cases, flatworm Hox genes are found to be widely dispersed in the genome and have been
shown previously to reside on at least two different chromosomes in S. mansoni (139). RNA-seq data indicate the presence of multiple non-Hox coding regions flanking the Hox genes in the Hymenolepis genome and thus further confirm the complete lack of clustering of flatworm Hox genes. The genomic structure of Hymenolepis orthologs appears normal, and full-length transcripts Selleck Depsipeptide range in size between ∼1500 (HmHox1)–2600 (HmPost-2) bp and are
made up of 2–4 exons separated by introns 81–8946 bp in length. The abdominal-B ortholog HmPost-2 shows a characteristic intron interrupting the homeobox region. In contrast, typically structured Post-1 orthologs have not been described in flatworms, and the one (possibly two) Hymenolepis Post-1 orthologs appear as pseudogenes, and full-length exons cannot be deduced from present data. Expression of Hox genes in parasitic flatworms is so far known only from quantitative PCR and RNA-seq data that indicate dynamic patterns throughout their complex life cycles. Stage-specific expression has been demonstrated in S. mansoni (139), the ‘monogenean’Polystoma gallieni (143), and in Hymenolepis and RNA-seq data in Hymenolepis also indicate at least minimal expression levels during both adult and larval development, with peaks of expression seen in central and posterior genes. How the dispersed structure of their genes affects the principal of colinearity is not known, and only a few studies of Hox spatial expression have been conducted in free-living flatworms, with somewhat inconsistent results (144), and none in parasitic flatworms.