Abstract
BackgroundMicrosporidian Nosema bombycis has received much attention because the pébrine disease of domesticated silkworms results in great economic losses in the silkworm industry. So far, no effective treatment could be found for pébrine. Compared to other known Nosema parasites, N. bombycis can unusually parasitize a broad range of hosts. To gain some insights into the underlying genetic mechanism of pathological ability and host range expansion in this parasite, a comparative genomic approach is conducted. The genome of two Nosema parasites, N. bombycis and N. antheraeae (an obligatory parasite to undomesticated silkworms Antheraea pernyi), were sequenced and compared with their distantly related species, N. ceranae (an obligatory parasite to honey bees).ResultsOur comparative genomics analysis show that the N. bombycis genome has greatly expanded due to the following three molecular mechanisms: 1) the proliferation of host-derived transposable elements, 2) the acquisition of many horizontally transferred genes from bacteria, and 3) the production of abundnant gene duplications. To our knowledge, duplicated genes derived not only from small-scale events (e.g., tandem duplications) but also from large-scale events (e.g., segmental duplications) have never been seen so abundant in any reported microsporidia genomes. Our relative dating analysis further indicated that these duplication events have arisen recently over very short evolutionary time. Furthermore, several duplicated genes involving in the cytotoxic metabolic pathway were found to undergo positive selection, suggestive of the role of duplicated genes on the adaptive evolution of pathogenic ability.ConclusionsGenome expansion is rarely considered as the evolutionary outcome acting on those highly reduced and compact parasitic microsporidian genomes. This study, for the first time, demonstrates that the parasitic genomes can expand, instead of shrink, through several common molecular mechanisms such as gene duplication, horizontal gene transfer, and transposable element expansion. We also showed that the duplicated genes can serve as raw materials for evolutionary innovations possibly contributing to the increase of pathologenic ability. Based on our research, we propose that duplicated genes of N. bombycis should be treated as primary targets for treatment designs against pébrine.
Highlights
Microsporidian Nosema bombycis has received much attention because the pébrine disease of domesticated silkworms results in great economic losses in the silkworm industry
We sequenced the genome of two microsporidian parasites: N. bombycis and N. antheraeae. By comparing their genomes with a published distantly related Nosema genome, N. ceranae [10], we show that the N. bombycis genome surprisingly expands due to the production of duplicated genes, the proliferation of host-derived transposable elements, and the acquisitions of many horizontally transferred genes from bacteria
Genomic architecture of N. bombycis and N. antheraeae By using various sequencing platforms, 6.7X, 10X, and 28X physical coverage of whole genome sequence of N. bombycis were obtained from the Sanger sequencing method, the miniBAC end sequencing method, and the Illumina short-read sequencing method respectively (Additional file 1)
Summary
Microsporidian Nosema bombycis has received much attention because the pébrine disease of domesticated silkworms results in great economic losses in the silkworm industry. Compared to other known Nosema parasites, N. bombycis can unusually parasitize a broad range of hosts. Pébrine is caused by the infection of the microsporidian parasite, Nosema bombycis. This disease was first recognized during the destruction of the European silk industry in 1857 [4]. Since no effective treatment methods have been developed up to this point, the infections by N. bombycis inevitably cause devastating economic losses in the silkworm industry. Apart from the domesticated silkworms, N. bombycis can infect various lepidopteran insects [6,7,8], indicative of their broad hosts range
Sign-in/Register to view highlights & summary 
Published Version (
Free)
Talk to us
Join us for a 30 min session where you can share your feedback and ask us any queries you have
Schedule a call