Long-read assembly and comparative evidence-based reanalysis of Cryptosporidium genome sequences reveal expanded transporter repertoire and duplication of entire chromosome ends including subtelomeric regions

生物 微小隐孢子虫 基因组 遗传学 参考基因组 顺序装配 基因组计划 基因组浏览器 亚端粒 基因复制 基因 注释 基因注释 全基因组测序 染色体 隐孢子虫 计算生物学 基因组学 转录组 粪便 基因表达 古生物学
作者
Rodrigo P. Baptista,Yiran Li,Adam Sateriale,Mandy Sanders,Karen Brooks,Alan Tracey,Brendan R. E. Ansell,Aaron R. Jex,Garrett W. Cooper,Ethan Smith,Rui Xiao,Jennifer E. Dumaine,Peter Georgeson,Bernard J. Pope,Matthew Berriman,Boris Striepen,James A. Cotton,Jessica C. Kissinger
出处
期刊:Genome Research [Cold Spring Harbor Laboratory]
卷期号:32 (1): 203-213 被引量:57
标识
DOI:10.1101/gr.275325.121
摘要

Cryptosporidiosis is a leading cause of waterborne diarrheal disease globally and an important contributor to mortality in infants and the immunosuppressed. Despite its importance, the Cryptosporidium community has only had access to a good, but incomplete, Cryptosporidium parvum IOWA reference genome sequence. Incomplete reference sequences hamper annotation, experimental design, and interpretation. We have generated a new C. parvum IOWA genome assembly supported by Pacific Biosciences (PacBio) and Oxford Nanopore long-read technologies and a new comparative and consistent genome annotation for three closely related species: C. parvum , Cryptosporidium hominis , and Cryptosporidium tyzzeri . We made 1926 C. parvum annotation updates based on experimental evidence. They include new transporters, ncRNAs, introns, and altered gene structures. The new assembly and annotation revealed a complete Dnmt2 methylase ortholog. Comparative annotation between C. parvum , C. hominis , and C. tyzzeri revealed that most “missing” orthologs are found, suggesting that the biological differences between the species must result from gene copy number variation, differences in gene regulation, and single-nucleotide variants (SNVs). Using the new assembly and annotation as reference, 190 genes are identified as evolving under positive selection, including many not detected previously. The new C. parvum IOWA reference genome assembly is larger, gap free, and lacks ambiguous bases. This chromosomal assembly recovers all 16 chromosome ends, 13 of which are contiguously assembled. The three remaining chromosome ends are provisionally placed. These ends represent duplication of entire chromosome ends including subtelomeric regions revealing a new level of genome plasticity that will both inform and impact future research.

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