This is the first report of the complete genome sequence of Rickettsia asiatica strain Maytaro1284, isolated from an Ixodes ovatus tick in Japan. The genome contains a 1,344,324-bp circular chromosome and one plasmid of 74,761 bp. There was no outer membrane protein A (ompA) gene encoded in the genome.
ABSTRACT
This is the first report of the complete genome sequence of Rickettsia asiatica strain Maytaro1284, isolated from an Ixodes ovatus tick in Japan. The genome contains a 1,344,324-bp circular chromosome and one plasmid of 74,761 bp. There was no outer membrane protein A (ompA) gene encoded in the genome.
ANNOUNCEMENT
The members of the genus Rickettsia are Gram-negative obligate intracellular bacteria belonging to the class Alphaproteobacteria (1) with 32 designated species divided into four groups, spotted fever (SFG), typhus (TG), transitional (TGR), and ancestral (AG) groups (2). Molecular classification of rickettsial species can be achieved based on the sequences of the 16S rRNA gene, ompA, ompB, sca4, gltA, and htrA (3).
SFG rickettsiae are mainly associated with ticks, and some are pathogenic for humans. In Japan, six validated SFG rickettsiae, namely, Rickettsia japonica, R. helvetica, R. heilongjiangensis, R. tamurae, R. monacensis, and R. asiatica, and several other uncharacterized rickettsial species/genotypes have been detected (4, 5). R. asiatica is the only named species of these whose genome sequence is not available.
R. asiatica, initially described as a Rickettsia strain IO-1T, was first isolated from Ixodes ovatus ticks collected in Fukushima Prefecture, Japan, in 1993 (6, 7). A recent study revealed that R. asiatica had a strong host specificity, where it was detected only in I. ovatus (5).
R. asiatica strain Maytaro1284 was isolated from an I. ovatus tick collected in Yamagata prefecture, Japan (8). In brief, tick homogenate was inoculated into Ixodes scapularis ISE6 cells and incubated at 32°C. The isolate was obtained at 28 days after inoculation without showing any cytopathic effect. Rickettsia DNA was purified from infected cells by centrifugation and filtration with a 5.0-μm-pore-size membrane filter. DNA was extracted using a MagAttract HMW DNA kit (Qiagen, Hilden, Germany). An Illumina (Hayward, CA) library was constructed with the Nextera DNA library prep kit and run on an Illumina MiSeq 600-cycle instrument. For PacBio sequencing, genomic DNA was sheared using a G-Tube (Covaris, Woburn, MA) to generate 20-kb fragments. A PacBio library was constructed using the SMRTbell template prep kit 1.0 (Pacific Biosciences, Menlo Park, CA) and sequenced using C4 chemistry on a PacBio RS II instrument.
We acquired 10,353,766 reads with 2,789,655,408 bp and 92,498 reads with 1,954,307,128 bp by MiSeq and PacBio RS II, respectively. The PacBio reads were assembled using PacBio’s Hierarchical Genome Assembly Process (HGAP3, SMRT Analysis 2.3.0) (9), and 3,693 contigs with 8,182,413 bp were obtained. The contigs and raw reads from MiSeq were further assembled using SPAdes 3.11.1 (10), resulting in five contigs of 535,925 bp, 417,525 bp, 311,286 bp, 77,822 bp, and 74,888 bp. The first four contigs were merged into one circular sequence by filling the gaps between contigs using Sanger sequencing. The last contig was manually circularized by eliminating an overlapping end. All software was run with default parameters.
The assembled circular chromosome of 1,344,324 bp had an overall GC content of 32.3%, while one plasmid (pRA1) was 74,761 bp in size with an overall GC content of 33.8%. The average coverages obtained for the chromosome and plasmid genomes were 832× and 1,787×, respectively. Annotation was performed with DFAST (11). The chromosome contains 1,513 protein-coding sequences (CDSs), 3 rRNA genes (5S, 16S, and 23S), and 34 tRNA genes. The plasmid is predicted to contain 194 CDSs.
R. asiatica was suspected to lack the ompA gene due to the failure of PCR amplification of the gene (7). However, it is also evident that PCR failures of polymorphic genes such as ompA, ompB, and sca4 are common issues in the genetic characterization of rickettsiae because of nucleotide mismatches in the primer annealing sites (5, 12). This study confirmed that there is no ompA gene in the genome of R. asiatica.
Data availability.
The genome sequences have been deposited at DDBJ/EMBL/GenBank under the accession numbers AP019563 and AP019564, BioProject number PRJDB8064, and BioSample number SAMD00165215. The raw sequencing reads were submitted to the DRA under the accession number DRA008361.
ACKNOWLEDGMENTS
This study was supported by JSPS KAKENHI grant numbers 15H05633, 16H06431, and 19H03118.
Computations were partially performed on the NIG supercomputer at the ROIS National Institute of Genetics and Human Genome Center (The University of Tokyo).
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Data Availability Statement
The genome sequences have been deposited at DDBJ/EMBL/GenBank under the accession numbers AP019563 and AP019564, BioProject number PRJDB8064, and BioSample number SAMD00165215. The raw sequencing reads were submitted to the DRA under the accession number DRA008361.