Abstract
Background
Anopheles sinensis (Diptera: Culicidae) is a primary vector of Plasmodium vivax and Brugia malayi in most regions of China. In addition, its phylogenetic relationship with the cryptic species of the Hyrcanus Group is complex and remains unresolved. Mitochondrial genome sequences are widely used as molecular markers for phylogenetic studies of mosquito species complexes, of which mitochondrial genome data of An. sinensis is not available.
Methods
An. sinensis samples was collected from Shandong, China, and identified by molecular marker. Genomic DNA was extracted, followed by the Illumina sequencing. Two complete mitochondrial genomes were assembled and annotated using the mitochondrial genome of An. gambiae as reference. The mitochondrial genomes sequences of the 28 known Anopheles species were aligned and reconstructed phylogenetic tree by Maximum Likelihood (ML) method.
Findings
The length of complete mitochondrial genomes of An. sinensis was 15,076 bp and 15,138 bp, consisting of 13 protein-coding genes, 22 transfer RNA (tRNA) genes, 2 ribosomal RNA (rRNA) genes, and an AT-rich control region. As in other insects, most mitochondrial genes are encoded on the J strand, except for ND5, ND4, ND4L, ND1, two rRNA and eight tRNA genes, which are encoded on the N strand. The bootstrap value was set as 1000 in ML analyses. The topologies restored phylogenetic affinity within subfamily Anophelinae. The ML tree showed four major clades, corresponding to the subgenera Cellia, Anopheles, Nyssorhynchus and Kerteszia of the genus Anopheles.
Conclusions
The complete mitochondrial genomes of An. sinensis were obtained. The number, order and transcription direction of An. sinensis mitochondrial genes were the same as in other species of family Culicidae.
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Multilingual abstracts
Please see Additional file 1 for translations of the abstract into the six official working languages of the United States.
Background
Anopheles sinensis Wiedemann, 1828 is an oriental species with a wide distribution in China [1]. It is a vector of Plasmodium vivax in plain regions of central China, and certain worms such as Brugia malayi that cause lymphatic filariasis [2, 3]. Despite its disputable malaria vector capacity, An. sinensis is still incriminated as a competent vector for Plasmodium vivax malaria due to its abundant population size and wide distribution, which have led to occasional local malaria epidemics or outbreaks throughout history [4].
Anopheles sinensis is one of the members in the Hyrcanus Group. The Hyrcanus Group is an extremely complex species assemblage of the genus Anopheles subgenus Anopheles, which includes above 20 closely related species in China [1, 5, 6]. Because of similar morphological characters of female adult, the identification of these species in the group has been taxonomically problematic. Such as, An. sinensis was almost impossible distinguished from its sibling species (An. lesteri, An. yatsushiroensis, An. kleini, and so on) [1]. The PCR assay was established by sequences of second internal transcribed spacer (ITS2) region of the ribosomal DNA (rDNA) to identify An. sinensis from its cryptic species members of Hyrcanus Group [5]. The genetic structure of An. sinensis populations in China were also detected by molecular markers, and the weak genetic structure may be a consequence of low genetic differentiation and high gene flow among populations in central China [7,8,9,10]. However, there are still some issues to be elucidated in the molecular classification of An. sinensis, such as natural hybrid between An. kleini and An. sinensis was discovered in the Republic of Korea [11, 12] and China (unpublished data). So, the evolutionary relationship of An. sinensis, such as speciation and other issues need to be elucidated further.
Mitochondrial genomes strictly follow maternal inheritance in structure and evolution, and contain abundant information for population genetic and phylogenetic studies [13,14,15,16,17,18,19,20,21]. There is no adequate mitogenome information available for An. sinensis. In this study, we used next-generation sequencing to characterize the mitochondrial genomes of An. sinensis, and to reconstruct phylogenetic tree of the known Anopheles species.
Methods
Mosquito collection and species identification
Wild mosquito adults were collected by CDC mini light traps (BioQuip, USA) or artificial catching aspirator at livestock corrals from Jining and Caoxian County in Shandong Province, China in July, 2012. With the owners’ consent, the light traps were set up in cow pens from 18:30 pm to 8:30 am next day. Mosquitoes of the An. hyrcanus group were sorted out in the field by morphology using the identification keys [1], and kept individually in silica gel filled tubes at 4 °C until DNA extraction. After being brought back to the laboratory, the female adults were separated into head and body. The single head was used to identify species by PCR assay based on rDNA ITS2 sequences [5]. Twenty bodies pool of An. sinensis species was extracted genomic DNA using Meta-G-Nome™ DNA Isolation Kit (Epicentre, USA), followed by Illumina sequencing.
Metagenome sequencing
Genomic DNA was fragmented and sequencing libraries were prepared, which insert size was about 700 bp. Double-end pairing sequencing was performed using Illumina HiSeq 2000 (Genewiz, USA). Each library was sequenced to generate about 20 million paired-end reads from each sample. The mean length of reads was 101 base pairs.
Mitochondrial genome assembly and annotation
The quality of total reads was controlled by FASTQC (http://www.bioinformatics.babraham.ac.uk/projects/fastqc/), then the high quality reads were mapping to An. sinensis genome (SAMN02910229) [22]. The contigs were assembled by KmerGenie softwares [23], and aligned with mitochondrial genome of Culicidae mosquitoes on GenBank BLAST website, which identity threshold value was set as 90%. The complete mitochondrial genome of An. sinenesis was obtained, including 13 protein coding genes, 22 transfer RNA (tRNA) genes, 2 ribosomal RNA (rRNA) genes and AT-rich control region. The genes and region of the mitochondrial genome were identified by comparison with the reference mitogenome sequences of An. gambiae (GenBank Accession No. L20934.1) and other Anopheles mosquitoes. Some parts fragments such as CO1 and CO2 region were verified by PCR products [7, 24].
Phylogenetic analysis
A total of 28 Anopheles species (including An. sinensis in this study) mitochondrial genome sequences from NCBI database available were analyzed by MEGA 6 software [25]. The phylogenetic relationships of the mitogenome DNA sequences for Anopheles mosquitoes were reconstructed using Maximum Likelihood (ML) method with PhyML 3.0 [26]. The best fit model of nucleotide substitution, the GTR + I + G model, was determined for the ML tree inference with Modeltest 3.7 [27]. The bootstrap values for 1000 replicates were calculated.
Results and discussion
Mitogenome organization and composition
The length of two complete mitochondrial genomes of An. sinensis were obtained from two samples, which were 15,076 bp and 15,138 bp, respectively. Both sequences was conserved, except the length of AT-rich control region. One of the complete mitochondrial genome sequence was chosen for further analysis, which was submitted to GenBank (Accession No. KT218684.1).
The mitochondrial genomes of An. sinensis mosquitoes consisted of circular DNA molecules, contained 13 protein-coding genes, 22 transfer RNA (tRNA) genes, 2 rRNA genes (12S rRNA and 16S rRNA), and an AT-rich control region (Fig. 1). The mitochondrial genes showed no length variation on either the J or N strand. The AT-rich control region was located between the SrRNA and tRNA-Ile genes.
Protein coding genes
The mitochondrial genome of An. sinensis species consisted of 13 intron-less protein coding genes. The gene number, order and transcription direction of mitochondrial genes were the same as in other species of Culicidae species [13,14,15, 17, 19, 21, 28,29,30,31,32,33]. There were 9 genes located in the J strand, as ND2, CO1, CO2, ATPase8, ATPase6, CO3, ND3, ND6 and CytB, while ND1, ND5, ND4 and ND4L located in the N strand. The length of nucleotides and amino acids of these 13 genes were showed in Table 1.
Transfer and ribosomal RNAs genes
All 22 tRNA genes were dispersed in the mitochondrial genome of An. sinensis, the length and position of them was similar with the reported Culicidae mosquitoes (Table 2) [13,14,15, 20, 21, 28, 29, 31,32,33]. Among them, there were two kinds of transfer genes for serine and leucine, and the remaining 18 tRNA genes correspond to the other amino acid respectively. The arrangement of tRNA-Arg and tRNA-Ala was inverse compared with the insects of family Drosophilidae, Tephritidae, Calliphoridae, Muscidae and Ceratopogonidae [34,35,36].
There were 2 rRNA genes in mitochondrial genome of An. sinensis, both located in the N strand. The length of SrRNA gene was 692 bp encoding 12S rRNA, and the LrRNA gene was 1329 bp encoding 16S rRNA.
Phylogenetic analysis
The molecular phylogenetic relationship using complete mitochondrial genome sequence of 28 Anopheles species was analyzed. All sequences generated in this study have been deposited in the GenBank. The topologies restored phylogenetic affinity within subfamily Anophelinae (Fig. 2). The ML tree showed that two major clades with mosquitoes in subgenus Kerteszia (n = 4) and the other three subgenera, as Cellia (n = 16), Anopheles (n = 3), Nyssorhynchus (n = 5) in genus Anopheles. The latter subgenera Cellia, Anopheles and Nyssorhynchus were monophyly, and the subgenera Cellia with Anopheles was sister relationship. The bootstrap values were almost above 50%.
Conclusions
The complete mitochondrial genomes of An. sinensis were obtained. The number, order and transcription direction of An. sinensis mitochondrial genes were the same as in other species of Culicidae. And the complete mitogenome data can provide basic information for analyzing phylogenetic relationship of mosquito species.
Abbreviations
- ITS2:
-
Second internal transcribed spacer
- ML:
-
Maximum likelihood
- rDNA:
-
Ribosomal DNA
- rRNA:
-
Ribosomal RNA
- tRNA:
-
Transfer RNA
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Acknowledgements
We are grateful to Mao-Qing Gong and Peng Cheng (Shandong Provincial Institute of Parasitic diseases control), Chun-Yan Nan, Tong Wu, who provided field assistance in the study.
Funding
This work was supported by the National Natural Sciences Foundation of China (No. 81371848) and the Infective Diseases Prevention and Cure Project of China (No. 2017ZX10303404–002).
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All data generated or analyzed during this study are included in this published article.
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All authors read and approved the final version of the manuscript. YM designed the study and did morphological identification. YM and XL collected mosquito specimens in the field, YW did species molecular identification. KC, YW and HP did data analysis. KC, YW, HP and YM wrote the manuscript.
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No specific permits were required for this study. The study did not involve endangered or protected species. Therefore, the local ethics committee deemed that approval was unnecessary.
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The authors declared that they have no competing interests.
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Additional file 1:
Multilingual abstracts in the six official working languages of the United Nations. (PDF 666 kb)
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Chen, K., Wang, Y., Li, XY. et al. Sequencing and analysis of the complete mitochondrial genome in Anopheles sinensis (Diptera: Culicidae). Infect Dis Poverty 6, 149 (2017). https://doi.org/10.1186/s40249-017-0362-7
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DOI: https://doi.org/10.1186/s40249-017-0362-7