Abstract
Theileria annulata is a haemoprotozoan parasite that causes a cancer-like illness known as tropical theileriosis in cattle. In the course of analyzing the genetic diversity of T. annulata in Sri Lanka, we observed that merozoite-piroplasm surface antigen (tams1) and surface protein (tasp)-like gene sequences obtained from bovine blood DNA samples, which were PCR-positive for T. annulata, were conserved but shared low identity with T. annulata GenBank sequences. Moreover, the 18S rRNA sequences from the Sri Lankan samples contained ten unique single-nucleotide polymorphisms compared with all known T. annulata sequences. The cytochrome b (cob) gene sequences isolated from the Sri Lankan samples were highly conserved and shared low identity scores with similarly conserved T. annulata sequences from GenBank. Phylogenetic analysis showed that the Sri Lankan tams1-like, tasp-like, 18S rRNA, and cob sequences clustered together and formed sister clades to the common ancestors of all known T. annulata and Theileria lestoquardi sequences. These findings demonstrated that the Sri Lankan cattle were not infected with T. annulata but with a new Theileria sp. (designated as Theileria sp. Yokoyama) closely related to T. annulata.
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Introduction
The Theileria genus consists of tick-borne haemoprotozoan parasites of ruminants1. Among them, Theileria annulata infects cattle and buffalo, and causes a lymphoproliferative disease known as tropical theileriosis2. The disease is usually characterised by enlarged lymph nodes, fever, increased pulse and respiratory rates, swollen eyelids, profuse lachrymation, anaemia, jaundice, and sometimes death3,4. Therefore, tropical theileriosis is considered an economically significant disease in endemic countries5,6,7. Long-term survival of T. annulata in host animals is facilitated by the protozoan’s genetic diversity, which helps the parasite escape the host’s immune response8,9. Therefore, T. annulata’s genetic diversity has been analysed in several endemic countries based on genes that encode surface proteins, such as the Theileria annulata merozoite-piroplasm surface antigen (tams1) and Theileria annulata surface protein (tasp) genes10,11,12,13. The tams1 and tasp genes have been demonstrated to be highly diverse in most endemic countries investigated to date.
Sri Lanka is a tropical country, and previous PCR-based studies found that infection with T. annulata is common among the country’s cattle populations14,15. However, the genetic diversity of T. annulata remains to be investigated in Sri Lanka. Therefore, in the present study, we analysed the tams1 and tasp gene sequences in DNA samples from Sri Lankan bovine blood, which were PCR-positive for T. annulata. As the findings suggested that the genetic backgrounds of Sri Lankan isolates might be different from those of T. annulata, further analyses were conducted using the 18S rRNA and cytochrome b (cob) gene sequences.
Results
Thirty-nine bovine blood DNA samples from the Polonnaruwa and Nuwara Eliya districts in Sri Lanka, which had tested positive on a T. annulata-specific PCR assay, were used in the present study15. From these samples, tams1-like gene sequences were successfully isolated from 34 samples (GenBank accession no. LC467536 - LC467569), including 28 from Polonnaruwa and 6 from Nuwara Eliya. The newly determined tams1-like nucleotide and translated amino acid sequences were highly conserved but shared low identity scores with T. annulata sequences (n = 125) from ten countries: Sudan, Tunisia, Mauritania, Bahrain, Turkey, Italy, Spain, Portugal, India, and China (Table 1). Multiple alignment of nucleotide sequences revealed that the TCC nucleotides, which were conserved across all T. annulata sequences at positions 598–600, were deleted in the Sri Lankan sequences (Fig. S1). The deletion of these nucleotides resulted in deletion of amino acid serine in Sri Lankan sequences (Fig. S2). Phylogenetically, the tams1 nucleotide and amino acid sequences from GenBank formed multiple clades, and the clade formed by the tams1 homologous sequences in Theileria lestoquardi was nested within the T. annulata clades (Figs 1 and S3). However, the Sri Lankan sequences formed a sister clade to the common ancestor of all T. annulata and T. lestoquardi sequences in GenBank (Figs 1 and S3).
The tasp gene sequences were isolated from 32 DNA samples (GenBank accession no. LC467570 - LC467601), including 25 and 7 sequences from Polonnaruwa and Nuwara Eliya, respectively. Length polymorphism was observed among the newly determined sequences, with 22 and 10 sequences containing 1,023 bp and 1,020 bp, respectively. As previously reported, the tasp-like sequences had two short introns12, which were removed from the primer-trimmed Sri Lankan sequences to obtain 839- and 842-bp coding sequences. The Sri Lankan coding nucleotide and amino acid sequences shared 97.3–100% and 95.4–100% identity scores, respectively, with each other and 77.9–83.2% and 67.5–73.9% identity scores, respectively, with the T. annulata sequences (n = 14) from Tunisia, Morocco, Turkey, India, and China (Table 1). The nucleotide and amino acid sequences at both ends of the tasp gene are usually conserved12. In contrast, the sequences in these regions, especially at the 5′ end in nucleotide sequences and N-terminal region in amino acid sequences, were poorly conserved between the Sri Lankan and T. annulata sequences (Figs S4 and S5). Phylogenetic analysis showed that that T. lestoquardi surface protein gene sequences formed a sister clade to the tasp sequences from GenBank, while all the Sri Lankan sequences formed a sister clade to the common ancestor of clades formed by the T. annulata and T. lestoquardi gene sequences (Fig. 2). A phylogeny constructed based on translated amino acid sequences had the same topology (Fig. S6). These findings suggested that the Sri Lankan isolates have genetic backgrounds that differed from those of T. annulata.
However, although the tams1 and tasp genes are markers for analysing genetic diversity among T. annulata, these genes are unsuitable for evolutionary studies because they evolved under immune pressure. Therefore, we isolated 1,185-bp 18S rRNA fragment (1,130 bp after primer regions were trimmed) from 37 DNA samples (GenBank accession no. LC467602 - LC467638), including 31 from Polonnaruwa and 6 from Nuwara Eliya. These 18S rRNA sequences were highly conserved (99.5%–100% identities) and shared marginally low identities (98.0%–99.2%) with 63 T. annulata sequences from six countries, including Iran, Turkey, Spain, India, China, and Pakistan (Table 1). Phylogenetic analysis showed that the Sri Lankan sequences formed a monophyletic sister clade to the common ancestors of the T. annulata and T. lestoquardi 18S rRNA sequences (Fig. 3). However, the clades were supported with low bootstrap values. Thus, we isolated relatively long fragment (1,536 bp after primer regions were trimmed) of 18S rRNA sequences (GenBank accession no. LC495907 - LC495915), using a set of universal forward and reverse primers, from nine samples with single infection. In these sequences, we identified ten unique single-nucleotide polymorphisms (SNPs), including a deletion and nine substitutions compared with the GenBank-derived T. annulata sequences (Fig. S7). The topologies of phylogenetic trees constructed with short and long 18S rRNA sequences were similar, but the bootstrap support for clades drastically increased in the later (Fig. 4).
Although the phylogenetic position and unique SNPs may identify the Sri Lankan isolates as a new Theileria sp., this assumption remains inconclusive as the 18S rRNA sequences shared high identity scores with the T. annulata sequences. Therefore, we obtained 30 cob gene sequences (GenBank accession no. LC467639 - LC467668), including 28 from Polonnaruwa and 2 from Nuwara Eliya, and compared them with the 43 T. annulata sequences from Sudan, Tunisia, Egypt, Turkey, India, and China. The T. annulata cob nucleotide and translated amino acid sequences from these countries were highly conserved, sharing 98.5–100% and 97.1–100% identity scores, respectively (Table 1). In contrast, these sequences shared only 87.2–88.0% and 82.5–84.8% identities with the Sri Lankan cob nucleotide and amino acid sequences, respectively (Figs S8 and S9). In addition, the Sri Lankan cob gene sequences were characterized by 122 unique SNPs compared with the GenBank-derived T. annulata sequences (Fig. S8). Phylogenetic analysis showed that the Sri Lankan cob nucleotide as well as amino acid sequences clustered together and formed a sister clade to the T. annulata clade (Figs 5 and S10), further supporting our assumption that the Theileria sp. from the cattle in Sri Lanka is not T. annulata but a Theileria sp. closely related to T. annulata.
Discussion
The unique polymorphisms, low identity scores shared with the T. annulata sequences, and distinct phylogenetic positions collectively indicated that the parasite species from Sri Lanka, identified via PCR as T. annulata, was indeed a new Theileria sp. closely related to T. annulata.
Although the present study was initiated to analyse the genetic diversity of T. annulata in Sri Lanka, the tams1- and tasp-like sequences from the Sri Lankan samples diverged from known T. annulata sequences. However, there is no bootstrap support for the T. annulata clade in tams1 phylogeny. The genetic diversity of tams1 is thought to be due to random intragenic recombination, which results in a mosaic pattern of diversity16. This could explain the lack of bootstrap support for the T. annulata clade. In addition, there are no bootstrap values for the separation of Sri Lankan clades in both tams1 and tasp phylogenies due to lack of additional outgroup sequences. In tams1 phylogeny, addition of further outgroup sequences, such as those from Theileria taurotragi and Theileria orientalis, however resulted in altered topology due to deletion of regions shared between T. annulata and T. lestoquardi from the alignment during phylogeny construction. Therefore, we refrained from using additional outgroup sequences in the tams1 phylogeny. For the tasp phylogeny, we could not find suitable additional outgroup sequences.
Next, short 18S rRNA sequences from the Sri Lankan samples were analysed. In phylogeny, the Sri Lankan sequences occurred in a clade unrelated to T. annulata. However, T. annulata, T. lestoquardi, and Sri Lanka clades and their separation were not supported by bootstrap values. Phylogenies constructed with short 18S rRNA sequences are sometimes characterized by low bootstrap values, which usually improve when longer sequences are used17. Therefore, we isolated relatively longer 18S rRNA sequences and used them for phylogeny construction. The topology of this phylogeny was similar to that constructed with short 18S rRNA sequences, but the bootstrap support for each clade and their separation drastically improved. Theileria lestoquardi is thought to have recently evolved from T. annulata, following a host jump from cattle/buffalo to sheep/goat18. Despite the similarities between T. lestoquardi and T. annulata, they are considered as distinct parasite species because of the stringent host-specificity of the former as confirmed by in vitro and in vivo experiments19. Therefore, our observation that the Sri Lankan clade in 18S rRNA phylogeny formed sister clade to the common ancestor of T. lestoquardi and T. annulata indicated that the Sri Lankan samples were infected with a new Theileria sp.
However, in terms of identity scores, the Sri Lankan 18S rRNA sequences differed only marginally from the T. annulata sequences. High identities are common between 18S rRNA sequences from different Theileria species possibly due to recent speciation events20. The hypervariable region of the 18S rRNA from T. lestoquardi differs by only two nucleotides compared with T. annulata21. Similarly, 18S rRNA is highly conserved between Theileria parva and Theileria sp. (buffalo)22. However, mitochondrial gene sequences adequately discriminated these parasite species20. Among the T. annulata mitochondrial genes, only the cob sequences were available in sufficient numbers in the GenBank. Therefore, we obtained the cob sequences from the Sri Lankan samples and compared them with those from T. annulata isolates in different countries23,24. The Sri Lankan sequences were conserved but highly diverse compared with the similarly conserved T. annulata sequences. To the best of our knowledge, such a high diversity of mitochondrial genes was never reported for any species of protozoan parasites. These observations suggest that the parasite species, which had been previously identified as T. annulata in Sri Lanka, is a novel Theileria sp.
The tams1-like gene sequences in the new Theileria sp. were highly conserved. Similarly, although the tasp-like sequences from Sri Lanka had some diversity, the gene was relatively conserved compared with the T. annulata sequences. Low genetic diversity among Theileria parasites is thought to be due to their short evolutionary histories. For example, the genetic diversity of T. parva in buffalo is greater than that in cattle because this pathogen has evolved longer in the former host than in the later8. Similarly, in T. lestoquardi, the genetic diversity of the tams1 homologous gene is lower than that of the tams1 gene because T. lestoquardi is thought to have recently evolved18. Therefore, there is a possibility that the new Theileria sp. was introduced in Sri Lanka relatively recently as a clonal population. If so, countries other than Sri Lanka may also be endemic to this Theileria sp. Epidemiological surveys to detect the new Theileria sp. in cattle from other countries may clarify this.
Previously, phylogenetic analyses conducted using 18S rRNA sequences found that the transforming Theileria species, including T. parva, T. annulata, T. taurotragi, Theileria sp. (buffalo), and T. lestoquardi, have a common ancestor20,25. Therefore, detecting the new Theileria sp. as a sister clade to the common ancestor of the T. annulata and T. lestoquardi sequences infers that the Theileria sp. may also be a transforming Theileria. However, isolation and in vitro cultivation of the schizont stage, together with genome sequencing analysis to identity the host cell transformation-related genes26, are essential to confirm whether the new Theileria sp. is a transforming species.
In conclusion, the present study, which aimed to analyse the genetic diversity of T. annulata in Sri Lanka, unexpectedly revealed a novel Theileria sp. However, the morphological, clinical, and pathological distinctions of this novel Theileria sp. are yet to be investigated. Therefore, the new species was provisionally designated as Theileria sp. Yokoyama.
Methods
DNA samples
Thirty-nine archived DNA samples from blood collected from cattle in Polonnaruwa (n = 32) and Nuwara Eliya (n = 7) in June 2014 were used in the present study15. All animals were apparently healthy during sampling. DNA samples were prepared from 200 µl of whole blood using a commercial kit (Qiagen, Hilden, Germany) following the manufacturer’s instructions. All DNA samples were positive for T. annulata via PCR assay based on the tams1 gene15,27.
PCR amplification, cloning, and sequencing of tams1, tasp, 18S rRNA, and cob
The 18S rRNA and the tams1, tasp, and cob gene sequences were amplified via PCR assays using primer sets designed in the present study. Briefly, three sets of forward and reverse primers were designed to amplify the full-length tams1, tasp, and cob genes using multiple alignments based on the T. annulata gene sequences retrieved from GenBank (Table 2). For the 18S rRNA, T. annulata-specific forward and reverse primers were designed to amplify an 1,185-bp fragment based on multiple alignment of the 18S rRNA sequences from bovine Babesia and Theileria species, including B. bovis, B. bigemina, and T. orientalis, because some of the T. annulata-positive DNA samples were coinfected with these species15. In addition, previously described universal forward28 and reverse29 primers were used to amplify a long fragment of 18S rRNA (≈1600 bp) from nine DNA samples with single infection. Each PCR assay was conducted in a 10-µl reaction mixture containing 1 µl of T. annulata-positive genomic DNA, 1 × PCR buffer (10 × PCR buffer, Applied Biosystems, Branchburg, NJ, USA), 200 µM of each dNTP (Applied Biosystems), 0.5 µM of each forward and reverse primer, 0.1 µl of 5 U/µl taq polymerase (Applied Biosystems), and 5.9 µl distilled water. The reaction mixture was then subjected to an initial predenaturation step at 95 °C for 5 min, followed by 45 cycles each of denaturation at 95 °C for 30 sec, an annealing step at the appropriate temperature (listed in Table 1) for 30 sec, and an extension step at 72 °C for 2 min. After a final elongation step at 72 °C for 7 min, the PCR products were resolved by 1.5% agarose gel electrophoresis, stained with ethidium bromide, and visualized under ultraviolet (UV) illumination. PCR bands with appropriate sizes were gel-extracted, ligated to PCR 2.1 plasmid vectors, and sequenced using an ABI PRISM 3100 genetic analyser (Applied Biosystems). All sequences generated in the present study were trimmed to remove the primer regions before conducting the sequencing and phylogenetic analyses.
Gene sequences from GenBank
The T. annulata tams1 gene sequences (n = 125) and coding sequences (n = 14) of the tasp gene with 100% coverage to the Sri Lankan sequences were retrieved from GenBank. Similarly, 63 and 38 T. annulata 18S rRNA sequences with 100% coverage to the Sri Lankan short and long 18S rRNA sequences, respectively, were also retrieved from GenBank. Nucleotide sequences with degenerate bases or an “n” symbol were omitted. In addition, some 18S rRNA sequences registered as derived from T. annulata (MF287917, MF287919, MF287920, MF287924, MF287934, MF287937, MF287939, MF287942, MF287948, MF287949, MF287950, KT736499, KT367869, and KT367870) were ignored because they shared high identity scores with T. orientalis compared with T. annulata in our BLAST search. The GenBank-derived T. annulata nucleotide and amino acid sequences were aligned with the Sri Lankan sequences, and then trimmed to remove the excess nucleotides or amino acids. For the cob gene, the T. annulata sequences (n = 43) from GenBank with 98% coverage to the Sri Lankan sequences were obtained. These cob nucleotide sequences and translated amino acid sequences were aligned with the Sri Lankan sequences. Excess nucleotides or amino acids in the alignment were removed at the 3ʹ end or C-terminal based on the Sri Lankan sequences and at the 5ʹ end or N-terminal based on the Sudanese sequences.
Calculation of identity scores
Alignments of the 18S rRNA sequences and nucleotide and amino acid sequences of tams1, tasp (coding region), and cob genes, which contained both the GenBank-derived T. annulata and Sri Lankan sequences, were analysed using MatGAT software30 to calculate the identity scores among the Sri Lankan sequences, among the GenBank-derived sequences, and between the Sri Lankan and GenBank-derived sequences.
Phylogenetic analyses
18S rRNA sequences and nucleotide and amino acid sequences of tams1, tasp (coding region), and cob genes from GenBank and those determined in the present study were subjected to multiple alignment using Multiple Alignment using Fast Fourier Transform (MAFFT) online software31. The aligned sequences were analysed using Molecular Evolutionary Genetics Analysis (MEGA), version 6.0 software32 to predict the best-fitting substitution models based on the lowest Akaike information criterion (AIC) values. Subsequently, using nucleotide sequences, five maximum likelihood phylogenetic trees were constructed based on general time reversible33 (tams1, tasp, and 18S rRNA-short) and Tamura-Nei34 (18S rRNA-long and cob) substitution models, using MEGA software32. Similarly, three maximum likelihood phylogenetic trees were constructed using amino acid sequences based on Dayhoff35 (TAMS1), Whelan And Goldman36 (TASP), and JTT37 (COB) substitution models. All positions containing gaps were removed from the alignments before phylogeny construction.
Ethical approval
The Animal Care and Use Committee of Obihiro University of Agriculture and Veterinary Medicine, Japan, approved all animal procedures (approval number: 29–53). All experiments were carried out in accordance with the Fundamental Guidelines for Proper Conduct of Animal Experiment and Related Activities in Academic Research Institutions coming under the Ministry of Education, Culture, Sports, Science and Technology, Japan.
Data availability
The materials and datasets generated in the present study are available from the corresponding author upon reasonable request.
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Acknowledgements
We thank the staff at the Veterinary Research Institute, Sri Lanka, and Ms. Hiroko Yamamoto, Obihiro University of Agriculture and Veterinary Medicine, Japan, for their excellent technical assistance. This study was supported by grants from the Japan Society for Promotion of Science (JSPS) Grant-in-Aid for Scientific Research (JSPS KAKENHI Numbers 26257417 and 16H05033), Open Partnership Joint Projects of the JSPS Bilateral Joint Research Projects, and the AMED/JICA Science and Technology Research Partnership for Sustainable Development (SATREPS) project (Grant number 17jm0110006h0005).
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T.S. and N.Y. conceived the study. T.S., S.F. and B.T. conducted the experiments and analysed the data. H.K. and S.S.P.S. conducted the cattle surveys and provided the laboratory facilities for the initial screening. T.S. and N.Y. wrote the manuscript, which all authors subsequently edited.
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Sivakumar, T., Fujita, S., Tuvshintulga, B. et al. Discovery of a new Theileria sp. closely related to Theileria annulata in cattle from Sri Lanka. Sci Rep 9, 16132 (2019). https://doi.org/10.1038/s41598-019-52512-y
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DOI: https://doi.org/10.1038/s41598-019-52512-y
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