Literature DB >> 24572609

PCR detection of Babesia ovata from questing ticks in Japan.

Thillaiampalam Sivakumar1, Muncharee Tattiyapong1, Kazuhiro Okubo1, Keisuke Suganuma1, Kyoko Hayashida1, Ikuo Igarashi1, Satoshi Zakimi2, Kotaro Matsumoto3, Hisashi Inokuma3, Naoaki Yokoyama4.   

Abstract

Babesia ovata is a tick-transmitted hemoprotozoan parasite of cattle. In the present study, we analyzed tick DNA samples (n=1459) prepared from questing ticks collected from various cattle pastures in Hokkaido (Shibecha, Taiki, Otofuke, Memuro, and Shin-Hidaka districts) and Okinawa (Yonaguni Island) prefectures of Japan for B. ovata. When all the tick DNA samples were screened by a previously described B. ovata-specific apical membrane antigen-1 (AMA-1) gene-based polymerase chain reaction (PCR) assay, none of the DNA samples was positive. Therefore, we developed a PCR assay based on the protozoan beta-tubulin (β-tubulin) gene to detect B. ovata from ticks in Japan. In the specificity test, the PCR assay amplified the expected 444-bp target gene fragment from B. ovata DNA. No PCR products were amplified from DNA samples from other blood pathogens, bovine blood, or ticks. In addition, the PCR assay detected 100 fg of B. ovata-genomic DNA extracted from an in vitro culture of the parasites. Subsequently, when all the tick DNA samples were screened by this new PCR assay, 18 were positive for B. ovata. Positive samples were found only in the Yonaguni and Memuro areas. In Okinawa, where all the ticks were identified as Haemaphysalis longicornis, 9.7% of the samples were PCR-positive, while a single tick (Ixodes ovatus) from Memuro was infected with B. ovata. When the nucleotide sequences of the PCR amplicons were phylogenetically analyzed, they formed a separate clade containing a previously described β-tubulin gene sequence from B. ovata (Miyake strain), confirming that the PCR assay had detected only B. ovata from the tick DNA samples. This is the first report that describes the PCR detection of B. ovata in ticks. The findings warrant transmission experiments to evaluate I. ovatus as a potential vector of B. ovata.
Copyright © 2014 Elsevier GmbH. All rights reserved.

Entities:  

Keywords:  Babesia ovata; Beta-tubulin; Japan; PCR; Ticks

Mesh:

Substances:

Year:  2014        PMID: 24572609     DOI: 10.1016/j.ttbdis.2013.12.006

Source DB:  PubMed          Journal:  Ticks Tick Borne Dis        ISSN: 1877-959X            Impact factor:   3.744


  7 in total

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Journal:  Parasitol Res       Date:  2018-12-17       Impact factor: 2.289

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Journal:  Front Cell Infect Microbiol       Date:  2022-06-21       Impact factor: 6.073

3.  Establishment of a novel tick-Babesia experimental infection model.

Authors:  Hiroki Maeda; Takeshi Hatta; M Abdul Alim; Daigo Tsubokawa; Fusako Mikami; Makoto Matsubayashi; Takeharu Miyoshi; Rika Umemiya-Shirafuji; Shin-Ichiro Kawazu; Ikuo Igarashi; Masami Mochizuki; Naotoshi Tsuji; Tetsuya Tanaka
Journal:  Sci Rep       Date:  2016-11-14       Impact factor: 4.379

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Journal:  J Arthropod Borne Dis       Date:  2017-09-08       Impact factor: 1.198

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Authors:  Mpho Tawana; ThankGod E Onyiche; Tsepo Ramatla; Sibusiso Mtshali; Oriel Thekisoe
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Authors:  Qingli Niu; Zhijie Liu; Peifa Yu; Jifei Yang; Mirza Omar Abdallah; Guiquan Guan; Guangyuan Liu; Jianxun Luo; Hong Yin
Journal:  Parasit Vectors       Date:  2015-10-09       Impact factor: 3.876

Review 7.  The specificity of Babesia-tick vector interactions: recent advances and pitfalls in molecular and field studies.

Authors:  Anna Bajer; Dorota Dwużnik-Szarek
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  7 in total

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