Real-time PCR biochip for on-site detection of Coxiella burnetii in ticks

A-Tai Truong; Bo-Ram Yun; Jiyeon Lim; Subin Min; Mi-Sun Yoo; Soon-Seek Yoon; Young-Min Yun; Jong-Taek Kim; Yun Sang Cho

doi:10.1186/s13071-021-04744-z

Real-time PCR biochip for on-site detection of Coxiella burnetii in ticks

Parasit Vectors. 2021 May 6;14(1):239. doi: 10.1186/s13071-021-04744-z.

Authors

A-Tai Truong^{1

2}, Bo-Ram Yun¹, Jiyeon Lim¹, Subin Min¹, Mi-Sun Yoo¹, Soon-Seek Yoon¹, Young-Min Yun³, Jong-Taek Kim⁴, Yun Sang Cho⁵

Affiliations

¹ Parasitic and Honeybee Disease Laboratory, Bacterial and Parasitic Disease Division, Department of Animal & Plant Health Research, Animal and Plant Quarantine Agency, Gimcheon, 39660, Republic of Korea.
² Faculty of Biotechnology, Thai Nguyen University of Sciences, Thai Nguyen, 250000, Vietnam.
³ Department of Veterinary Internal Medicine, College of Veterinary Medicine, Jeju National University, Jeju, 63243, Republic of Korea.
⁴ College of Veterinary Medicine, Gangwon National University, Chuncheon, 24341, Republic of Korea.
⁵ Parasitic and Honeybee Disease Laboratory, Bacterial and Parasitic Disease Division, Department of Animal & Plant Health Research, Animal and Plant Quarantine Agency, Gimcheon, 39660, Republic of Korea. choys@korea.kr.

Abstract

Background: Q fever, a zoonosis caused by Coxiella burnetii, has adverse effects on public health. Ticks are vectors of C. burnetii and they contribute to the transmission of the pathogen. A tool for rapid, sensitive, and accurate detection of C. burnetii from ticks is important for the prevention of Q fever.

Methods: Ultra-rapid real-time PCR (UR-qPCR) as a chip-based real-time PCR system was developed for the detection of C. burnetii from ticks. The UR-qPCR system was established and evaluated for the rapidity, sensitivity, and specificity of C. burnetii detection.

Results: C. burnetii was detected using UR-qPCR from 5644 larval, nymphal, and adult ticks from 408 pools collected from livestock and epidemiologically linked environments in two provinces, Gangwon and Jeju, in Korea. Ticks from three species were identified; Haemaphysalis longicornis accounted for the highest number, present in 333 of 408 pools (81.62%), followed by Haemaphysalis flava in 62 pools (15.19%) and Ixodes nipponensis in 13 pools (3.19%). The rapidity and sensitivity of PCR detection was demonstrated with the sufficient amplification and detection of approximately 56 copies of C. burnetii DNA with only 20 min of PCR amplification. The kappa value for the diagnostic agreement between UR-qPCR and stationary qPCR was in perfect agreement (κ = 1). PCR detection and sequencing indicated that C. burnetii was present in 5 of the 408 pools (1.23%), in which four pools contained H. longicornis and one pool contained H. flava. The infection rates of C. burnetii in the tick pools collected from Gangwon and Jeju Provinces were 1.70% and 0.58%, respectively. Phylogenetic analysis indicated a close relationship between the detected C. burnetii and those originating from goats, humans, and ticks in different countries, such as the USA, France, Germany, and Serbia.

Conclusions: The methods described in this study could be important for the prevention and control of Q fever in the two provinces. The UR-qPCR, with its features of mobility, sensitivity, and rapidity, is helpful for constructing early alert systems in the field for C. burnetii in ticks and could help alleviate the transmission of and economic damage due to Q fever.

Keywords: Asian longhorned tick; Haemaphysalis longicornis; Q fever; Tick-borne diseases; Ultra-rapid real-time PCR.

MeSH terms

Animals
Arthropod Vectors / microbiology
Coxiella burnetii / genetics
Coxiella burnetii / isolation & purification*
Genes, Bacterial
Humans
Ixodidae / microbiology*
Q Fever / diagnosis
Q Fever / prevention & control
Q Fever / transmission
Real-Time Polymerase Chain Reaction / methods*
Sensitivity and Specificity
Tick-Borne Diseases / microbiology
Tick-Borne Diseases / prevention & control
Tick-Borne Diseases / transmission

Grants and funding

B-1543081-2020-22-03/Animal and Plant Quarantine Agency