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Rapid isothermal duplex real-time recombinase polymerase amplification (RPA) assay for the diagnosis of equine piroplasmosis.

Authors :
Lei, Rong
Wang, Xinyi
Zhang, Di
Liu, Yize
Chen, Qijun
Jiang, Ning
Source :
Scientific Reports; 3/5/2020, Vol. 10 Issue 1, p1-11, 11p
Publication Year :
2020

Abstract

Equine piroplasmosis (EP) is a severe disease of horses caused by the tick-borne protozoa Theileria equi (T. equi) and Babesia caballi (B. caballi). Infectious carriers are not always symptomatic, meaning there is a risk to non-enzootic areas. Regulatory tests for EP include sero-epidemiological methods for equine babesiosis, but these lack specificity due to cross-reactivity with other Babesia species. In this study, we present a real-time quantitative recombinase polymerase amplification (qRPA) method for fast simultaneous detection of both T. equi and B. caballi. In this method, primers and probes targeting the 18S rRNA gene of both T. equi and B. caballi, the ema-1 gene of T. equi and the bc48 gene of B. caballi were designed and evaluated. The sensitivity of qRPA was evaluated using the pUC57 plasmid DNA containing the target gene. For the pUC57-bc48 gene DNA, the R<superscript>2</superscript> value was 0.983 for the concentration range 0.2 ng (4.1 × 10<superscript>7</superscript> DNA copies) to 2.0 fg (4.1 × 10<superscript>1</superscript> DNA copies). For the pUC57-ema gene DNA, the R<superscript>2</superscript> value was 0.993 for the concentration range 0.2 ng (5.26 × 10<superscript>7</superscript> DNA copies) to 2.0 fg (5.26 × 10<superscript>2</superscript> DNA copies). For the pUC57-Bc18S gene DNA the R<superscript>2</superscript> value was 0.976 for the concentration range 2.0 ng (4.21 × 10<superscript>8</superscript> DNA copies) to 2.0 fg (4.21 × 10<superscript>2</superscript> DNA copies). For the pUC57-Te18S gene DNA, the R<superscript>2</superscript> value was 0.952 (Fig. S3b) for the concentration range 2.0 ng (4.16 × 10<superscript>8</superscript> DNA copies) to 2.0 fg (4.16 × 10<superscript>2</superscript> DNA copies). Furthermore, a duplex qRPA analysis was developed and optimized and the results showed that primers and probes targeting for the bc48 gene of B. caballi and the 18S rRNA gene of T. equi is the best combination for a duplex qRPA analysis in one reaction. The developed duplex qRPA assay has good specificity, and had negative amplification for several similar parasite. For DNA extracted from real horse blood specimens, this qRPA method has comparable sensitivity to traditional qPCR, but a simpler and more rapid operating process to obtain positive amplification. The qRPA, including the duplex strategy described here, could allow fast identification of the EP-causing T. equi and B. caballi, showing great potential for on-site EP screening of horses. [ABSTRACT FROM AUTHOR]

Details

Language :
English
ISSN :
20452322
Volume :
10
Issue :
1
Database :
Complementary Index
Journal :
Scientific Reports
Publication Type :
Academic Journal
Accession number :
142084406
Full Text :
https://doi.org/10.1038/s41598-020-60997-1