Development of a multiplex PCR assay for simultaneous detection of Theileria annulata, Babesia bovis and Anaplasma marginale in cattle

被引:88
|
作者
Bilgic, Huseyin B. [1 ]
Karagenc, Tulin [1 ]
Simuunza, Martin [3 ]
Shiels, Brian [2 ]
Tait, Andy [2 ]
Eren, Hasan [1 ]
Weir, William [2 ]
机构
[1] Adnan Menderes Univ, Dept Parasitol, Fac Vet Med, TR-09016 Isikli Mevki, Aydin, Turkey
[2] Univ Glasgow, Inst Infect Immun & Inflammat, Glasgow G61 1QH, Lanark, Scotland
[3] Univ Zambia, Sch Vet Med, Dept Dis Control, Lusaka 32379, Zambia
基金
英国惠康基金;
关键词
Theileria annulata; Anaplasma marginale; Babesia bovis; PCR; Multiplex PCR; POLYMERASE-CHAIN-REACTION; LINE BLOT HYBRIDIZATION; VES MULTIGENE FAMILY; REAL-TIME PCR; ANTIGENIC VARIATION; INFECTED ERYTHROCYTES; ENDEMIC AREA; DNA; SURFACE; GENOME;
D O I
10.1016/j.exppara.2012.11.005
中图分类号
R38 [医学寄生虫学]; Q [生物科学];
学科分类号
07 ; 0710 ; 09 ; 100103 ;
摘要
Tropical theileriosis, bovine babesiosis and anaplasmosis are tick-borne protozoan diseases that impose serious constraints on the health and productivity of domestic cattle in tropical and sub-tropical regions of the world. A common feature of these diseases is that, following recovery from primary infection, animals become persistent carriers of the pathogen and continue to play a critical role in disease epidemiology, acting as reservoirs of infection. This study describes development and evaluation of multiplex and single PCR assays for simultaneous detection of Theileria annulata, Babesia bovis and Anaplasma marginate in cattle. Following in silico screening for candidate target genes representing each of the pathogens, an optimised multiplex PCR assay was established using three primer sets, cytob1, MAR1bB2 and bovar2A, for amplification of genomic DNA of T. annulata, A. marginate and B. bovis respectively. The designed primer sets were found to be species-specific, generating amplicons of 312, 265 and 166 base pairs, respectively and were deemed suitable for the development of a multiplex assay. The sensitivity of each primer pair was evaluated using serial dilutions of parasite DNA, while specificity was confirmed by testing for amplification from DNA of different stocks of each pathogen and other Theileria, Babesia and Anaplasma species. Additionally, DNA preparations derived from field samples were used to evaluate the utility of the single and multiplex PCRs for determination of infection status. The multiplex PCR was found to detect each pathogen species with the same level of sensitivity, irrespective of whether its DNA was amplified in isolation or together with DNA representing the other pathogens. Moreover, single and multiplex PCRs were able to detect each species with equal sensitivity in serially diluted DNA representing mixtures of T. annulata, B. bovis and A. marginate, and no evidence of non-specific amplification from non-target species was observed. Validation that the multiplex PCR efficiently detects single and mixed infections from field samples was demonstrated. The developed assay represents a simple and efficient diagnostic for co-detection of tropical theileriosis, bovine babesiosis and anaplasmosis, and may be a valuable tool for epidemiological studies aimed at assessing the burden of multiple infection with tick-borne pathogens and improving control of the associated diseases in endemic regions. (C) 2012 Elsevier Inc. All rights reserved.
引用
收藏
页码:222 / 229
页数:8
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