A new multiplex PCR protocol to detect mixed trypanosomatid infections in species of Apis and Bombus

被引:25
作者
Bartolome, Carolina [1 ,2 ]
Buendia, Maria [3 ]
Benito, Maria [3 ]
De la Rua, Pilar [4 ]
Ornosa, Concepcion [5 ]
Martin-Hernandez, Raquel [3 ,6 ]
Higes, Mariano [3 ]
Maside, Xulio [1 ,2 ,7 ]
机构
[1] Univ Santiago de Compostela, Grp Med Xenom, CIMUS, Santiago De Compostela 15782, Galicia, Spain
[2] IDIS, Grp Xenom Comparada Pararsitos Humanos, Santiago De Compostela, Galicia, Spain
[3] JCCM, Lab Patol Apicola, Ctr Invest Apicola & Agroambiental, Inst Reg Invest & Desarrollo Agroalimentario & Fo, Guadalajara 19180, Spain
[4] Univ Murcia, Dept Zool & Antropol Fis, Fac Vet, E-30100 Murcia, Spain
[5] Univ Complutense, Dept Biodiversidad Ecol & Evoluc, Fac Ciencias Biol, E-28040 Madrid, Spain
[6] Fdn Parque Cient Tecnol Albacete, Inst Recursos Humanos Ciencia & Tecnol, Albacete, Spain
[7] Univ Santiago de Compostela, Dept CC Forenses Anaemia Patolox Xinecol & Obstet, Santiago De Compostela 15782, Galicia, Spain
关键词
Crithidia mellificae; Crithidia bombi; Loimaria passim; Apis mellifera; Bombus terrestris; Multiplex PCR; PARASITES LOTMARIA-PASSIM; CRITHIDIA-BOMBI; BEE PATHOGENS; POLLINATORS; BUMBLEBEES; TRANSMISSION; DIAGNOSTICS; TERRESTRIS; PHYLOGENY; PATTERNS;
D O I
10.1016/j.jip.2018.03.015
中图分类号
Q95 [动物学];
学科分类号
071002 ;
摘要
Trypanosomatids are highly prevalent pathogens of Hymenoptera; however, most molecular methods used to detect them in Apis and Bombus spp. do not allow the identification of the infecting species, which then becomes expensive and time consuming. To overcome this drawback, we developed a multiplex PCR protocol to readily identify in a single reaction the main trypanosomatids present in these hymenopterans (Lotmaria passim, Crithidia mellificae and Crithidia bombi), which will facilitate the study of their epidemiology and transmission dynamics. A battery of primers, designed to simultaneously amplify fragments of the RNA polymerase II large subunit (RPB1) of L. passim, the glyceraldehyde-3-phosphate dehydrogenase (GAPDH) of C. mellificae and the DNA topoisomerase II (TOPII) of C. bombi, was tested for target specificity under single and mixed template conditions using DNA extracted from cell cultures (L. passim ATCC PRA403; C. mellificae ATCC 30254) and from a bumblebee specimen infected with C. bombi only (14349). Once validated, the performance of the method was assessed using DNA extractions from seven Apis mellifera (Linnaeus, 1758) and five Bombus terrestris (Linnaeus, 1758) field samples infected with trypanosomatids whose identity had been previously determined by PCR-cloning and sequencing (P-C-S). The new method confirmed the results obtained by P-C-S: two of the honeybee samples were parasitized by L. passim, C. mellificae and C. bombi at the same time, whereas the other five were infected with L. passim only. The method confirmed the simultaneous presence of L. passim and C. mellificae in two B. terrestris, where these parasites had not previously been reported.
引用
收藏
页码:37 / 41
页数:5
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