Table 1.
Sequences of primers set used for detection of hemoparasites DNAs
| Pathogen | Assays | Oligonucleotide sequences (5' > 3') | Product size (bp) | Reference |
|---|---|---|---|---|
| Target gene | ||||
| B. bovis SBP-4 | PCR | AGTTGTTGGAGGAGGCTAAT | 907 | [21] |
| TCCTTCTCGGCGTCCTTTTC | ||||
| nPCR | GAAATCCCTGTTCCAGAG | 503 | ||
| TCGTTGATAACACTGCAA | ||||
| B. bigemina RAP-1a | PCR | GAGTCTGCCAAATCCTTAC | 879 | |
| TCCTCTACAGCTGCTTCG | ||||
| nPCR | AGCTTGCTTTCACAACTCGCC | 412 | ||
| TTGGTGCTTTGACCGACGACAT | ||||
| semi nPCR | GAGTCTGCCAAATCCTTAC | 690 | ||
| TTGGTGCTTTGACCGACGACAT | ||||
| Theileria spp. 18S rRNA | PCR | GAAACGGCTACCACATCT | 778 | [20] |
| AGTTTCCCCGTGTTGAGT | ||||
| nPCR | TTAAACCTCTTCCAGAGT | 581 | ||
| TCAGCCTTGCGACCATAC | ||||
| T. parva p 104 | PCR | ATTTAAGGAACCTGACGTGACTGC | 496 | [23] |
| TAAGATGCCGACTATTAATGACACC | ||||
| nPCR | GGCCAAGGTCTCCTTCAGATTACG | 277 | ||
| TGGGTGTGTTTCCTCGTCATCTGC | ||||
| T. orientalis MPSP | PCR | CTTTGCCTAGGATACTTCCT | 776 | [24] |
| ACGGCAAGTGGTGAGAACT | ||||
| A. marginale Msp5 | PCR | GTGTTCCTGGGGTACTCCTATGTGAACAAG | 547 | [22] |
| AAGCATGTGACCGCTGACAAACTTAAACAG | ||||
| nPCR | AAGCACATGTTGGTAATATTCGGCTTCTCA | 195 | ||
| AATTCTCGCATCAAAAGACTTGTGGTACTC |
Note: The primers sets forSBP-4, 18S rRNA, p104 and MPSP genes were used for detection of corresponding pathogens and the products of the last amplification served as template for genetic characterisation. With regard to BbigRAP-1a and Msp5, PCR and nPCR primers were used in pathogen detection, however for genetic characterization, amplicons from a semi-nPCR (BbigRAP-1) and from the first PCR (Msp5) were used