Table 1.
Primers used for pathogen detection and tick genomic DNA amplificationa
| Pathogen | Region amplified | Primer Forward (5’-3’) | Primer Reverse (5’-3’) | Final [primer] (μM) | PCR Product (bp) | Reference |
|---|---|---|---|---|---|---|
| Hepatozoon felis | 18S rRNA | CTTACCGTGGCAGTGACGGT | TGTTATTTCTTGTCACTACCTCTCTTATGC | 0.3 | 146 | [11] |
| Ehrlichia/ Anaplasma spp. | 16S rRNA | GCAAGCYTAACACATGCAAGTCG | CTACTAGGTAGATTCCTAYGCATTACTCACC | 0.5 | 102b | [11] |
| Piroplasmid | 18S rRNA | GACGATCAGATACCGTCGTAGTCC | CAGAACCCAAAGACTTTGATTTCTCTC | 0.3 | 114b | VetGenomic In-house design |
| Rickettsia spp. | ITS1 | GCTCGATTGRTTTACTTTGCTGTGAG | CATGCTATAACCACCAAGCTAGCAATAC | 0.5/0.3 | 300b | [11] |
| Bartonella spp. | ITS1 | AGATGATGATCCCAAGCCTTCTG | CCTCCGACCTCACGCTTATCA | 0.3 | 180b | Modified from [12] and [13] |
| Hemotropic Mycoplasma spp. | 16S | GGAATCACTAGTAATCCYGTGTCAGCTATAT | GGCGGTGTGTACAAGCCTGG | 0.3 | 187b | [14] |
aThe eukaryotic 18S RNA Pre-Developed TaqMan Assay Reagents (AB, Life technologies) was used as an internal reference for genomic DNA amplification to ensure the proper PCR amplification of each sample. bTargeted size could vary depending on the species