Table 1. Pairs of primers used in qRT-PCR analysis.
| Gene | Forward Primer (5′- > 3′) | Reverse Primer (5′- > 3′) | Product Length (base pairs) |
|---|---|---|---|
| ATP6V0D2 | TTCTTGAGTTTGAGGCCGAC | CAGCTTGAGCTAACAACCGC | 144 |
| CTSK | ATATGTGGGCCAGGATGAAAGTT | TCGTTCCCCACAGGAATCTCT | 90 |
| CD47 | CGATGCCATGGTGGGAAACT | TCAGTGTTGAAGGCCGTGC | 99 |
| CD9 | GCTGGGATTGTTCTTCGGGT | GCTTTGAGTGTTTCCCGCTG | 171 |
| DC-STAMP | AAGCGGAACTTAGACACAGGG | CAGCTAGGGCTTCGTGGAAA | 101 |
| GADPH | GCCTTCCGTGTTCCTACC | AGAGTGGGAGTTGCTGTTG | 183 |
| MCP-1 | AGCCAACTCTCACTGAAGCC | GCGTTAACTGCATCTGGCTG | 131 |
| MMP-9 | CGACTTTTGTGGTCTTCCCC | TAGCGGTACAAGTATGCCTCTG | 83 |
| OPG | GTGGAATAGATGTCACCCTGTGT | TTTGGTCCCAGGCAAACTGT | 110 |
| RANKL | CCCATCGGGTTCCCATAAAGT | AGCAAATGTTGGCGTACAGG | 114 |
| TRAcP5b | CGACCATTGTTAGCCACATACG | TCGTCCTGAAGATACTGCAGGTT | 77 |
| Y1R | CTCGCTGGTTCTCATCGCTGTGGAACGG | GCGAATGTATATCTTGAAGTAG | 325 |
All primers used were located on two different exons to ensure that only properly spliced mRNA and not genomic DNA contaminants was amplified.