Table 1.
Oligonucleotide primer sequences, PCR conditions and restriction enzymes used for genotyping and sequencing of the three polymorphisms.
| Gene | Polymorphism | Primers | PCR pr. length (bp) | Annealing temp (°C) | Restriction enzyme |
|---|---|---|---|---|---|
| TLR2 | Arg753Gln | F: 5′-GAGTGGTGCAAGTATGAACTGGA-3′ | 260 | 62 | Pst I |
| R: 5′-TCCCAACTAGACAAAGACTGGTCT-3′ | |||||
| TLR4 | Asp299Gly | F: 5′-GATTAGCATACTTAGACTACTACCTCCATG-3′ | 263 | 56 | Nco I |
| R: 5′-GATCAACTTCTGAAAAAGCATTCCCAC-3′ | |||||
| TLR4 | Thr399Ile | F: 5′-TGGCAACATTTAGAATTAGTTAAC-3′ | 227 | 52 | Msp I |
| R: 5′-CTCAGATCTAAATACTTTAGGCCG-3′ |
The underlined bases in the primers differ from the original sequences and served to introduce a restriction site or to disrupt a natural restriction site within the primer sequence.