Table 1.
Primers and Restriction Enzymes Used
| Exon/Intron | Mutations/Polymorphisms | Enzyme | Primer Pair |
|---|---|---|---|
| Exon 4A | 735C→T | MspI | 4AF: 5′-AGCCGCCAGAGAAGCCACCAG-3′ |
| 4AR: 5′-GGAACGTCAGAAGCAGCAGGAGTC-3′ | |||
| Exon 9 | G272V | Hinf I | 9F: 5′-GCCCAGGGCCTTTTCTGACC-3′ |
| 9R: 5′-CACTCTCACTTCCCGCCTC-3′ | |||
| Intron 9 | −177C→T* | Hinf I | 10F: 5′-AGCCCTCTATCCCTTCAG-3′ |
| 10RM: 5′-GCATGGGACGTGTGAAGGTAC-3′ | |||
| −58G→A* | TaqI | ModF: 5′-TCATCGAAAGTGGAGGCGTCCTTTC-3′ | |
| ModR: 5′-GGCTACATTCACCCAGAGGTCGC-3′ | |||
| Intron 10 | 10F: 5′-AGCCCTCTATCCCTTCAG-3′ | ||
| 10R: 5′-GGCTACATTCACCCAGAGGT-3′ | |||
| Intron 12 | 12F: 5′-GCACAGAACCACAGAAGATGATGGCA-3′ | ||
| 12R: 5′-AGCATCCAACCCACCCTACCC-3′ | |||
| Intron 13 | G389R | NciI | 13F: 5′-GTCCCTCCCTTCCTCTTCTTG-3′ |
| R406W | NcoI | 13R: 5′-GAGTGACAAAAGCAGGTTAAGTGAT-3′ |
*
New sequence variations described in the present study (see “Results” and Table 3).