TABLE 4.
pM and pVP16 (BD Biosciences, Palo Alto, CA) clones
In frame cloning of sequences into pM and VP16 generate fusion proteins of the GAL4-DNA binding domain and the viral protein 16 (VP16) activation domain, respectively. These plasmids were used in combinations to access interaction of proteins in mammalian cells. The multiple cloning sites of the plasmids are identical, therefore cloned sequences are interchangeable. The luciferase reporter employed in the mammalian 2-hybrid assays was pFR-Luc (Stratagene, La Jolla, CA).
| Name | Primers | Amino Acids |
Restriction Sites |
|---|---|---|---|
| CAR1 | FP: GATCGAATTCGTCATGGCCAGTAGGGAAGATGAG | 1–348 | EcoR1/Xba1 |
| RP: BGH | |||
| CAR1-LBD | FP: GATCGAATTCGCCACCATGGTACTGTCGGCAGAAGCCC | 80–348 | EcoR1/Xba1 |
| RP: BGH | |||
| CAR3- | FP: GATCGAATTCGTCATGGCCAGTAGGGAAGATGAG | 1–352 | EcoR1/Xba1 |
| RP: BGH | |||
| CAR1-LBD | FP: GATCGAATTCGCCACCATGGTACTGTCGGCAGAAGCCC | 80–352 | EcoR1/Xba1 |
| RP: BGH | |||
| SRC-1 RID | FP: GATCGAATTCCCTAGCAGATTAAATATACAACCAG | 570–780 | EcoR1/Xba1 |
| RP: GATCTCTAGATCACATCTGTTCTTTCTTTTCCACTT | |||
| RXRα | FP: GATCGAATTCGCCGCCATGGACACCAAACATTTCCTG | 1–462 | EcoR1/Xba1 |
| RP: GATCTCTAGACTAAGTCATTT GGTGCGGCGC | |||
| RXRα-LBD | FP: GGAATTCGCCGCCATGGGCATGAAGCGGGAAG | 198–462 | EcoR1/Xba1 |
| RP: GATCTCTAGACTAAGTCATTT GGTGCGGCGC |
FP, forward primer; RP, reverse primer.