Table 1.
Modification of tandem transcription activator-like effector intermediate vectors
| Vector | Backbone | Insert type | Subcloning enzymes | Sequence of short oligos or PCR primers |
|---|---|---|---|---|
| pFusX1* | pFus_A30A | N/A | N/A | N/A |
| pFusX2 | pFus_A30B | Short oligos | AgeI/AatII | pFusX2-S: |
| CCGGTGGTCTCTGGCGGCAAGCAAGCGCTCGAAACGGTGCAGCGGCTGTTGCCGGTGCTGTGCCAGGACCATGGCGAGACGT | ||||
| pFusX2-AS: CTCGCCATGGTCCTGGCACAGCACCGGCAACAGCCGCTGCACCGTTTCGAGCGCTTGCTTGCCGCCAGAGACCA | ||||
| pFusX3 | pFus_A30B | PCR | AflII/AatII | pFusX3-F: ATTCTTAAGCGTCTCCATGGCCTGACCCCG |
| pFusX3-R: ATTGACGTCTCGCAGGCCATGGTCCTGG | ||||
| pFusX4 | pFus_A30B | PCR | AflII/AatII | pFusX4-F: GTTCTTAAGCGTCTCCCCTGACCCCG |
| pFusX4-R: GTTGACGTCTCGGCCATGGTCCTGG |
Shown are restriction enzymes and sequences of short oligos or primers used in modification of pFus_A30B into pFusX2, pFusX3, and pFusX4. For pFusX2, annealed reverse complementary short oligos are used directly as the insert. For pFusX3 and pFusX4, PCR products from primers with pFus_A30B as template are used as inserts. No modification is needed for pFusX1, which is identical to pFus_A30B.
N/A, not applicable.