This selleck chemical product was
purified and used as template for a second PCR with the oligonucleotides Mal-C2Kpn and Ttrack2-U; the amplification product was named T2-U. A third PCR amplification product obtained with the primers RBS-C and Ttrack1-L, and pH3 DNA as the template, was purified and used as a template in a new PCR reaction with the primers RBS-C and Ttrack2-L. The amplification product was named T2-L. Finally, PCR products T2-U and T2-L were then mixed and used as the template for the last PCR. In this reaction, the www.selleckchem.com/products/azd1390.html primers Mal-C2Kpn and RBS-C were used, and the final PCR product was cloned into pDOP. Construction of repC hybrid genes Overlap extension PCR was also employed to obtain repC hybrid genes. RepC gene amplification products from pSymA were obtained using pDOP-CsA as the template, and the repC p42d products were obtained using pH3 as the template. Most of the hybrid genes described here required the overlap of two PCR products. The insert of plasmid
pDOP/C420-1209 was obtained using the primers C-SymA and AL-2Uc for the first PCR product and AL-2U and Mal-C2 for the second BLZ945 product. The final PCR product was obtained with the external primers C-SymA and Mal-C2. The insert of plasmid pDOP/C1-420 was constructed with primers RBS-C and 1L-B2c and the primers 1L-B2 and K-SymAL for the first and second PCR products, respectively. These products were combined using the primers RBS-C and K-SymAL. The pDOP/C841-1209 insert was constructed with the primers C-SymA and BL-3Uc for the first PCR product and BL-3U and Mal-C2 for the second. These products were joined in a third PCR with the primers C-SymA and Mal-C2. The hybrid gene in pDOP/C1-990 was acquired with the primers RBS-C and Sal-CdL for the first PCR product and Sal-CdU and Mal-C2 for the second. These PCR products were integrated in a third PCR with the primers RBS-C and
Mal-C2. Similarly, the hybrid gene of pDOP/C1-990 was obtained with the primers RBS-C and Cd-1086 for the first amplification product. To obtain the second PCR product, the primers Cs-1087U and Mal-C2 were used, and both PCR products were fused with the primers RBS-C and Mal-C2. The inserts of two of the constructs, pDOP/C421-840 and pDOP/Cs421-840, required the fusion RANTES of three PCR products. The hybrid gene located in pDOP/C421-840 required the primers C-SymA and AL-2Uc for the first PCR product, the primers AL-2U and AL-2Uc for the second PCR product, and the primers 2L-CU and K-SymA for the third PCR product. The three PCR products were fused in the final PCR with the primers C-SymA and K-SymA. The hybrid gene present in pDOP/Cs421-840 was obtained using the primers RBS-C and 1L-B2c for the first PCR product, the primers 1L-B2 and B2-3Uc for the second PCR product, and the primers BL-2U and Mal-C2 for the third PCR product. These PCR products were linked using the primers RBS-C and Mal-C2 in the final PCR.