Part:BBa_K422015

pSEVA132

Victor de Lorenzo's lab, Ampicillin resistance, pBBR1 ori

Plasmid features

• Ampicillin resistance
• pBBR1 origin of replication

Characterization

Figure 1: Plasmid copy number estimation of pEVA 132 compared to a high copy plasmid pUC19.

As pBBR1 is not a widely known origin of replication, the plasmid copy number was determined in relation to a commonly used high-copy vector pUC19. The experimental procedure included normalization of cell number via optical density measurement followed by plasmid concentration measurements (using a commercial Miniprep kit). The results are represented in figure 1.

Design features

Compatible with the cloning strategy BBF RFC28.

The genes for the repressor protein AraC and the corresponding ParaBAD promotor/operator sites were introduced into the vector pSEVA 132 followed by an insert, which is flanked by AarI-recognition sites. Digest with AarI releases this insert and generates a vector with assembly-compatible overhangs.

Sequence and Features