Part:BBa_K615000:Design

E. coli strain for His3-URA3 one-hybrid selection system

Design Notes

This selection strain was adapted from the one-hybrid system presented by Meng et al (2005), but instead of having the zinc finger binding site and associated genes on a plasmid, we placed the selection construct directly onto the genome, thus ensuring that the system will not be lost in subsequent generations and that each cell has exactly one copy.

Genotype:

• HisB KO: 6 nucleotides (694-699) coding for amino acids V and E were deleted using MAGE.
• PyrF KO: Two early in-frame stop codons were made using MAGE to substitute 8T-->A and 16C-->G
• rpoZ KO: Lambda red was used to replace gene with Zeocin resistance cassette.
• Kanamycin resistance cassette—Zif268 binding site and weak promoter—His3—URA3: inserted into 1529620 genomic locus using lambda red.
• MutS KO: replaced by chloramphenicol resistance cassette.

For verification of the genotype, please see the 2011 Harvard iGEM team's [http://2011.igem.org/Team:Harvard/Results/MAGE MAGE results] and [http://2011.igem.org/Team:Harvard/Results/Lambda_Red Lambda Red results]

Source

• Selection system was adapted from Meng et al (2005).
• Base strain was EcNR2, a modified E. coli strain as described in Wang et al (2009).
• URA3 and His3 genes were synthesized.

References

Harris H. Wang, Farren J. Isaacs, Peter A. Carr, Zachary Z. Sun, George Xu, Craig R. Forest, George M. Church. Programming cells by multiplex genome engineering and accelerated evolution. (2009). Nature, 460(7257):894-8.

Xiangdong Meng, Michael H Brodsky, Scot A Wolfe. A bacterial one-hybrid system for determining the DNA-binding specificity of transcription factors. (2005). Nature Biotechnology, 23(8): 988-994.