Team:Uppsala University/Backbones/Details
From 2012.igem.org
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The copy number of the pSB4x15 series, especially the pSB4C15, has been estimated by three methods all pointing to it being maintained at a consistent low copy number in E coli cells.
Flow cytometry Quadruplicates (for +IPTG) or triplicates (-IPTG) of E coli MG1655 strains carrying pSB3C5-red, pSB4C5-red, pSB4C15-red, and a DH5alpha strain carrying pSB1C3 with a non-coding construct, were inoculated in 2 mL LB media with chloramphenicol (12 µg/mL) and with or without IPTG (0.5 mM). Cultures were grown shaking at 37° C for 15 hours (+IPTG) or 19 hours (-IPTG), and were visibly confirmed to have grown at steady state for at least 4 hours. Samples were equilibrated in PBS solution at 1:160 dilution for 2 hours, and then measured in a BD Biosciences FACSaria III. 10^5 cells of each sample were individually measured and averaged, with dead and other non-flourescent cells excluded.
Results indicate that that the pSB4C5 has similar or higher copy number than the low to medium copy number plasmid pSB3C5. The pSB4C15 strain shows a lower fluorescence by more than an order of magnitude. In the +IPTG experiment, it expresses less than 1/20 of the flourescence of the other strains, and even is lower without induction.
Plasmid yields
Significantly higher plasmid yields were observed in pSB3C5 and pSB4C5 than in pSB4C15, suggesting a higher copy number. The variance in yield is however large.
Color development Figure 3: Color assesment plates grown for two days. In clockwise order: A. Three clones each of pSB4C15-red and pSB4C5-red. Grown at 37° C. B. Two clones each of pSB4C15-red, pSB8C15-red and pSB4C5-red. Grown at 30° C. Strong RFP expression was observed in pSB4C5-red strains, weak color in pSB8C15-red strains and no color in pSB4C15-red strains. This points to higher plasmid copy number in pSB4C5 than of the other plasmids. The native lacI system of MG1655 likely repressed the lacI promoter well, inhibiting color development.
Conclusion The results also show that pSB4C5 has a significantly higer copy number than specified, of the same magnitude as pSB3C5. We are confident to conclude that the copy number regulation of pSB4C5 is broken. This conclusion can also be expanded to the other pSB4x5 backbones, since they an identical origin of replication. Casual observations also support this result. Thus, we recommend replacing the pSB4x5 series with the pSB4x15 for all low copy applications | ||||||||||||||||||||||||||||||||||||||
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IPTG induction Cassettes of the Plac, PLlacO (BBa_R0011) and PT5lac (BBa_K592008) promoters and the pUCori-Plac were assembled with RFP in the pSB4C15Iq backbone, and transformed into E coli DH5alpha. Single clones of these were inoculated in 2 mL LB media with chloramphenicol (12 µg/mL) and with or without IPTG (0.5 mM). Cultures were grown shaking at 37° C for 18 hours, and were visibly confirmed to have grown at steady state for at least 4 hours. Samples were equilibrated in PBS solution at 1:160 dilution for 1 hour, and then measured in a BD Biosciences FACSaria III . 10^5 cells of each sample were individually measured and averaged, with dead and other non-flourescent cells excluded. Since the purpose of the experiment was to investigate overall repression functionality and the possibility of induction, the samples of with Plac, PT5lac and PLlacO can be considered a triplicate measurement.
Conclusions Induction at different IPTG levels
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