Part:BBa_K2447000

Extracellular phosphate sensor with GFP reporter

PhoB and PhoR proteins are part of the Pho regulon inherent in E.coli. When low concentration of extracellular phosphate ions is present, PhoR can phosphorylate PhoB to form active phosphorylated-PhoB. PhoB promoter is activated as a result of active binding of phosphorylated-PhoB, resulting in downstream expression of GFP. When high concentration of extracellular phosphate ions is present, PhoR will dephosphorylate phosphorylated-PhoB, and therefore inactivating it, and repressing PhoB promoter for downstream expression of GFP.

Improvement over previous iGEM part BBa_K116404 (NYMU Taipei 2008)

The two parts (Bba_K2447000 & BBa_K116404) listed below are inserted into pBbE2k backbones and subsequently characterised in E.coli MG1656. These cells are grown in MOPS medium (a minimal nutrient medium) and varying concentrations of phosphate ions from 0 to 1000 uM are added.

By replacing the weaker RBS 32 (as utilised by the Taiwanese team) with a stronger binding affinity RBS 34 as proposed by iGEM NUS team 2017, we have elucidated much stronger GFP expression and also improved the sensitivity of the part to varying concentrations of phosphate ions. Previously, the Taiwanese part [http://2008.igem.org/Team:NYMU-Taipei/Project/Phosphate had reported]much lower levels of GFP productions for all phosphate concentrations. Our improved construct had yielded on average 40 fold increase (Figure 2) in GFP expression when compared to the original construct. In addition, our proposed phosphate sensor is more sensitive (Figure 3) at higher levels of phosphate concentrations, and able to yield different levels of repressed GFP productions. On the other hand, the Taiwanese construct remains not sensitive to high amount of phosphate concentrations, yielding similar level of repressed GFP productions (Figure 4) when the phosphate concentrations is above 50 uM.

Sequence and Features