Difference between revisions of "Part:BBa K1682015"
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[[File:Team HKUST-Rice 2015 Phosmech pr.PNG|thumb|500px|center|<b>Fig.1 </b>Phosphate sensing mechanism of P<sub>phoBR</sub>.]] | [[File:Team HKUST-Rice 2015 Phosmech pr.PNG|thumb|500px|center|<b>Fig.1 </b>Phosphate sensing mechanism of P<sub>phoBR</sub>.]] | ||
− | + | <i>E. coli</i> has multiple native phosphorus sensing and regulation systems that we could use in the construct. Among them, we chose the PhoR/PhoB two-component system (TCS). It contains a sensory histidine kinase PhoR and a partner DNA-binding response regulator PhoB. PhoR is activated under low phosphate concentration, which will then phosphorylate PhoB. The phospho-PhoB is then capable of activating expression of the Pho regulon genes, one of the examples is <i>phoA</i>. In high phosphate concentration, <i>phoR</i> is turned into an inhibitory state, which interferes with phosphorylation of PhoB. PhoB is, thus, not capable of activating expression of <i>phoA</i>. | |
==Constructs for characterization== | ==Constructs for characterization== | ||
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===RFU measurement=== | ===RFU measurement=== | ||
[[File:Team HKUST-Rice 2015 Phobrrrr.PNG|thumb|500px|center|<b>Fig.3 </b>Activity of <i>P<sub>phoBR</sub></i> in <i>E. coli</i> DH10B in different phosphate concentrations]] | [[File:Team HKUST-Rice 2015 Phobrrrr.PNG|thumb|500px|center|<b>Fig.3 </b>Activity of <i>P<sub>phoBR</sub></i> in <i>E. coli</i> DH10B in different phosphate concentrations]] | ||
− | As shown in Figure 3, <i>P<sub>phoBR</sub></i> is induced under phosphate limitation and repressed under high phosphate concentration. The fluorescence intensity dropped by 2.99 folds between 0 to | + | As shown in Figure 3, <i>P<sub>phoBR</sub></i> is induced under phosphate limitation and repressed under high phosphate concentration. The fluorescence intensity dropped by 2.99 folds between 0 to 300 μM concentration of phosphate. Furthermore, a plateau is observed starting from the 200 μM phosphate concentration point, suggesting that the dynamic range of <i>P<sub>phoBR</sub></i> is from 0-200 μM of phosphate. |
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Revision as of 02:51, 19 September 2015
Contents
PphoBR - I13504 - phosphate responsive promoter with GFP generator
Biology of PphoBR
E. coli has multiple native phosphorus sensing and regulation systems that we could use in the construct. Among them, we chose the PhoR/PhoB two-component system (TCS). It contains a sensory histidine kinase PhoR and a partner DNA-binding response regulator PhoB. PhoR is activated under low phosphate concentration, which will then phosphorylate PhoB. The phospho-PhoB is then capable of activating expression of the Pho regulon genes, one of the examples is phoA. In high phosphate concentration, phoR is turned into an inhibitory state, which interferes with phosphorylation of PhoB. PhoB is, thus, not capable of activating expression of phoA.
Constructs for characterization
With the phosphate (pho) regulon from E. coli, it can be utilized for detecting phosphate level. To make a phospahte-sensing device, we obtained the promoter, PphoBR, and combined it with a GFP reporter, BBa_E0240, in BioBrick RFC10 standard so that the promoter activity in different phosphate level can be detected and characterized.
RFU measurement
As shown in Figure 3, PphoBR is induced under phosphate limitation and repressed under high phosphate concentration. The fluorescence intensity dropped by 2.99 folds between 0 to 300 μM concentration of phosphate. Furthermore, a plateau is observed starting from the 200 μM phosphate concentration point, suggesting that the dynamic range of PphoBR is from 0-200 μM of phosphate.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12COMPATIBLE WITH RFC[12]
- 21COMPATIBLE WITH RFC[21]
- 23COMPATIBLE WITH RFC[23]
- 25COMPATIBLE WITH RFC[25]
- 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI.rc site found at 755