Difference between revisions of "Part:BBa K3034005"

(The Mechanism of PtisAB)
 
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P<sub>tisAB</sub> is a promoter which can be induced by ciprofloxacin(CIP) through SOS response, and the promoter activity of it varies with different concentrations of CIP. This part is capable for starting to express subsequent genes once it sensed CIP.
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P<sub>tisAB</sub> sequence was derived from ''Escherichia coli K12 MG1655'' and has been codon optimized.(GenBank:AE000445.1, MG1655 complete genome 383127...385344)
  
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===Usage and Biology===
 
===Usage and Biology===
  
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====The Mechanism of P<sub>tisAB</sub>====
<span class='h3bb'>Sequence and Features</span>
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Ciprofloxacin can cause the SOS reaction of the bacteria, and the SOS reaction activates the RecA enzyme. When the RecA enzyme is activated, the LexA repressor will be cleared, whereby the promoter starts and expresses the downstream genes [1].
<partinfo>BBa_K3034005 SequenceAndFeatures</partinfo>
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[[File:T--UESTC-China--Module001加原理.png|800px|thumb|center|'''Fig. 1''' Schematic diagram of CIP-induced P<sub>tisAB</sub> principle]]
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As the schematic of the piGEM2019-01 shown above(Fig. 1), when P<sub>tisAB</sub> senses ciprofloxacin, subsequent genes will express, and one of them is GFP. By detecting the fluorescence intensity of GFP, the promoter activity of P<sub>tisAB</sub> can be reflected.
  
==Contribution ==
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====Detection of green fluorescence intensity &mdash; Methods====
*'''Group:''' [http://2019.igem.org/Team:UESTC-China iGEM Team UESTC-China 2019]
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*'''Author:''' Yubing Zhou, Jiayi Lu
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*'''Summary:''' PtisAB is a promoter which can be induced by ciprofloxacin(CIP) through SOS response, and the expression of it varies with different concentrations of CIP. This part is responsible for starting to express subsequent genes once it sensed CIP.
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===Characterization from iGEM19-UESTC-China===
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====The Mechanism of PtisAB====
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Ciprofloxacin can cause the SOS reaction of the bacteria, and the SOS reaction activates the RecA enzyme. When the RecA enzyme is activated, the lexA repressor is cleared, whereby the promoter starts to start and express the downstream gene.
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(缺图1)
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As the schematic of the piGEM2019-Module001 shown above(Fig.1), when pTisAB senses ciprofloxacin, subsequent genes will express, one of them is eGFP. By detecting the fluorescence intensity of eGFP, the expression of PtisAB can be reflected.
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====Detection of Green fluorescence intensity—Methods====
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Fixed strain:
 
Fixed strain:
The experimental group used CD072 of DH5α.
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The experimental group used ''E.coli'' DH5α carrying piGEM2019-01.
The control group used DH5α blank carrier bacteria.
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The control group used wild-type Ⅰ ''E.coli'' DH5α and wild-type Ⅱ ''E.coli'' DH5α.
  
1. A blank vector and a single clone of CD072 were taken from the crossed plates, and 5 ml of LB and 5 μl of ampicillin were added to a 12 ml BD tube, and shaken for 11 hours.
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1. A blank vector and a single clone of ''E.coli'' DH5α carrying piGEM2019-01 and wild-type ''E.coli'' DH5α were taken from the crossed plates, and 5 mL of LB and 5 μL of ampicillin were added to a 12 mL BD tube, and incubated for 11 hours.
  
2. Take 800μl from yesterday's bacteria and prepare a 15ml system  (100ml small conical flask), cultivate the bacteria to the logarithmic growth phase(1.5h).
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2. Take 800μL from yesterday's bacteria and prepare a 15mL system  (100mL small conical flask), cultivate the bacteria to the logarithmic growth phase(1.5h).
  
3. separately add CIP to prepare a system having a CIP concentration of 0, 0.1, 1, 6, 10 μg/ml.
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3. Separately add CIP to prepare a system having a CIP concentration of 0, 0.1, 1, 6, 10 mg/L.
  
4. Detect OD600 and green fluorescence after 0h, 2h,4h,6h by a multi-function microplate reader.
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4. Detect OD600 and green fluorescence after 0h, 2h, 4h, 6h by a multi-function microplate reader.
  
 
• OD600 detection method: in 96-well plate, 3 duplicate holes, minus LB blank.
 
• OD600 detection method: in 96-well plate, 3 duplicate holes, minus LB blank.
  
• Green fluorescence intensity detection method: At each time point, 1.5ml of bacterial liquid was taken in a light-proof tube,centrifuged at 12000rpm for 20 minutes, washed once with distilled water, and resuspended once. Add 96-well plate 200μl, excitation wavelength at 475nm, emission wavelength520nm.
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• Green fluorescence intensity detection method: At each time point, 1.5mL of bacterial liquid was taken in a light-proof tube, centrifuged at 12000rpm for 20 minutes, washed once with distilled water, and resuspended once. Add 96-well plate 200μL, excitation wavelength at 475nm, emission wavelength at 520nm.
  
====Detection of Green fluorescence intensity—Result ====
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====Detection of Green fluorescence intensity &mdash; Results ====
  
  [[File:T--UESTC-China--PtisAB.png|800px|thumb|center|'''Fig. 2''' Fluorescence in unit OD
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  [[File:T--UESTC-China--PtisABWT1.png|800px|thumb|center|'''Fig. 2''' Fold of Fluorescence Intensity per OD for control (P<sub>tisAB</sub>-, a) and ''E.coli'' DH5α carrying piGEM2019-01 (P<sub>tisAB</sub>+, b). When cells grow to exponential phase, they were exposed to 0 0.1 1 6 10 mg/L CIP in LB to induce the expression of P<sub>tisAB</sub>. Fold means GFP unit fluorescence after 2/4/6 h of exposure to CIP normalized to initial unit fluorescence. Unit fluorescence is fluorescence intensity per OD. This graph is a representative of two independent experiments with similar results; error bars indicate the standard error.]]
CD072(DH5α)carries piGEM2019-Module001, which obtain PtisAB, GFP, Qnrs and AmpR.  
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Control group(DH5α)carries a plasmid which only have AmpR.  
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Cells were exposed to 0 0.1 1 6 10ug/ml CIP in exponential phase.
 
Fold induction is GFP fluorescence after 2/4/6 h of exposure normalized to initial fluorescence.This graph is a representative of three independent experiments with similar results; error bars indicate the standard error.]]
 
  
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Compared ''E.coli'' DH5α carrying piGEM2019-01 with wild-type ''E.coli'' Ⅰ DH5α, we can see that the fluorescence intensity in ''E.coli'' DH5α carrying piGEM2019-01 is significantly stronger than wild-type Ⅰ ''E.coli'' DH5α.
  
Compared CD072 group with control group, we can see that the the fluorescence intensity in CD072 is significantly stronger than control group. And for CD072 group, we can see PtisAB responds differently to CIP at different concentrations, among them, 1ug/ml is the most appropriate response concentration for PtisAB.
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Next, we narrowed the range of CIP concentration and found the linear relationship between green fluorescence intensity and CIP concentration(Fig. 3). In this experiment, we chose wild-typeⅡ as the control (with an arabinose-inducible promoter), since arabinose-inducible promoter won’t be induced by CIP. No similar phenomenon was observed for the control group.
  
====References====
 
[1]Vogel J, Argaman L, Wagner EG, Altuvia S: The small RNA IstR inhibits synthesis of an SOS-induced toxic peptide. Current biology : CB 2004, 14(24):2271-2276.
 
  
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[[File:T--UESTC-China--PtisAB小范围改.png|800px|thumb|center|'''Fig. 3''' Fold of Fluorescence Intensity per OD for ''E.coli'' DH5α carrying piGEM2019-01 (P<sub>tisAB</sub>+) and control (P<sub>tisAB</sub>-). When cells grow to exponential phase,they were exposed to 0 0.2 0.4 0.6 1.0 mg/L CIP in LB to induce the expression of P<sub>tisAB</sub>. Fold means GFP unit fluorescence after 2h of exposure to CIP normalized to initial unit fluorescence. Unit fluorescence is fluorescence intensity per OD. This graph is a representative of three independent experiments with similar results; error bars indicate the standard error.]]
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====Conclusions====
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For ''E.coli'' DH5α carrying piGEM2019-01, we could see P<sub>tisAB</sub> responds differently to CIP at different concentrations, and comparison shows that 1 mg/L is the most appropriate response concentration for P<sub>tisAB</sub>.
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Besides, we could infer the concentration of ciprofloxacin from the green fluorescence intensity. At a concentration of 0 – 1 mg/L of ciprofloxacin, it followed the formula y = 0.3698x + 0.5477. R<sup>2</sup> = 0.9721 (y: the green fluorescence intensity; x: the ciprofloxacin concentration).
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====References====
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[1]Dörr, T., Vulić, M., & Lewis, K. (2010). Ciprofloxacin causes persister formation by inducing the TisB toxin in Escherichia coli. PLoS biology, 8(2), e1000317.
  
[2]Dörr T, Vulić M, Lewis K: Ciprofloxacin causes persister formation by inducing the TisB toxin in Escherichia coli. PLoS Biol 2010, 8(2):e1000317-e1000317.
 
  
  
  
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===Functional Parameters===
 
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<span class='h3bb'>Sequence and Features</span>
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<partinfo>BBa_K3034005 SequenceAndFeatures</partinfo>
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===Functional Parameters===
 
===Functional Parameters===
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<partinfo>BBa_K3034005 SequenceAndFeatures</partinfo>
 
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Latest revision as of 02:22, 22 October 2019

PtisAB

PtisAB is a promoter which can be induced by ciprofloxacin(CIP) through SOS response, and the promoter activity of it varies with different concentrations of CIP. This part is capable for starting to express subsequent genes once it sensed CIP.

PtisAB sequence was derived from Escherichia coli K12 MG1655 and has been codon optimized.(GenBank:AE000445.1, MG1655 complete genome 383127...385344)

Usage and Biology

The Mechanism of PtisAB

Ciprofloxacin can cause the SOS reaction of the bacteria, and the SOS reaction activates the RecA enzyme. When the RecA enzyme is activated, the LexA repressor will be cleared, whereby the promoter starts and expresses the downstream genes [1].

Fig. 1 Schematic diagram of CIP-induced PtisAB principle

As the schematic of the piGEM2019-01 shown above(Fig. 1), when PtisAB senses ciprofloxacin, subsequent genes will express, and one of them is GFP. By detecting the fluorescence intensity of GFP, the promoter activity of PtisAB can be reflected.

Detection of green fluorescence intensity — Methods

Fixed strain: The experimental group used E.coli DH5α carrying piGEM2019-01. The control group used wild-type Ⅰ E.coli DH5α and wild-type Ⅱ E.coli DH5α.

1. A blank vector and a single clone of E.coli DH5α carrying piGEM2019-01 and wild-type E.coli DH5α were taken from the crossed plates, and 5 mL of LB and 5 μL of ampicillin were added to a 12 mL BD tube, and incubated for 11 hours.

2. Take 800μL from yesterday's bacteria and prepare a 15mL system (100mL small conical flask), cultivate the bacteria to the logarithmic growth phase(1.5h).

3. Separately add CIP to prepare a system having a CIP concentration of 0, 0.1, 1, 6, 10 mg/L.

4. Detect OD600 and green fluorescence after 0h, 2h, 4h, 6h by a multi-function microplate reader.

• OD600 detection method: in 96-well plate, 3 duplicate holes, minus LB blank.

• Green fluorescence intensity detection method: At each time point, 1.5mL of bacterial liquid was taken in a light-proof tube, centrifuged at 12000rpm for 20 minutes, washed once with distilled water, and resuspended once. Add 96-well plate 200μL, excitation wavelength at 475nm, emission wavelength at 520nm.

Detection of Green fluorescence intensity — Results

Fig. 2 Fold of Fluorescence Intensity per OD for control (PtisAB-, a) and E.coli DH5α carrying piGEM2019-01 (PtisAB+, b). When cells grow to exponential phase, they were exposed to 0 0.1 1 6 10 mg/L CIP in LB to induce the expression of PtisAB. Fold means GFP unit fluorescence after 2/4/6 h of exposure to CIP normalized to initial unit fluorescence. Unit fluorescence is fluorescence intensity per OD. This graph is a representative of two independent experiments with similar results; error bars indicate the standard error.


Compared E.coli DH5α carrying piGEM2019-01 with wild-type E.coli Ⅰ DH5α, we can see that the fluorescence intensity in E.coli DH5α carrying piGEM2019-01 is significantly stronger than wild-type Ⅰ E.coli DH5α.

Next, we narrowed the range of CIP concentration and found the linear relationship between green fluorescence intensity and CIP concentration(Fig. 3). In this experiment, we chose wild-typeⅡ as the control (with an arabinose-inducible promoter), since arabinose-inducible promoter won’t be induced by CIP. No similar phenomenon was observed for the control group.


Fig. 3 Fold of Fluorescence Intensity per OD for E.coli DH5α carrying piGEM2019-01 (PtisAB+) and control (PtisAB-). When cells grow to exponential phase,they were exposed to 0 0.2 0.4 0.6 1.0 mg/L CIP in LB to induce the expression of PtisAB. Fold means GFP unit fluorescence after 2h of exposure to CIP normalized to initial unit fluorescence. Unit fluorescence is fluorescence intensity per OD. This graph is a representative of three independent experiments with similar results; error bars indicate the standard error.

Conclusions

For E.coli DH5α carrying piGEM2019-01, we could see PtisAB responds differently to CIP at different concentrations, and comparison shows that 1 mg/L is the most appropriate response concentration for PtisAB.

Besides, we could infer the concentration of ciprofloxacin from the green fluorescence intensity. At a concentration of 0 – 1 mg/L of ciprofloxacin, it followed the formula y = 0.3698x + 0.5477. R2 = 0.9721 (y: the green fluorescence intensity; x: the ciprofloxacin concentration).

References

[1]Dörr, T., Vulić, M., & Lewis, K. (2010). Ciprofloxacin causes persister formation by inducing the TisB toxin in Escherichia coli. PLoS biology, 8(2), e1000317.



Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    COMPATIBLE WITH RFC[12]
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]