Difference between revisions of "Part:BBa K1847009"

 
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<partinfo>BBa_K1847009 SequenceAndFeatures</partinfo>
 
<partinfo>BBa_K1847009 SequenceAndFeatures</partinfo>
 
<h1>Usage and Biology</h1>
 
<h1>Usage and Biology</h1>
[[File:Activation_repression_lldR.png|thumb|right|Theoretical model for the dual function as repressor and activator of LldR.]]
+
[[File:Activation_repression_lldR.png|thumb|right|Figure 1. Theoretical model for the dual function as repressor and activator of LldR.]]
 
<p>The natural promoter of LldR ([[Part:BBa_K822000]]) consists of two operators (O1 and O2) and a promoter which is intercalated between the operators. It regulates the expression of the <i>lldPRD</i> operon, and it is involved in L-lactate metabolism. This promoter is repressed by a dimer of LldR, possibly by forming a DNA loop that does not allow the RNA polymerase to bind to the promoter. LldR can also have a function as an activator [1]. The repression of the promoter can be removed by lactate.</p>  
 
<p>The natural promoter of LldR ([[Part:BBa_K822000]]) consists of two operators (O1 and O2) and a promoter which is intercalated between the operators. It regulates the expression of the <i>lldPRD</i> operon, and it is involved in L-lactate metabolism. This promoter is repressed by a dimer of LldR, possibly by forming a DNA loop that does not allow the RNA polymerase to bind to the promoter. LldR can also have a function as an activator [1]. The repression of the promoter can be removed by lactate.</p>  
  
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<h3>Genetic design for characterization with LldR</h3>
 
<h3>Genetic design for characterization with LldR</h3>
To test our promoter we designed a plasmid containing the promoter with sfGFP in a medium copy plasmid pSEVA261 and transformed it into <i>Escherichia coli</i> TOP10. Then, we added a second plasmid containing lldR with a medium strong promoter ([[Part:BBa_J23118]]) and a strong RBS ([[Part:BBa_B0034]]) in pSEVA371 backbone. According to literature, LldR will repress the promoter and by the addition of lactate the production of GFP will start, as the repressor will be removed.  
+
To test our promoter we designed a plasmid containing the promoter with sfGFP in a medium copy plasmid pSEVA261 and transformed it into <i>Escherichia coli</i> TOP10. Then, we added a second plasmid containing lldR with a medium strong promoter ([[Part:BBa_J23118]]) and a strong RBS ([[Part:BBa_B0034]]) in pSEVA371 backbone. According to literature [1], LldR will repress the promoter and by the addition of lactate the production of GFP will start, as the repressor will be removed.  
 
<h3>Genetic design for characterization with LldP-LldP</h3>
 
<h3>Genetic design for characterization with LldP-LldP</h3>
 
The second step for our characterization was to add an L-lactate permease (LldP), which despite its name is an active transporter of L-lactate, D-lactate and glycolate. To understand the effect of LldP (L-lactatep permease) in our system, we tried the following conditions:
 
The second step for our characterization was to add an L-lactate permease (LldP), which despite its name is an active transporter of L-lactate, D-lactate and glycolate. To understand the effect of LldP (L-lactatep permease) in our system, we tried the following conditions:
 
<ul>
 
<ul>
   <li>Plasmid with the promoter and sfGFP in medium copy number plasmid+ J23114-B0032-lldP-lldR (LldP and LldR are under the control of the same promoter) in low copy number plasmid</li>
+
   <li>Plasmid with the promoter and sfGFP in medium copy number plasmid+ J23114-B0032-lldP-lldR (LldP and LldR are under the control of the same low promoter) in low copy number plasmid</li>
   <li>Plasmid with the promoter and sfGFP in medium copy number plasmid + J23118-B0032-lldP-lldR (LldP and LldR are under the control of the same promoter) in low copy number plasmid</li>
+
   <li>Plasmid with the promoter and sfGFP in medium copy number plasmid + J23118-B0034-lldP-lldR (LldP and LldR are under the control of the same medium promoter) in low copy number plasmid</li>
 
</ul>  
 
</ul>  
  
 
<h3>Plate reader</h3>
 
<h3>Plate reader</h3>
<i>E. coli</i> TOP10 strains were grown overnight in Lysogeny Broth (LB) containing kanamycin (1 &micro;/mL) and chloramphenicol (0.36 &micro;/mL) at 37&deg;C and 200 rpm. Cultures were diluted 1:50 in fresh LB with the corresponding antibiotic and transferred to a 96-well plate (200 &micro;L/well). Cultures were grown for 90 min to arrive to exponential phase and then different concentrations of lactate were added. Samples were always made in triplicates and a blank of LB with the corresponding lactate concentration was done. During 7 h the absorbance at OD600 and fluorescence (excitation 488 nm and emission 530 nm) were measured with intervals of 7 min. The plate was always kept at 37&deg;C. We calculated dose-response curves from the exponential phase of the bacteria.  
+
<i>E. coli</i> TOP10 strains were grown overnight in Lysogeny Broth (LB) containing kanamycin (50 &micro;g/mL) and chloramphenicol (12.5 &micro;g/mL) at 37&deg;C and 200 rpm. Cultures were diluted 1:50 in fresh LB with the corresponding antibiotic and transferred to a 96-well plate (200 &micro;L/well). Cultures were grown for 90 min to arrive to exponential phase and then different concentrations of lactate were added. Samples were always made in triplicates and a blank of LB with the corresponding lactate concentration was done. During 7 h the absorbance at OD600 and fluorescence (excitation 488 nm and emission 530 nm) were measured with intervals of 7 min. The plate was always kept at 37&deg;C in a Tecan Infinite M200 Pro Plate Reader. We calculated dose-response curves from the exponential phase of the bacteria using normalized fluorescence corrected by optical density.  
  
 
<h2>Modeling</h2>
 
<h2>Modeling</h2>
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     <li>al: leakiness in &micro;M/min</li>
 
     <li>al: leakiness in &micro;M/min</li>
 
     <li>mu: constant in &micro;M/min</li>
 
     <li>mu: constant in &micro;M/min</li>
     <li>Km: half-maximum effective concentration (a representation of sensitivity) in &micro;M</li>
+
     <li>K<sub>M</sub>: half-maximum effective concentration (a representation of sensitivity) in &micro;M</li>
 
     <li>n: Hill coefficient (a representation of cooperativity), unitless</li>
 
     <li>n: Hill coefficient (a representation of cooperativity), unitless</li>
 
</ul>
 
</ul>
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|-
 
|-
 
! rowspan="4" scope="row" | Coefficient values  
 
! rowspan="4" scope="row" | Coefficient values  
| K=977.5  (812.6, 1142) || K=2361  (1051, 3671)|| K=459.8  (121.5, 798)
+
| K<sub>M</sub>=977.5  (812.6, 1142) || K<sub>M</sub>=2361  (1051, 3671)|| K<sub>M</sub>=459.8  (121.5, 798)
 
|-
 
|-
 
| al =    1.1e+04  (fixed at bound)||al = 516.7  (-1522, 2555)||al = 1.775e+04  (1.619e+04, 1.93e+04)
 
| al =    1.1e+04  (fixed at bound)||al = 516.7  (-1522, 2555)||al = 1.775e+04  (1.619e+04, 1.93e+04)
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|}
 
|}
  
[[File:ETH15_EngineeredPromoterinLB_medium.png|thumb|center|500px|Comparison of the fluorescence levels obtained using the wild-type promoter alone and in combination with LldR and LldP-LldR]]
+
[[File:ETH15_EngineeredPromoterinLB_medium.png|thumb|center|500px|Figure 2. Comparison of the fluorescence levels obtained using the lldR promoter alone and in combination with LldR and LldP-LldR. Mean fluorescence obtained with n=3 ± SD.]]
  
As can be seen in the picture above, when P<sub>lldR</sub> GFP is alone, the fluorescence levels do not vary with lactate concentration. However, if P<sub>lldR</sub> GFP is expressed in a system with constitutive expression of LldR, at low concentrations of lactate there is repression of the promoter, while at high concentrations there is activation. Activation is higher when there is constitutive expression of LldP-LldR (symbolized in the graph as LldPR).
+
As can be seen in the picture above, when P<sub>lldR</sub> GFP is alone, the fluorescence levels do not vary with lactate concentration. However, if P<sub>lldR</sub> GFP is expressed in a system with constitutive expression of LldR, at low concentrations of lactate there is repression of the promoter, while at high concentrations there is activation. Activation is higher when there is constitutive expression of LldP-LldR (symbolized in the graph as LldPR).  
  
 
This promoter has leakiness when it is expressed with LldP-LldR. Its ON/OFF ratio is smaller than the one in the natural promoter (see Table 1).  
 
This promoter has leakiness when it is expressed with LldP-LldR. Its ON/OFF ratio is smaller than the one in the natural promoter (see Table 1).  
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Table 1: ON/OFF ratio
 
Table 1: ON/OFF ratio
 
{|class="wikitable"
 
{|class="wikitable"
 +
! !!LldR
 +
!colspan="2" scope="column"| Additional LldP
 
|-
 
|-
 
! !!J23118-B0034-lldR!!J23118-B0034-lldP-lldR!!J23114-B0032-lldP-lldR
 
! !!J23118-B0034-lldR!!J23118-B0034-lldP-lldR!!J23114-B0032-lldP-lldR
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|-
 
|-
 
|[[Part:BBa_K1847008]]||15.26||23.96||1.42
 
|[[Part:BBa_K1847008]]||15.26||23.96||1.42
 +
!rowspan="3" scope="row"|Increasing promoter strength
 
|-
 
|-
|[[Part:BBa_K1847009]]||1.56||24.34||0.96
+
|[[Part:BBa_K1847009]]||2.5||24.34||0.96
 
|-
 
|-
|[[Part:BBa_K1847007]]||1.34||3.85||1.29
+
|[[Part:BBa_K1847007]]||2.15||3.85||1.29
 
|-
 
|-
 
|}
 
|}

Latest revision as of 22:31, 27 September 2015

lldRO1-J23118-lldRO2

Collection of promoters regulated by LldR.

Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal NheI site found at 78
    Illegal NheI site found at 101
  • 21
    COMPATIBLE WITH RFC[21]
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    COMPATIBLE WITH RFC[25]
  • 1000
    COMPATIBLE WITH RFC[1000]

Usage and Biology

Figure 1. Theoretical model for the dual function as repressor and activator of LldR.

The natural promoter of LldR (Part:BBa_K822000) consists of two operators (O1 and O2) and a promoter which is intercalated between the operators. It regulates the expression of the lldPRD operon, and it is involved in L-lactate metabolism. This promoter is repressed by a dimer of LldR, possibly by forming a DNA loop that does not allow the RNA polymerase to bind to the promoter. LldR can also have a function as an activator [1]. The repression of the promoter can be removed by lactate.

Characterization of the promoter

We wanted to know how the promoter would respond to the lactate presence and how important is the architecture of the promoter in this response. For this regard, we built several promoters. Part:BBa_K1847002, Part:BBa_K1847003, Part:BBa_K1847004, Part:BBa_K1847005, Part:BBa_K1847006, Part:BBa_K1847007, Part:BBa_K1847008, and Part:BBa_K1847009.

Genetic design for characterization with LldR

To test our promoter we designed a plasmid containing the promoter with sfGFP in a medium copy plasmid pSEVA261 and transformed it into Escherichia coli TOP10. Then, we added a second plasmid containing lldR with a medium strong promoter (Part:BBa_J23118) and a strong RBS (Part:BBa_B0034) in pSEVA371 backbone. According to literature [1], LldR will repress the promoter and by the addition of lactate the production of GFP will start, as the repressor will be removed.

Genetic design for characterization with LldP-LldP

The second step for our characterization was to add an L-lactate permease (LldP), which despite its name is an active transporter of L-lactate, D-lactate and glycolate. To understand the effect of LldP (L-lactatep permease) in our system, we tried the following conditions:

  • Plasmid with the promoter and sfGFP in medium copy number plasmid+ J23114-B0032-lldP-lldR (LldP and LldR are under the control of the same low promoter) in low copy number plasmid
  • Plasmid with the promoter and sfGFP in medium copy number plasmid + J23118-B0034-lldP-lldR (LldP and LldR are under the control of the same medium promoter) in low copy number plasmid

Plate reader

E. coli TOP10 strains were grown overnight in Lysogeny Broth (LB) containing kanamycin (50 µg/mL) and chloramphenicol (12.5 µg/mL) at 37°C and 200 rpm. Cultures were diluted 1:50 in fresh LB with the corresponding antibiotic and transferred to a 96-well plate (200 µL/well). Cultures were grown for 90 min to arrive to exponential phase and then different concentrations of lactate were added. Samples were always made in triplicates and a blank of LB with the corresponding lactate concentration was done. During 7 h the absorbance at OD600 and fluorescence (excitation 488 nm and emission 530 nm) were measured with intervals of 7 min. The plate was always kept at 37°C in a Tecan Infinite M200 Pro Plate Reader. We calculated dose-response curves from the exponential phase of the bacteria using normalized fluorescence corrected by optical density.

Modeling

Each experimental data set was fitted to a Hill function using the Least Absolute Residual method (Fitting Toolbox in MatLab).

ETH15 equation.png

Where:

  • al: leakiness in µM/min
  • mu: constant in µM/min
  • KM: half-maximum effective concentration (a representation of sensitivity) in µM
  • n: Hill coefficient (a representation of cooperativity), unitless


J23118-B0034-lldR J23118-B0034-lldP-lldR J23114-B0032-lldP-lldR
Coefficient values KM=977.5 (812.6, 1142) KM=2361 (1051, 3671) KM=459.8 (121.5, 798)
al = 1.1e+04 (fixed at bound) al = 516.7 (-1522, 2555) al = 1.775e+04 (1.619e+04, 1.93e+04)
mu = 1.717e+04 (1.634e+04, 1.8e+04) mu = 1.256e+04 (9078, 1.603e+04) mu = 1.711e+04 (1.366e+04, 2.057e+04)
n1 = 1.084 (0.8159, 1.352) n1 = 0.7986 (0.3991, 1.198) n1 = 0.7485 (0.3491, 1.148)
Goodness to fit sse: 5.5485e+08 sse: 3.3911e+08 sse: 9.3519e+09
rsquare: 0.9967 rsquare: 0.9894 rsquare: 0.9835
fe: 8 dfe: 7 dfe: 7
adjrsquare: 0.9959 adjrsquare: 0.9848 adjrsquare: 0.9764
rmse: 8.3280e+03 rmse: 6.9602e+03 rmse: 3.6551e+04
Figure 2. Comparison of the fluorescence levels obtained using the lldR promoter alone and in combination with LldR and LldP-LldR. Mean fluorescence obtained with n=3 ± SD.

As can be seen in the picture above, when PlldR GFP is alone, the fluorescence levels do not vary with lactate concentration. However, if PlldR GFP is expressed in a system with constitutive expression of LldR, at low concentrations of lactate there is repression of the promoter, while at high concentrations there is activation. Activation is higher when there is constitutive expression of LldP-LldR (symbolized in the graph as LldPR).

This promoter has leakiness when it is expressed with LldP-LldR. Its ON/OFF ratio is smaller than the one in the natural promoter (see Table 1).

This promoter is one from our designed and tested synthetic promoters based on the wild-type PlldR. In the following table, one can see the ON/OFF ratios and the KM of the wild-type promoter and the three more prominent members of the library.

Table 1: ON/OFF ratio

LldR Additional LldP
J23118-B0034-lldR J23118-B0034-lldP-lldR J23114-B0032-lldP-lldR
Part:BBa_K822000 (wild-type) 10.35 8.04 1.16
Part:BBa_K1847008 15.26 23.96 1.42 Increasing promoter strength
Part:BBa_K1847009 2.5 24.34 0.96
Part:BBa_K1847007 2.15 3.85 1.29

Table 2: KM (µM)

J23118-B0034-lldR J23118-B0034-lldP-lldR J23114-B0032-lldP-lldR
Part:BBa_K822000 (wild-type) 955 1930 720.2
Part:BBa_K1847008 1075 1751 337.5
Part:BBa_K1847009 977.5 2361 459.8
Part:BBa_K1847007 697.7 1977 1337

References

  1. J Bacteriol. 2008 Apr; 190(8): 2997–3005.