Difference between revisions of "Part:BBa K633014"
 
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The composite part includes a functional expression device for autotransporter membrane protein estA, with a linker united to a cellulase, attached to a membrane signaling peptide. This was our final construct missing a terminator.
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The composite part includes a functional expression device for autotransporter membrane protein estA, with a linker united to a cellulase, attached to a membrane signaling peptide. This was our final construct missing a terminator. '''By the use of the restriction enzymes, NheI and SacI, more enzymes can be displayed outside the outer membrane of ''E. coli.'''''
  
  
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In order to find suitable arabinose concentrations to induce expression of the construct, the protein coding sequences were substituted by a GFP reporter, BBa_e0040. A double terminator, BBa_e0014, was added as well. The expression vehicle was Escherichia coli, BW27783 strain, due to its inability to metabolize arabinose. Fluorescence was measured in transformed E. coli cultures induced with different concentrations of L-arabinose (1%), following the protocol used by Cambridge (2009) and Tec-Monterrey (2010).  
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In order to find suitable arabinose concentrations to induce expression of the construct, the protein coding sequences were substituted by a GFP reporter, BBa_e0040. A double terminator, BBa_e0014, was added as well. The expression vehicle was ''Escherichia coli'', BW27783 strain, due to its inability to metabolize arabinose. Fluorescence was measured in transformed ''E. coli'' cultures induced with different concentrations of L-arabinose (1%), following the protocol used by Cambridge (2009) and Tec-Monterrey (2010).  
  
 
<center>[[Image:Induction_gfp.jpg‎]]</center>
 
<center>[[Image:Induction_gfp.jpg‎]]</center>
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The chart shows that at low concentrations of arabinose, poor induction levels are obtained since fluorescence changes very little over time. A noticeable increase of fluorescence is viewed from a concentration of 100 µM onwards. Similar results were found in BBa_I0500 characterization by Cambridge (2011) and Groningen (2011), proving further the effectiveness of using this concentration of arabinose as a minimum to induce expression of the construct.
 
The chart shows that at low concentrations of arabinose, poor induction levels are obtained since fluorescence changes very little over time. A noticeable increase of fluorescence is viewed from a concentration of 100 µM onwards. Similar results were found in BBa_I0500 characterization by Cambridge (2011) and Groningen (2011), proving further the effectiveness of using this concentration of arabinose as a minimum to induce expression of the construct.
 
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'''The Escherichia coli strain, Rosetta Gami, was choosen as a host for the chimeric protein because it has an improved folding system.'''
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Whole-Cell CelD+estA Activity
 
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<center>[[Image:ThelWhole.png‎]]
 
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We used the IUPAC Filter Paper Assay, to determine the activity of the cellulase. This method is based in the reduction of the DNS, generating a proportional colorimetric concentration.<br>
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Figure 2. Whole-Cell Cellulase Activity.  
The assay was assest to the whole-cells, but also, we lysated the cells and separated them in two main fractions: soluble and insoluble. We were expecting more activity in the insoluble because our protein has a transmembranal domain.
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The negative controls of the assay were non-transformed cells.
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The glucose concentration in celD + estA strain was of 332.04 µM and in the Negative Control (C-) was of 275.85 µM that is a difference in the glucose concentration of 57 µM. The result of the t- test was the rejection of the null hypothesis, suggesting that the difference between them is significant.
All samples were treated equally in the assay.
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In the “ Whole-cell cellulase Activity” chart, is observed that there is a difference in the glucose concentration between the Negative Control cells (C-) and the CelD+ estA cells. A t-student was done (sigma = 0.05) . The result was the rejection of the null hypothesis (Ho), this meant that the difference was significant.
 
 
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<center>[[Image:Graficathelma01.png]]</center>
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Cell-Lysate CelD+estA Activity
 
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In the “Cellulase Activity Cell Lysates” is analysed two fractions : Soluble ans Insoluble. As it can be seen, in both cases, there is a difference between the celD+estA cells and their respective Negative Controls (C-) . Also, it is noticed that there is a higher difference in the Insoluble fraction that in the Soluble one. A t-student was done (sigma = 0.05). The result was the rejection of the null hypothesis (Ho), this meant that the difference was significant.  
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<center>[[Image:Thelsolinsol.png‎]]
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Figure 3.Cellulase Activity of Cell lysates.
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In the cell-lysate cellulase activity assay (Figure 3) The glucose concentration in the soluble fraction of celD-estA was of 358 µM and in the Negative Control (C-) was of 323 µM.In the insoluble fraction, the glucose contentration of the celD-estA was 374 µM and in the Negative Control (C-) was of 264 µM. The difference in soluble and insoluble fractions with its negative control was 35 µM while the difference in the insoluble fraction was 110 µM. The result of the t-test was the rejection of the null hyphothesis, suggesting that the difference between them is also significant.
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<center>[[Image:Grafica02thelma.png‎]]</center>
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'''Note: There is an ilegal NheI restrition site in the promoter region, part BBa_K206000'''.
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'''References:'''
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<!-- Add more about the biology of this part here
 
<!-- Add more about the biology of this part here
 
===Usage and Biology===
 
===Usage and Biology===

Latest revision as of 01:25, 20 October 2011

AraC+Pbad promoter+RBS+signal peptide phoA+Cellulase+Linker+estA membrane protein

The composite part includes a functional expression device for autotransporter membrane protein estA, with a linker united to a cellulase, attached to a membrane signaling peptide. This was our final construct missing a terminator. By the use of the restriction enzymes, NheI and SacI, more enzymes can be displayed outside the outer membrane of E. coli.


The construct efectiveness was tested by an enzymatic assay, The results can be seen here: http://2011.igem.org/Team:Tec-Monterrey/projectresults


In order to find suitable arabinose concentrations to induce expression of the construct, the protein coding sequences were substituted by a GFP reporter, BBa_e0040. A double terminator, BBa_e0014, was added as well. The expression vehicle was Escherichia coli, BW27783 strain, due to its inability to metabolize arabinose. Fluorescence was measured in transformed E. coli cultures induced with different concentrations of L-arabinose (1%), following the protocol used by Cambridge (2009) and Tec-Monterrey (2010).

Induction gfp.jpg

The chart shows that at low concentrations of arabinose, poor induction levels are obtained since fluorescence changes very little over time. A noticeable increase of fluorescence is viewed from a concentration of 100 µM onwards. Similar results were found in BBa_I0500 characterization by Cambridge (2011) and Groningen (2011), proving further the effectiveness of using this concentration of arabinose as a minimum to induce expression of the construct.



Whole-Cell CelD+estA Activity

ThelWhole.png


Figure 2. Whole-Cell Cellulase Activity.


The glucose concentration in celD + estA strain was of 332.04 µM and in the Negative Control (C-) was of 275.85 µM that is a difference in the glucose concentration of 57 µM. The result of the t- test was the rejection of the null hypothesis, suggesting that the difference between them is significant.



Cell-Lysate CelD+estA Activity

Thelsolinsol.png

Figure 3.Cellulase Activity of Cell lysates.


In the cell-lysate cellulase activity assay (Figure 3) The glucose concentration in the soluble fraction of celD-estA was of 358 µM and in the Negative Control (C-) was of 323 µM.In the insoluble fraction, the glucose contentration of the celD-estA was 374 µM and in the Negative Control (C-) was of 264 µM. The difference in soluble and insoluble fractions with its negative control was 35 µM while the difference in the insoluble fraction was 110 µM. The result of the t-test was the rejection of the null hyphothesis, suggesting that the difference between them is also significant.


Note: There is an ilegal NheI restrition site in the promoter region, part BBa_K206000.


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal NheI site found at 1247
    Illegal NheI site found at 3168
  • 21
    INCOMPATIBLE WITH RFC[21]
    Illegal BamHI site found at 1187
    Illegal BamHI site found at 1981
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal NgoMIV site found at 1845
    Illegal NgoMIV site found at 3398
    Illegal AgeI site found at 979
    Illegal AgeI site found at 1488
    Illegal AgeI site found at 1904
    Illegal AgeI site found at 2733
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal SapI site found at 961