Difference between revisions of "Part:BBa K3093002"
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<html><img style="width:600px;padding-left:100px;" src="https://2019.igem.org/wiki/images/4/41/T--ECUST_China--regulator_circuit-cello.png"> </html><br><span style="font-size: 14px;">  
 
<html><img style="width:600px;padding-left:100px;" src="https://2019.igem.org/wiki/images/4/41/T--ECUST_China--regulator_circuit-cello.png"> </html><br><span style="font-size: 14px;">  
<b>Figure.1 Gene circuit of cellobiose response element</b> </span>
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<b>Figure.1 Gene circuit of cellobiose response element</b>  
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Cellobiose response element is the mutant of <i>chb</i> operon in <i>E.coli</i>. Wild‐type strains of <i>Escherichia coli</i> are normally unable to metabolize cellobiose. The <i>chb</i> operon is the inducible genetic system involved in the catabolism of N,N′‐diacetylchitobiose. However, single base‐pair changes in the transcriptional regulator chbR that translate into single‐amino‐acid substitutions constitute the cellobiose operon which can response cellobiose. So, ECUST_China iGEMers performed several types of mutation: chbRN137K, chbRY30C and chbRN238S, aiming to find a efficient cellobiose response element.
 
Cellobiose response element is the mutant of <i>chb</i> operon in <i>E.coli</i>. Wild‐type strains of <i>Escherichia coli</i> are normally unable to metabolize cellobiose. The <i>chb</i> operon is the inducible genetic system involved in the catabolism of N,N′‐diacetylchitobiose. However, single base‐pair changes in the transcriptional regulator chbR that translate into single‐amino‐acid substitutions constitute the cellobiose operon which can response cellobiose. So, ECUST_China iGEMers performed several types of mutation: chbRN137K, chbRY30C and chbRN238S, aiming to find a efficient cellobiose response element.
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<html><img style="width:600px;padding-left:100px;" src="https://2019.igem.org/wiki/images/b/bb/T--ECUST_China--regulator_cellomrfp.png"> </html><br><span style="font-size: 14px;">  
 
<html><img style="width:600px;padding-left:100px;" src="https://2019.igem.org/wiki/images/b/bb/T--ECUST_China--regulator_cellomrfp.png"> </html><br><span style="font-size: 14px;">  
 
<b>Figure.2 The PCR results of pCEL backbone and chbR</b>  
 
<b>Figure.2 The PCR results of pCEL backbone and chbR</b>  
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After constructing the mutation plasmids: pIN1-NK and pIN1-YC-NS. Both of the mutant clones and the wild-type strain were incubated in M9 medium containing 0.4% glycerol and 0.4% casamino acids, with or without 10 mM cellobiose for about 40 hours. All of the samples were transferred to 96-well plate to measure the mRFP fluorescence.
 
After constructing the mutation plasmids: pIN1-NK and pIN1-YC-NS. Both of the mutant clones and the wild-type strain were incubated in M9 medium containing 0.4% glycerol and 0.4% casamino acids, with or without 10 mM cellobiose for about 40 hours. All of the samples were transferred to 96-well plate to measure the mRFP fluorescence.
  
 
<html><img style="width:600px;padding-left:100px;" src="https://2019.igem.org/wiki/images/e/e2/T--ECUST_China--BBa_K3093002.jpg"> </html><br><span style="font-size: 14px;">  
 
<html><img style="width:600px;padding-left:100px;" src="https://2019.igem.org/wiki/images/e/e2/T--ECUST_China--BBa_K3093002.jpg"> </html><br><span style="font-size: 14px;">  
<b>Figure 3.11</b> Fluorescence intensity induced by cellobiose</span>
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<b>Figure.3 Fluorescence intensity induced by cellobiose</b>
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The results revealed that presence of both chbR mutants resulted in a high basal level of expression. More importantly, the transformant carrying ChbRYC-NS showed an approximately threefold induction.
 
The results revealed that presence of both chbR mutants resulted in a high basal level of expression. More importantly, the transformant carrying ChbRYC-NS showed an approximately threefold induction.

Revision as of 14:00, 20 October 2019


Cellobiose operon


Figure.1 Gene circuit of cellobiose response element


Cellobiose response element is the mutant of chb operon in E.coli. Wild‐type strains of Escherichia coli are normally unable to metabolize cellobiose. The chb operon is the inducible genetic system involved in the catabolism of N,N′‐diacetylchitobiose. However, single base‐pair changes in the transcriptional regulator chbR that translate into single‐amino‐acid substitutions constitute the cellobiose operon which can response cellobiose. So, ECUST_China iGEMers performed several types of mutation: chbRN137K, chbRY30C and chbRN238S, aiming to find a efficient cellobiose response element.

During the experiment, we used mRFP as the reporter. The sequence of Pcel and chbR was obtained from E.coli K12 MG1655 via PCR .Then we performed inverse PCR to achieve the site-directed mutation of amino acids of chbR. According to the literature, we chose three site-directed mutation : chbRN238S, chbRY30C and chbRN137K.


Figure.2 The PCR results of pCEL backbone and chbR


After constructing the mutation plasmids: pIN1-NK and pIN1-YC-NS. Both of the mutant clones and the wild-type strain were incubated in M9 medium containing 0.4% glycerol and 0.4% casamino acids, with or without 10 mM cellobiose for about 40 hours. All of the samples were transferred to 96-well plate to measure the mRFP fluorescence.


Figure.3 Fluorescence intensity induced by cellobiose


The results revealed that presence of both chbR mutants resulted in a high basal level of expression. More importantly, the transformant carrying ChbRYC-NS showed an approximately threefold induction. Over the basal level in the presence of 10 mM cellobiose whereas no induction was seen in the presence of wild-type ChbR.


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]