Difference between revisions of "Team:ECUST/Biofilm Remover"

 
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<div id="bannerspace">
 
<div id="bannerspace">
 
      
 
      
     <div id="bannerquote">Overview</div>
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     <div id="bannerquote">Biofilm Remover</div>
 
      
 
      
 
 
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<main>
 
<main>
 
<div class="contentbox">
 
<div class="contentbox">
<h1 class="box-heading">Design</h1>
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<h1 class="box-heading">Description</h1>
<p>“Human Practices is the study of how your work affects the world, and how the world affects the work.” (Peter Carr, Director of Judging) is the comment which gives a clear definition of all Human Practices activities. Therefore, we tried to answer two questions: how can synthetic biology affect the world? And in which way can the world affect Iron Guardian? To answer the former one, we chose to collaborate with different teams and thought the issues we are working on vary from team to team, we all wish and try to utilize what we learn to solve practical problems and make the world a better one. What’s more, we integrated the social influence into our project to answer the latter question. With communication, economic benefit and responsibility as our important focus, we interviewed professors and employees in related industry, and showcased the great economic benefit of our project. By distributing questionnaire and analyzing the data acquired, we managed to explain and improve our project according to the public concerns and suggestions. The new concept of “3+ net” raised by ECUST will also help all teams to create, to reflect, and to improve.</p>
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<p>Dispersin B is a β-hexosaminidase that specifically hydrolyzes β-1,6-glycosidic linkages of acetylglucosamine polymers found in biofilm. This enzyme is derived from <i>Aggregatibacter actinomycetemcomitans</i>, which secretes adherent cells from mature biofilm colonies by secreting disperse B. The active site of Disperse B contains three highly conserved acidic residues: aspartic acid at residue 183 (D183), glutamic acid at residue 184 (E184), and glutamic acid at residue 332 (E332). </p>
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<figure>
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<figure class="makeresponsive" style="width: 50%;margin-left:22%;margin-right:30%;">
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<img src="https://static.igem.org/mediawiki/2018/9/9e/T--ECUST--biofile1.png" alt="Figure1.1 OD600 reference point tab" class="zoom">
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<figcaption><b>Blue color shows the E184;Pink color shows the D183;Yellow color shows the E332.</b></figcaption>
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</figure>
 
</div>
 
</div>
  
 
<div class="contentbox">
 
<div class="contentbox">
<h1 class="box-heading">Construct</h1>
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<h1 class="box-heading">Design</h1>
<p>In order to test the biofilm removal effect of DSPB, we constructed the vector pET28a-DSPB</p>
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<p>We hope that DspB, like siderophore, is regulated by AHL, and when AHL is present, the dspb gene will express. Given that the DspB enzyme activity is low, we planed to make it accumulate in cells first, and then be released by the subsequent lysis system.</p>
<p>The plasmid was transformed into E. coli BL21, cultured at 37 °C for 12 h, and the plasmid was extracted and verified by PCR.</p>
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<figure>
 
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<figure class="makeresponsive" style="width: 50%;margin-left:23%;margin-right:30%;">
 +
<img src="https://static.igem.org/mediawiki/2018/f/f5/T--ECUST--biofile2.png" alt="Figure1.1 OD600 reference point tab" class="zoom">
 +
<figcaption><b></b></figcaption>
 +
</figure>
 
</div>
 
</div>
  
<div class="contentbox">
 
<h1 class="box-heading">Result</h1>
 
<p>In order to test the biofilm removal effect of DSPB, we constructed the vector pET28a-DSPB</p>
 
<p>The plasmid was transformed into E. coli BL21, cultured at 37 °C for 12 h, and the plasmid was extracted and verified by PCR.</p>
 
<p>To test the expression of DSPB, we cultured E. coli in LB medium containing 0.1% kan. E. coli was cultured at 37℃ and 220 rpm for all night, then inoculated into fresh medium and cultured until logarithmic phase.Add IPTG to final concentration of 20uM and culture E. coli over night at 25℃. Final OD600=0.437(diluted 16 fold) </p>
 
  
 +
<div class="contentbox">
 +
<h1 class="box-heading">Result:</h1>
 +
<p>In order to test the biofilm removal effect of DspB, we constructed the vector pET28a-dspB. </p>
 +
<figure>
 +
<figure class="makeresponsive" style="width: 50%;margin-left:22%;margin-right:30%;">
 +
<img src="https://static.igem.org/mediawiki/2018/5/5c/T--ECUST--result--biofilm_remove_BIOFILM1.jpg" alt=" class="B1">
 +
<figcaption><b>Figure 1. Construction of the expression vector pET28a-dspB. The Kan represents kanamycin resistance marker. The part dspB was inserted by the restriction site BamHI and XhoI</b></figcaption>
 +
</figure>
 +
<p>The plasmid was transformed into <i>E. coli</i> BL21, cultured at 37 °C for 12 h, and the plasmid was extracted and verified by PCR. </p>
 +
<p></p>
 +
<figure class="makeresponsive" style="width: 50%;margin-left:22%;margin-right:30%;">
 +
<img src="https://static.igem.org/mediawiki/2018/0/00/T--ECUST--result--biofilm_remove_BIOFILM2.jpg
 +
" alt=" class="b2">
 +
<figcaption><b>Figure 2. 1% Agarose Gel Electrophoresis of DNA extracted from the positive clones (a)and its identification by PCR(b), which shows that our vector was successfully constructed</b></figcaption>
 +
</figure>
 +
<p>To test the expression of DspB, we cultured <i>E. coli</i> in LB medium containing 0.1% kan. <i>E. coli</i> was cultured at 37℃ and 220 rpm for all night, then inoculated into fresh medium and cultured until logarithmic phase.Add IPTG to final concentration of 20uM and culture <i>E. coli</i> over night at 25℃. Final OD600=0.437(diluted 16 fold) </p>
 +
<p></p>
 +
<figure class="makeresponsive" style="width: 50%;margin-left:22%;margin-right:30%;">
 +
<img src="https://static.igem.org/mediawiki/2018/0/0d/T--ECUST--result--biofilm_remove_BIOFILM3.jpg" alt=" class="B3">
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<figcaption><b>Figure 3.The SDS-PAGE of DspB
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Lane 1,2  Lane 1,2 before induction
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        Lane 3  cell cultue media
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        Lane4,5,6 after induction
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</b></figcaption>
 +
</figure>
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<p>The expression of DspB was verified by SDS-PAGE(Figure 3). The cell culture medium was blank control, and the pre-induction cell supernatant was used as a negative control. </p>
 +
<p>In the figure 3 we can see that there are bands at about 37 kDa, these band of  experimental groups are thicker than the negative control. And our target protein is about 40kDa. We think the protein here may be DspB. </p>
 +
<p>Then, we tested whether the engineered bacteria expressed active DspB through enzyme activity experiments. </p>
 +
<p>4-nitrophenyl-N-acetyl -β-D-glucosaminide(NP-GlcNAc) is hydrolysed by DspB and become 4-nitrophenol with the maximum light absorption at 405 nm. 20 mLbacteria solution is disrupted and acted supernatant as DspB enzyme solution.
 +
We washed and shred the bacterial solution after induction, and took the supernatant as the enzyme reaction solution of DspB while NP-GlcNAc working as a substrate.The enzyme activity experiment was carried out by using 100 μL of enzyme reaction solution and 100 μL of substrate solution (substrate concentration is 5 mM). </p>
 +
<p></p>
 +
<figure>
 +
<figure class="makeresponsive" style="width: 50%;margin-left:22%;margin-right:30%;">
 +
<img src="https://static.igem.org/mediawiki/2018/b/b8/T--ECUST--result--biofilm_remove_BIOFILM4.jpg" alt=" class="B4">
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<figcaption><b>Figure 4:DspB enzyme activity assay curve
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</b></figcaption>
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</figure>
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<p>The enzyme activity of the supernatant calculated by the enzyme activity calculation formulais (Activity/(U/mL)=(kOD405-kseldecomposition)*18231.26 *dilution ratio) is 66.363U/mL. </p>
 +
<p>The experiment proved that the recombinant bacteria expressed active DspB, and we used the <i>E. coli</i> supernatant with DspB activity to carry out the biofilm removal experiment.DH5a was cultured overnight in LB at 37 ° C and 220 rpm, and transferred to a 96-well plate at 37 ° C and cultured for 48 h, then discarded the supernatant .The biofilm was washed with PBS, and 200 uL of the reaction solution was added to react for the whole night. Add crystal violet to stain, wash the solution into the new well plate after alcohol washing, and measure the absorbance at 570 nm. The smaller the absorbance value, the better the membrane removal effect. </p>
 +
<p></p>
 +
<figure>
 +
<figure class="makeresponsive" style="width: 50%;margin-left:22%;margin-right:30%;">
 +
<img src="https://static.igem.org/mediawiki/2018/2/2c/T--ECUST--result--biofilm_remove_BIOFILM5.jpg" alt=" class="B4">
 +
<figcaption><b>Figure 5. (a) Crystal violet staining results of different reaction solutions added to biofilm
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          (b) Biofilm removal rate of different reaction solutions added to biofilm
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          (c) DspB biofilm-removing curve
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OD570=51.96-51.24t0.0051
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R2=0.98385
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</b></figcaption>
 +
</figure>
 +
<p>From Fig.5, The supernatant of the recombinant <i>E. coli</i>  has the highest biofilm removal rate, and the biofilm removal effect is getting better with time. </p>
 
</div>
 
</div>
  
 +
 +
<div class="contentbox">
 +
<h1 class="box-heading">Reference</h1>
 +
<p>1. Nature Communications 11 April 2017 Engineered probiotic <i>Escherichia coli</i> can eliminate and prevent <i>Pseudomonas aeruginosa</i> gut infection in animal models in Young Hwang</p>
 +
<p>2. Biotechnological Products and Process Engineering 23 July 2004 Inhibiting mild steel corrosion from <i>sulfate-reducing</i> and <i>iron-oxidizing bacteria</i> using gramicidin-S-producing biofilms</p>
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</div>
  
  

Latest revision as of 01:34, 18 October 2018

Biofilm Remover

Description

Dispersin B is a β-hexosaminidase that specifically hydrolyzes β-1,6-glycosidic linkages of acetylglucosamine polymers found in biofilm. This enzyme is derived from Aggregatibacter actinomycetemcomitans, which secretes adherent cells from mature biofilm colonies by secreting disperse B. The active site of Disperse B contains three highly conserved acidic residues: aspartic acid at residue 183 (D183), glutamic acid at residue 184 (E184), and glutamic acid at residue 332 (E332).

Figure1.1 OD600 reference point tab
Blue color shows the E184;Pink color shows the D183;Yellow color shows the E332.

Design

We hope that DspB, like siderophore, is regulated by AHL, and when AHL is present, the dspb gene will express. Given that the DspB enzyme activity is low, we planed to make it accumulate in cells first, and then be released by the subsequent lysis system.

Figure1.1 OD600 reference point tab

Result:

In order to test the biofilm removal effect of DspB, we constructed the vector pET28a-dspB.

class=
Figure 1. Construction of the expression vector pET28a-dspB. The Kan represents kanamycin resistance marker. The part dspB was inserted by the restriction site BamHI and XhoI

The plasmid was transformed into E. coli BL21, cultured at 37 °C for 12 h, and the plasmid was extracted and verified by PCR.

class=
Figure 2. 1% Agarose Gel Electrophoresis of DNA extracted from the positive clones (a)and its identification by PCR(b), which shows that our vector was successfully constructed

To test the expression of DspB, we cultured E. coli in LB medium containing 0.1% kan. E. coli was cultured at 37℃ and 220 rpm for all night, then inoculated into fresh medium and cultured until logarithmic phase.Add IPTG to final concentration of 20uM and culture E. coli over night at 25℃. Final OD600=0.437(diluted 16 fold)

class=
Figure 3.The SDS-PAGE of DspB Lane 1,2 Lane 1,2 before induction Lane 3 cell cultue media Lane4,5,6 after induction

The expression of DspB was verified by SDS-PAGE(Figure 3). The cell culture medium was blank control, and the pre-induction cell supernatant was used as a negative control.

In the figure 3 we can see that there are bands at about 37 kDa, these band of experimental groups are thicker than the negative control. And our target protein is about 40kDa. We think the protein here may be DspB.

Then, we tested whether the engineered bacteria expressed active DspB through enzyme activity experiments.

4-nitrophenyl-N-acetyl -β-D-glucosaminide(NP-GlcNAc) is hydrolysed by DspB and become 4-nitrophenol with the maximum light absorption at 405 nm. 20 mLbacteria solution is disrupted and acted supernatant as DspB enzyme solution. We washed and shred the bacterial solution after induction, and took the supernatant as the enzyme reaction solution of DspB while NP-GlcNAc working as a substrate.The enzyme activity experiment was carried out by using 100 μL of enzyme reaction solution and 100 μL of substrate solution (substrate concentration is 5 mM).

class=
Figure 4:DspB enzyme activity assay curve

The enzyme activity of the supernatant calculated by the enzyme activity calculation formulais (Activity/(U/mL)=(kOD405-kseldecomposition)*18231.26 *dilution ratio) is 66.363U/mL.

The experiment proved that the recombinant bacteria expressed active DspB, and we used the E. coli supernatant with DspB activity to carry out the biofilm removal experiment.DH5a was cultured overnight in LB at 37 ° C and 220 rpm, and transferred to a 96-well plate at 37 ° C and cultured for 48 h, then discarded the supernatant .The biofilm was washed with PBS, and 200 uL of the reaction solution was added to react for the whole night. Add crystal violet to stain, wash the solution into the new well plate after alcohol washing, and measure the absorbance at 570 nm. The smaller the absorbance value, the better the membrane removal effect.

class=
Figure 5. (a) Crystal violet staining results of different reaction solutions added to biofilm (b) Biofilm removal rate of different reaction solutions added to biofilm (c) DspB biofilm-removing curve OD570=51.96-51.24t0.0051 R2=0.98385

From Fig.5, The supernatant of the recombinant E. coli has the highest biofilm removal rate, and the biofilm removal effect is getting better with time.

Reference

1. Nature Communications 11 April 2017 Engineered probiotic Escherichia coli can eliminate and prevent Pseudomonas aeruginosa gut infection in animal models in Young Hwang

2. Biotechnological Products and Process Engineering 23 July 2004 Inhibiting mild steel corrosion from sulfate-reducing and iron-oxidizing bacteria using gramicidin-S-producing biofilms