Difference between revisions of "Team:Nankai/Practices"

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                    <p>Your place:&nbsp;<a href="https://2015.igem.org/Team:Nankai">Home</a>&nbsp;&gt;&nbsp;<a href="https://2015.igem.org/Team:Nankai/Description">Project</a>&nbsp;&gt;&nbsp;<a href="https://2015.igem.org/Team:Nankai/project_background">Background</a></p>
   
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<h2 class="page-title">Project Background</h2>
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                            <h2 class="header-section-title">What Did we do on Human practice</h2>
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                            <h4 id="1">Human Practices is the study of how your work affects the world, and how the world affects your work.</h4>
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                                <h2>Communication</h2>
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<h4>1. Pudding health kit — Wound healing hydrogel based on γ-PGA</h4>
                                <p>Communication  means improvement and achievement of Double-win. For example, Tianjin University  is not only our neighbor but also our good collaborator on experiment and human  practice.</p>
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<p>Poly-γ-glutamic acid (γ-PGA) is a naturally occurring biopolymer that is water soluble, non-toxic, edible, and biodegradable, which has shown to promote cell migration and enhance cell adhesion. Besides, γ-PGA has been reported to prevent postsurgical tissue adhesion and the γ-PGA drug-loaded hydrogel to promote wound healing.</p>
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<p>We prepared two types of SOD-PGA hydrogels for wound healing. γ-PGA hydrogel had high water absorption properties delivering the important moist environment. SOD released from the hydrogel maintained high enzyme activity and SOD-PGA hydrogels could scavenge the superoxide anion effectively. In vivo results showed that SOD-PGAS/PGA-H could promote collagen deposition, epithelialization, and accelerate the healing of moderately exuding wounds. Therefore, SOD-PGA hydrogels would be a good candidate for wound healing applications.<a href="https://2015.igem.org/Team:Nankai/Design">Learn about more here.</a>
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<h4>2. γ-PGA producing strain — <em>Bacillus amyloliquefaciens</em> LL3</h4>
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<p>Strains capable for producing γ-PGA are divided into two categories based on their requirement for glutamate acid: glutamate-dependent strains and glutamate-independent strains. Glutamate-independent strains are preferable for industrial production because of their low cost and simplified fermentation process. However, compared with glutamate-dependent strains, their lower γ-PGA productivity limits their industrial application. Therefore, the construction of a glutamate-independent strain with high γ-PGA yield is important for industrial applications. </p>
 +
<p>
 +
<em>B. amyloliquefaciens</em> strains are ubiquitous in the soil and are great reservoirs of important natural products, such as α-amylase, levansucrase, and fibrinolytic enzymes. Besides important cell factories, <em>B. amyloliquefaciens</em> strains are also used as plant growth-promoting and bio-control bacteria partly due to their ability to produce substances with antifungal, antibacterial and nematocidal activities. <em>B. amyloliquefaciens</em> LL3, isolated from fermented food, is a glutamate-independent strain, which can produce γ-PGA with sucrose as its carbon source and ammonium sulfate as its nitrogen source.
 +
</p>
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<h4>3. Methods to increase poly-γ-glutamic acid production</h4>
 +
<p>In this study, we aimed to improve the γ-PGA production based on the <em>B. amyloliquefaciens</em> NK-1 strain (a derivative of LL3 strain with its endogenous plasmid and <em>upp</em> gene deleted). In order to improve γ-PGA production, we employed two strategies to fine-tune the synthetic pathways and balance the metabolism in the glutamate-independent <em>B. amyloliquefaciens</em> NK-1 strain.</p>
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<h5>3.1 Metabolic toggle switch</h5>
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<img src="https://static.igem.org/mediawiki/2015/f/f0/Nankai_pathwaydesign.jpg">
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<h6>Figure 4. Biosynthetic pathway of poly-γ-glutamic acid. Red arrows shows the metabolic flux towards γ-PGA synthesis. The blue arrow is the leakage of metabolic flux.</h6>
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<p>Firstly, we aimed to increase the intracellular concentration of γ-PGA precursor-- glutamate. In <em>B. amyloliquefaciens</em>,2-oxoglutarate is very important for the synthesis of glutamate, yet large amount of 2-oxoglutarate is consume by TCA cycle to turn into succinl-CoA in the action of enzyme ODHC (2-oxoglutarate dehydrogenase complex). Scientists had found that the activity of ODHC was rather low when glutamate was highly produced in a <em>Corynebacterium glutamicum</em> strain. This made us wonder, could we be able to increase the amount of intracellular glutamate by inhibiting the expression of ODHC at the stationary phase in <em>B. amyloliquefaciens</em>? Therefore, we constructed a metabolic toggle switch in the NK-1 strain to inhibit the expression of ODHC by adding IPTG in the stationary stage, trying to distribute the metabolic flux more frequently to be used for γ-PGA precursor-glutamate synthesis.</p>
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<img src="https://static.igem.org/mediawiki/2015/1/13/Nankai_switchdesign.jpg">
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<h6>Figure 5. Metabolic toggle switch to regulate the expression of ODHC.</h6>
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<p>Without IPTG, the promoter Pgrac is inhibited by suppressor LacI and the supreessor XylR will not synthesized, thus the promoter Pxyl is active and <em>odhAB</em> genes are expressed. When IPTG is added, the <em>xylR</em> gene is expressed and the suppressor XylR is synthesized thereafter inhibited the expression of <em>odhAB</em> genes.</p>
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<h5>3.2 Replacement of promoters</h5>
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<p>Secondly, to balance the increase of endogenous glutamate production, we optimized the expression level of <em>pgsBCA</em> genes (responsible for γ-PGA synthesis) by replacing its native promoter with six different strength promoters.</p>
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<img src="https://static.igem.org/mediawiki/2015/3/3a/Nankai_genesdesign.jpg">
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<h6>Figure 6.Genes responsible for γ-PGA synthesis</h6>
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<p>Through these two strategies, we aimed to obtain a γ-PGA production improved mutant strain.</p>
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<h6><a href="https://2015.igem.org/Team:Nankai/Description">Description</a></h6>
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<h6><a href="https://2015.igem.org/Team:Nankai/project_background">Background</a></h6>
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<h6><a href="https://2015.igem.org/Team:Nankai/Experiments">Experiments & Protocols</a></h6>
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<h6><a href="https://2015.igem.org/Team:Nankai/Results">Results</a></h6>
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<h6><a href="https://2015.igem.org/Team:Nankai/Design">Design - Pudding Health Kit</a></h6>
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                                                <p>Figure 1. Appearance and structural formula of γ-PGA.</p>
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<img src="https://static.igem.org/mediawiki/2015/b/b1/Nankai_Micro%CE%B3-PGA.jpg">
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                                                <p>Figure 2. MCS/γ-PGA mixture in solution (A). MCS/γ-PGA hydrogel (B). Microstructure of γ-PGAS/PGA hydrogel (C, D)</p>
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<img src="https://static.igem.org/mediawiki/2015/2/2a/Nankai_B.amyloliquefaciens_LL3.jpg">
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                                                <p>Figure 3. Stereoscan photograph of <em>B.amyloliquefaciens</em> LL3 strain</p>
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                                <h2>Cooperation</h2>
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                                <p>You can easily <strong>change top icons</strong> by looking at guidelines from <a rel="nofollow" href="http://fontawesome.info/font-awesome-icon-world-map/">Font Awesome</a>. Example: <strong>&lt;i class=&quot;fa fa-camera&quot;&gt;&lt;/i&gt;</strong></p>
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                                <h2>Conferences</h2>
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                                <p>Not  only can we get precious ideas from experts and other teams in conference but also broaden  our horizons on synthetic biology</p>
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                                <h2>iShare</h2>
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                                <p>iShare as  we pictured is the first step to an  all-round resource sharing platform. </p>
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    <div class="copyrights">Collect from <a href="http://www.cssmoban.com/"  title="网站模板">网站模板</a></div>
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                    <h4>Communications</h4>
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                    <p>What we have done</p>
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                            <h2>Latest Work wiht TJU iGEM team</h2>
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                            <h4>Communication and Win-win cooperation</h4>
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                    <h2>MEETING With  ZJU &amp; SYSU iGEM team</h2>
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                          <h4>Until now, we have built up the  collaboration with TJU, ZJU and SYSU. In the near future, we will further  communicate with more universities and build up collaborations. We have the  same wish for a better team! Let&rsquo;s communicate and collaborate! </h4>
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                                <img src="https://static.igem.org/mediawiki/2015/1/10/Nankai_HP_project7.jpg" alt="">
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                <h4>Cooperations</h4>
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                  <p>Let's do experiments better!          </p>
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                      <h2>Experiment materials sharing with TJU</h2>
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                      <h4>
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                        <p>This year, the igem team of Tianjin Universitiy is working on a special hydrophobin HGFII. Apart from the gene of IGFII, they also own the gene of HGFI. However, what they did is the prokaryotic expression in escherichia coli, so they lacked the conditions in eucells to test this gene. Coincidengly, there is a professor in our school which is working on the fermentation of HGFI. Hearing this, we visited his lab and successfully obtained these statistics. And finally, We support these data for their team.</p>
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                        <p>In the below are the real HPLC(High Performance Liquid Chromatography) results. From these pictures we can see that in the pure products the peak appeared at around 30 minutes while at the fermentation broth the peak appeared at aound 33 minutes.</p>
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                      </h4>
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                    <h4><P>&nbsp;</p></h4>
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                                <img src="https://static.igem.org/mediawiki/2015/9/93/Nankai_HP_project11.jpg" alt="">
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                    <h4>Conferences</h4>
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                    <p>Wilder horizons</p>
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                      <h2>The 3rd SYMPOSIUM OF BOHAI-RIM MICROBIOLOGY
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</h2>
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                            <h4><p>Dalian City, Liaoning Province</p><p><img src="https://static.igem.org/mediawiki/2015/1/15/Nankai_HP_BOHAI_RIM.jpg" alt="" width="1035" height="479" align="absmiddle"/></p> </h4>
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                    <h2>iGEM MEETUP:Peking CCiC</h2>
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                            <h4><p>Peking Univeristy, Beijing</p>
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                            <p><img src="https://static.igem.org/mediawiki/2015/5/58/Nankai_HP_PEKING_CCIC.jpg" alt="" width="1007" height="501" align="absmiddle"/></P></h4>
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                            <h4><img src="https://static.igem.org/mediawiki/2015/4/4e/Nankai_HP_Conference_Summery.jpg" alt="" width="1007" height="501" align="absmiddle"/></h4>
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                    <h4>iShare</h4>
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                    <p>Resource Sharing Platform</p>
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                      <h2><img src="https://static.igem.org/mediawiki/2015/a/a2/Nankai_HP_iShare_Info.jpg" width="261" height="71" alt=""/>iShare Introduction</h2>
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                      <h4>As we all know, iGEM has already established a functional platform for all the participators to share bio-bricks. However, the information about materials related to those Bio-bricks are still missing. These things are also important information. Where can we get these information? So we come up with the idea: iShare.</h4>
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                      <h4><img src="https://static.igem.org/mediawiki/2015/b/ba/Nankai_HP_iShare_Introduction.jpg" width="922" height="410" alt=""/></h4>
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                      <h4><img src="https://static.igem.org/mediawiki/2015/5/53/Nankai_HP_iShare_and_Get.jpg" width="1010" height="525" alt=""/></h4>
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                      <h2><img src="https://static.igem.org/mediawiki/2015/8/8d/Nankai_HP_iShare_Survey.jpg" width="241" height="66" alt=""/>iShare Survey</h2>
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                      <h4>To make iShare betetr, we sent online survey invitaions to more than 280 iGEM teams </h4>
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                      <h4><img src="https://static.igem.org/mediawiki/2015/a/a5/Nankai_HP_iShare_Survey1.jpg" width="1007" height="520" alt=""/></h4>
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                      <h4><img src="https://static.igem.org/mediawiki/2015/9/95/Nankai_HP_iShare_Survey2.jpg" width="1009" height="517" alt=""/></h4>
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                      <h4><img src="https://static.igem.org/mediawiki/2015/8/83/Nankai_HP_iShare_Survey3.jpg" width="1006" height="521" alt=""/></h4>
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                      <h2><img src="https://static.igem.org/mediawiki/2015/e/eb/Nankai_HP_iShare_Future.jpg" width="230" height="78" alt=""/>iShare Now and Futrue</h2>
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                      <h4> Now we have sent e-mails to more than 30 teams and more and more teams are joining together. What’s more, in the near future, we would like to transform iShare form a wiki to a PC software or Mobile phone App to make it more convenient for information sharing.  </h4>
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                      <h4><img src="https://static.igem.org/mediawiki/2015/7/72/Nankai_HP_iShare_Future1.jpg" width="1006" height="510" alt=""/></h4>
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Revision as of 07:12, 18 September 2015

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Your place: Home > Project > Background

Project Background

1. Pudding health kit — Wound healing hydrogel based on γ-PGA

Poly-γ-glutamic acid (γ-PGA) is a naturally occurring biopolymer that is water soluble, non-toxic, edible, and biodegradable, which has shown to promote cell migration and enhance cell adhesion. Besides, γ-PGA has been reported to prevent postsurgical tissue adhesion and the γ-PGA drug-loaded hydrogel to promote wound healing.

We prepared two types of SOD-PGA hydrogels for wound healing. γ-PGA hydrogel had high water absorption properties delivering the important moist environment. SOD released from the hydrogel maintained high enzyme activity and SOD-PGA hydrogels could scavenge the superoxide anion effectively. In vivo results showed that SOD-PGAS/PGA-H could promote collagen deposition, epithelialization, and accelerate the healing of moderately exuding wounds. Therefore, SOD-PGA hydrogels would be a good candidate for wound healing applications.Learn about more here.

2. γ-PGA producing strain — Bacillus amyloliquefaciens LL3

Strains capable for producing γ-PGA are divided into two categories based on their requirement for glutamate acid: glutamate-dependent strains and glutamate-independent strains. Glutamate-independent strains are preferable for industrial production because of their low cost and simplified fermentation process. However, compared with glutamate-dependent strains, their lower γ-PGA productivity limits their industrial application. Therefore, the construction of a glutamate-independent strain with high γ-PGA yield is important for industrial applications.

B. amyloliquefaciens strains are ubiquitous in the soil and are great reservoirs of important natural products, such as α-amylase, levansucrase, and fibrinolytic enzymes. Besides important cell factories, B. amyloliquefaciens strains are also used as plant growth-promoting and bio-control bacteria partly due to their ability to produce substances with antifungal, antibacterial and nematocidal activities. B. amyloliquefaciens LL3, isolated from fermented food, is a glutamate-independent strain, which can produce γ-PGA with sucrose as its carbon source and ammonium sulfate as its nitrogen source.

3. Methods to increase poly-γ-glutamic acid production

In this study, we aimed to improve the γ-PGA production based on the B. amyloliquefaciens NK-1 strain (a derivative of LL3 strain with its endogenous plasmid and upp gene deleted). In order to improve γ-PGA production, we employed two strategies to fine-tune the synthetic pathways and balance the metabolism in the glutamate-independent B. amyloliquefaciens NK-1 strain.

3.1 Metabolic toggle switch
Figure 4. Biosynthetic pathway of poly-γ-glutamic acid. Red arrows shows the metabolic flux towards γ-PGA synthesis. The blue arrow is the leakage of metabolic flux.

Firstly, we aimed to increase the intracellular concentration of γ-PGA precursor-- glutamate. In B. amyloliquefaciens,2-oxoglutarate is very important for the synthesis of glutamate, yet large amount of 2-oxoglutarate is consume by TCA cycle to turn into succinl-CoA in the action of enzyme ODHC (2-oxoglutarate dehydrogenase complex). Scientists had found that the activity of ODHC was rather low when glutamate was highly produced in a Corynebacterium glutamicum strain. This made us wonder, could we be able to increase the amount of intracellular glutamate by inhibiting the expression of ODHC at the stationary phase in B. amyloliquefaciens? Therefore, we constructed a metabolic toggle switch in the NK-1 strain to inhibit the expression of ODHC by adding IPTG in the stationary stage, trying to distribute the metabolic flux more frequently to be used for γ-PGA precursor-glutamate synthesis.

Figure 5. Metabolic toggle switch to regulate the expression of ODHC.

Without IPTG, the promoter Pgrac is inhibited by suppressor LacI and the supreessor XylR will not synthesized, thus the promoter Pxyl is active and odhAB genes are expressed. When IPTG is added, the xylR gene is expressed and the suppressor XylR is synthesized thereafter inhibited the expression of odhAB genes.

3.2 Replacement of promoters

Secondly, to balance the increase of endogenous glutamate production, we optimized the expression level of pgsBCA genes (responsible for γ-PGA synthesis) by replacing its native promoter with six different strength promoters.

Figure 6.Genes responsible for γ-PGA synthesis

Through these two strategies, we aimed to obtain a γ-PGA production improved mutant strain.

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