Difference between revisions of "Team:Austin UTexas/Demonstrate"

 
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<h2> Project Description </h2>
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<h2> Demonstrate </h2>
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<p>For the gold medal “Demonstrate your work” requirement, we have shown that we can recreate kombucha from scratch by adding isolated strains of microbes to tea media. Our tea media, made with water, black tea, and sucrose, simulates the starting mixture used to brew kombucha. We have performed extensive recapitulation trials to determine which strains of yeast and bacteria are necessary for brewing kombucha. Cataloguing these vital strains is a necessary step toward modifying the starting population to create a “designer beverage” with a variety of properties that could benefit kombucha consumers and manufacturers outside the lab. </p>
<img src="https://static.igem.org/mediawiki/2016/6/6d/T--Austin_UTexas--Timeline.png" style="width:100%">
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<p>Click the images below to learn more about our results!</p>
<h3>Gold Medal Part Characterization</h3>
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<p>The characterization of the BioBrick P-atp2 from the <a href="https://2015.igem.org/Team:BIT-China/Parts">BIT-China-2015</a> team was done to see if P-atp2 could be utilized as a basic pH sensor. The results are found <a href="https://2016.igem.org/Team:Austin_UTexas/Results">here</a> and on the iGEM Registry page under experience, <a href="http://parts.igem.org/Part:BBa_K1675021">BBa_K1675021</a></p>
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<h3>Our Project</h3>
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<p> Kombucha is a beverage made when a symbiotic community of bacteria and yeast ferments sugared tea. Although kombucha has been consumed for thousands of years in the East, the drink has enjoyed a recent resurgence in popularity [REFERENCE-HOMEPAGE]. Several kombucha breweries operate in Austin, Texas, our team’s hometown. The role microbes play in the production of the beverage has led our team to wonder if synthetic biology could allow us to create “designer kombucha” with enhanced properties, such as more appealing flavors or additional nutrients. In order to do so, our team attempted to isolate the strains responsible for the fermentation of kombucha, identify them, genetically modify them, and add the individual strains into tea media to recreate the drink. We additionally considered potential applications of the ability to genetically modify the microbial population of kombucha, such as reducing the ethanol content of the beverage and improving taste with brazzein, a sweet-tasting protein. AS PART OF OUR HUMAN PRACTICES WE.... [SOMETHING HERE about GMO concerns and alternative direction(s)?]  </p>
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<p>Click the images below to learn more about our project!</p>
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<input type="image" src="https://static.igem.org/mediawiki/2016/f/f7/T--Austin_UTexas--BrazzButton.png" style="width:100%;" onclick="showOne('section5')" /><br><br><br><p>Brazzein</p>
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<input type="image" src ="https://static.igem.org/mediawiki/2016/e/e7/T--Austin_UTexas--pHNavi.png" style="width:100%;" onclick="showOne('section6')" /><p>pH</p>
 
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<input type="image" src ="https://static.igem.org/mediawiki/2016/e/e7/T--Austin_UTexas--pHNavi.png" style="width:100%;" onclick="showOne('section6')" /><p>pH Sensors</p>
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<input type="image" src ="https://static.igem.org/mediawiki/2016/9/92/T--Austin_UTexas--GellanNavi.png" style="width:100%;" onclick="showOne('section7')" /><p>Gellan Gum</p>
 
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<h2> Kombucha Strains </h2>
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<h2>Kombucha Strains</h2>  
<p> One of the earliest goals of our project was to identify a specific set of microbes responsible for the production of kombucha. To do this, samples of store-bought kombucha were plated onto a variety of media with various dilutions to isolate microbes. Then, morphologically different colonies were cultured and frozen in glycerol for further use. Once we obtained a collection of microbial isolates, each microbe was sequenced and identified using polymerase chain reaction (PCR) to amplify a particular ribosomal RNA gene. The 16S gene was selected for bacterial strains, and the ITS gene was amplified for the fungal samples.<sup>1</sup> After the samples were sequenced, we utilized the <a href="http://rdp.cme.msu.edu/seqmatch/seqmatch_intro.jsp">Ribosomal Database Project (RDP) SeqMatch Tool</a> to identify our isolated species of bacteria and yeast. By identifying these kombucha strains, we were able to use our own experimentally isolated strains for our future kombucha experiments.
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<h3>References</h3>
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<ol type="1">
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*Successfully isolated microbes from various samples of kombucha.
<li>Marsh, A. J., O'Sullivan, O., Hill, C., Ross, R. P., and Cotter, P. D. (2014) Sequence-based analysis of the bacterial and fungal compositions of multiple kombucha (tea fungus) samples. Food Microbiology.
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*Identified strains of bacteria and yeast using rRNA gene sequencing.
</li>
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*Characterized each of the isolated microbes to facilitate further experimentation.  
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<a href ="https://2016.igem.org/Team:Austin_UTexas/Results#section1">Results</a> (May need to open in a new tab.)
 
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<h2> Conjugation </h2>
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<h2>Conjugation</h2>  
<p> In order to demonstrate that we can genetically engineer the bacterial strains that we identified, <i>Gluconobacter oxydans</i> and <i>Gluconacetobacter xylinus</i>, we attempted to conjugate various plasmids encoding fluorescent devices, such as GFP and Crimson, into these bacteria using a DAP (Diaminopimelic Acid) auxotroph strain of <i>E. coli</i> [REFERENCES]. To assist in this process, we also conducted minimal inhibitory concentration studies with each of these bacteria using [THESE ANTIBIOTICS]. Ultimately, [BLAH BLAH BLAH]. The plasmid, pBTK520, contains GFP and a spectinomycin resistance gene. Once the bacteria are successfully conjugated we can.... [BLAH BLAH BLAH].
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*Attempted conjugation with <i>G. oxydans</i>.
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*Performed minimum inhibitory concentration experiments between <i>G. oxydans</i> and spectinomycin, carbenicillin and kanamycin.
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*Determined that <i>G. oxydans</i> is resistant to spectinomycin and carbenicillin.
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<a href = "https://2016.igem.org/Team:Austin_UTexas/Results#section2">Results </a> (May need to open in a new tab.)
 
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<h2>Recapitulation </h2>
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<h2>Recapitulation</h2>
<p>One of the primary focuses of our project is to study the nature of the symbiotic community of fermenting kombucha. Recapitulation refers to the reformation of kombucha by singly adding isolated microbes to a mixture of black tea, sucrose, and water similar to the mixture used in home-brewing practices. Through this process we determined that the microbial community could be recreated from its constituent bacteria and yeast. We also identified the microbes that appear to be vital for the proper recapitulation of kombucha. However, because we cannot taste our lab-brewed kombucha, these conclusions are solely based on qualitative observations. Successful recapitulations indicate that it is in fact possible to produce kombucha with known microbes rather then simply propagating new kombucha from a previous batch. These results elucidate the symbiotic relationships that must exist in order for kombucha to form. Future research may allow us to create kombucha with distinct flavor profiles by varying the combination of strains added to the brew. <p>
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*In a process called "recapitulation," we successfully created a kombucha-like culture by adding individual strains of microbes instead of a living culture containing the entire kombucha microbiome.
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*Determined that the microbe <i>Ga. hansenii</i> is essential for the fermentation of kombucha.
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*Determined that two distinct strains of the yeast <i>Lachancea fermentati</i> are necessary for the fermentation of kombucha, including one that appears to produce high quantities of C02.
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<a href = "https://2016.igem.org/Team:Austin_UTexas/Results#section3">Results </a> (May need to open in a new tab.)
 
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<h2> Ethanol </h2>
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<h2>Ethanol</h2>
<P> During the fermentation process, yeast in kombucha produce ethanol, the type of alcohol present in beer, wine, and other alcoholic beverages. This presents a challenge to kombucha brewers who wish to market their product as a non-alcoholic beverage. If the alcohol content of a manufacturer’s kombucha exceeds 0.5% at any point during production, the manufacturer may not market their beverage as non-alcoholic and must be regulated as a producer of alcoholic beverages.<sup>1</sup> One way to tackle this problem with synthetic biology is to ferment with yeast that produce less ethanol. However, this may be impractical. Some bacteria in the SCOBY oxidize ethanol produced by the yeast to produce acetic acid, which is a major component of the beverage’s distinctive, tart flavor. </p>
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<p>Another approach is to increase the rate at which the bacteria convert the ethanol to acetic acid. Two enzymes are responsible for this process: an alcohol dehydrogenase and an aldehyde dehydrogenase.<sup>2</sup> Using Golden Gate assembly, we plan to assemble a construct containing the coding sequences for these genes and insert the construct into <i>Gluconacetobacter hansenii</i>, an acetic acid-producing bacterium similar to those found in kombucha. Then, we plan to recapitulate kombucha with both the transformed and control <i>Ga. hansenii</i> to evaluate the ethanol content over the course of the fermentation with gas chromatography-mass spectrometry. We also plan to determine whether increasing the acetic acid production will lead to a pH change that could affect the flavor of the beverage by testing the pH and observing the cultures for visible differences. If we are able to create a microbial community that results in a lower ethanol content within the kombucha during fermentation, kombucha brewers could use the modified bacterium to help ensure the ethanol content of their product stays below the legal limit.
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<h3>References</h3>
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*Found literature describing sequences for genes involved in the metabolism of ethanol to acetic acid in the bacterium <i>Ga. hansenii</i>.
<li>Alcohol and Tobacco Tax and Trade Bureau. Kombucha Information and Resources. 2016. https://www.ttb.gov/kombucha/kombucha-general.shtml</li>
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*Designed Golden Gate parts for the assembly of these genes into a functional construct.
<li>Mamlouk, D., and Gullo, M. (2013) Acetic Acid Bacteria: Physiology and Carbon Sources Oxidation. <i>Indian Journal of Microbiology</i> 53, 377–384.</li>
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*Used a bromothymol blue assay to compare changes in pH resulting from fermentation in multiple strains of <i>Lachancea fermentati</i> isolated from our kombucha.
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<a href = "https://2016.igem.org/Team:Austin_UTexas/Results#section4">Results </a>( May need to open in a new tab.)
 
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<h2> Brazzein </h2>
 
<P> One of the potential methods to create designer kombucha is to add a brazzein gene into the bacterial strains. Brazzein, a protein found in the pulp of the edible fruit of the African plant <i>Pentadiplandra brazzeana Baill</i>, is an extremely sweet substance<sup>1</sup>. It is 2,000 times sweeter than sucrose by weight. This makes it a healthy and economical alternative to sugar.  Commercial production of brazzein is limited, however, because it comes from a tropical plant. If it could be more easily harvested, it could be used to improve the flavor of various foods and drinks, including kombucha. By genetically engineering the brazzein gene into the bacteria in kombucha, the drink could be sweetened without adding sugar or excessive calories.  While still being a GMO product, this beverage would be low in sugar and could appeal to a health-conscious consumer.</p>
 
  
<h3>References</h3>
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<h2>pH Sensors</h2>
<li>Yan, Sen et al. “Expression of Plant Sweet Protein Brazzein in the Milk of Transgenic Mice.” Ed. Xiao-Jiang Li. PLoS ONE 8.10 (2013): e76769. </li>
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<li>Brazzein protein structure acquired from European Bioinformatics Institute </li>
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*Successfully created a neutral pH sensor with a reporter.
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*Further characterized the P-atp2 Biobrick.
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*Found literature describing three putative promoters in <i>Gluconobacter oxydans</i> that increase transcription under acidic conditions, and currently characterizing these sequences.
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<a href = "https://2016.igem.org/Team:Austin_UTexas/Results#section6">Results</a> (May need to open in a new tab.)
 
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<h2> pH Sensors </h2>
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<h2>Gellan Gum</h2>
<p>Many of the microorganisms involved in the fermentation of kombucha produce acidic metabolites that lower the pH of the culture. Using pH-sensitive promoters to control the expression of reporter proteins, such as GFP or a chromoprotein, would allow visualization of the pH change. The promoters Cpx, P-atp2, and Cadc were selected as pH sensors to indicate pH in the neutral, basic, and acidic ranges, respectively.<sup>1,3,5,6</sup> These constructs have been or will be transformed into <i>Escherichia coli</i> to confirm pH sensitivity prior to introduction to kombucha and to see if these constructs could be utilized as sensors in mediums besides kombucha.</p>
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<p>Modification of <i>Gluconobacter oxydans</i>, a bacterium in kombucha, is also planned to avoid disturbing the kombucha microbiome. Three endogenous upstream regions of loci that were reported to show increased mRNA synthesis as pH decreased were obtained.<sup>2</sup> Golden Gate assembly is currently being used to quickly assemble these promoters upstream of Venus (pYTK033).<sup>4</sup> Once successful, these pH-sensitive promoters with different reporters will be used to visualize the different members of the kombucha microbiome overtime.</p>
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<h3>References</h3>
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<ol type="1">
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* Successfully made Gellan Gum plates from <i>Sphingomonas paucimobilis</i>
<html><li><a href="https://2015.igem.org/Team:BIT-China/Parts">BIT-China-2015</a></li></html>
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* Successfully grew other bacteria on the Gellan Gum plates
<li>Hanke, T., Richhardt, J., Polen, T., Sahm, H., Bringer, S., and Bott, M. (2012) Influence of oxygen limitation, absence of the cytochrome bc1 complex and low pH on global gene expression in Gluconobacter oxydans 621H using DNA microarray technology. <i>Journal of Biotechnology 157</i>, 359–372.</li>
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* Shared this DIY technology with the Texas Tech iGEM team
<li>Kuper, C., and Jung, K. (2005) CadC-mediated activation of the cadBA promoter in Escherichia coli. <i>Journal of Molecular and Microbiological Biotechnology 1</i>, 26–39.</li>
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<li>Lee ME, DeLoache, WC A, Cervantes B, Dueber, JE. (2015) A Highly-characterized Yeast Toolkit for Modular, Multi-part Assembly. <i>ACS Synthetic Biology 4</i> 975-986</li>
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<a href = "https://2016.igem.org/Team:Austin_UTexas/Results#section7">Results </a> (May need to open in a new tab.)
<li>Nakayama, S.-I., and Watanabe, H. (1998) Identification of cpxR as a Positive Regulator Essential for Expression of the Shigella sonnei virF Gene. <i>Journal of Bacteriology 180</i>, 3522–3528.</li>
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<li>Nakayama, S.-I., and Watanabe, H. (1995) Involvement of cpxA, a Sensor of a Two-Component Regulatory System, in the pH-Dependent Regulation of Expression of Shigella sonnei virF Gene. <i>Journal of Bacteriology 177</i>, 5062–5069.</li>
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<p>Tell us about your project, describe what moves you and why this is something important for your team.</p>
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<h5>What should this page contain?</h5>
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<li> A clear and concise description of your project.</li>
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<li>A detailed explanation of why your team chose to work on this particular project.</li>
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We encourage you to put up a lot of information and content on your wiki, but we also encourage you to include summaries as much as possible. If you think of the sections in your project description as the sections in a publication, you should try to be consist, accurate and unambiguous in your achievements.
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Judges like to read your wiki and know exactly what you have achieved. This is how you should think about these sections; from the point of view of the judge evaluating you at the end of the year.
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<p>See how other teams have described and presented their projects: </p>
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<li><a href="https://2014.igem.org/Team:Imperial/Project"> Imperial</a></li>
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<li><a href="https://2014.igem.org/Team:UC_Davis/Project_Overview"> UC Davis</a></li>
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<li><a href="https://2014.igem.org/Team:SYSU-Software/Overview">SYSU Software</a></li>
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<h2>Kombucha Strains</h2>  
  
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*Identified strains of bacteria and yeast using rRNA gene sequencing.
 
*Identified strains of bacteria and yeast using rRNA gene sequencing.
 
*Characterized each of the isolated microbes to facilitate further experimentation.  
 
*Characterized each of the isolated microbes to facilitate further experimentation.  
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<a href = "https://2016.igem.org/Team:Austin_UTexas/Results#section1">Results </a>
 
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<h2>Recapitulation</h2>
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<h2>Conjugation</h2>  
  
 
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*In a process called "recapitulation," we successfully created a kombucha-like culture by adding individual strains of microbes instead of a living culture containing the entire kombucha microbiome.
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*Attempted conjugation with <i>G. oxydans</i>.
*Determined that the microbe <i>Ga. hansenii</i> is essential for the fermentation of kombucha.
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*Performed minimum inhibitory concentration experiments between <i>G. oxydans</i> and spectinomycin, carbenicillin and kanamycin.
*Determined that two distinct strains of the yeast <i>Lachancea fermentati</i> are necessary for the fermentation of kombucha, including one that appears to produce high quantities of C02.
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*Determined that <i>G. oxydans</i> is resistant to spectinomycin and carbenicillin.
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<h2>Recapitulation</h2>
<h2>Conjugation</h2>  
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*Attempted conjugation with <i>G. oxydans</i>.
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*In a process called "recapitulation," we successfully created a kombucha-like culture by adding individual strains of microbes instead of a living culture containing the entire kombucha microbiome.
*Performed minimum inhibitory concentration experiments between <i>G. oxydans</i> and spectinomycin, carbenicillin and kanamycin.
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*Determined that the microbe <i>Ga. hansenii</i> is essential for the fermentation of kombucha.
*Determined that <i>G. oxydans</i> is resistant to spectinomycin and carbenicillin.
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*Determined that two distinct strains of the yeast <i>Lachancea fermentati</i> are necessary for the fermentation of kombucha, including one that appears to produce high quantities of C02.
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<h2>Ethanol</h2>
 
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*Designed Golden Gate parts for the assembly of these genes into a functional construct.
 
*Designed Golden Gate parts for the assembly of these genes into a functional construct.
 
*Used a bromothymol blue assay to compare changes in pH resulting from fermentation in multiple strains of <i>Lachancea fermentati</i> isolated from our kombucha.
 
*Used a bromothymol blue assay to compare changes in pH resulting from fermentation in multiple strains of <i>Lachancea fermentati</i> isolated from our kombucha.
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*Further characterized the P-atp2 Biobrick.
 
*Further characterized the P-atp2 Biobrick.
 
*Found literature describing three putative promoters in <i>Gluconobacter oxydans</i> that increase transcription under acidic conditions, and currently characterizing these sequences.
 
*Found literature describing three putative promoters in <i>Gluconobacter oxydans</i> that increase transcription under acidic conditions, and currently characterizing these sequences.
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Latest revision as of 00:48, 20 October 2016

Demonstrate

For the gold medal “Demonstrate your work” requirement, we have shown that we can recreate kombucha from scratch by adding isolated strains of microbes to tea media. Our tea media, made with water, black tea, and sucrose, simulates the starting mixture used to brew kombucha. We have performed extensive recapitulation trials to determine which strains of yeast and bacteria are necessary for brewing kombucha. Cataloguing these vital strains is a necessary step toward modifying the starting population to create a “designer beverage” with a variety of properties that could benefit kombucha consumers and manufacturers outside the lab.

Click the images below to learn more about our results!

Kombucha Strains

Conjugation

Recapitulation

Ethanol

pH

Gellan Gum