Difference between revisions of "Team:DTU-Denmark/substrate"
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<div><a class="anchor" id="section-1"></a> | <div><a class="anchor" id="section-1"></a> | ||
| − | <h2 class="h2"> | + | <h2 class="h2">Introduction</h2> |
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<span class="close Y.lMicro">×</span> | <span class="close Y.lMicro">×</span> | ||
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As seen in the table <i> Y. Lipolytica </i> is able to grow on all the waste sources we tested, while <i>S. cerevisiae</i> is only able to grow on molasses. | As seen in the table <i> Y. Lipolytica </i> is able to grow on all the waste sources we tested, while <i>S. cerevisiae</i> is only able to grow on molasses. | ||
</p> | </p> | ||
| − | + | ||
| − | + | ||
</div> <!-- /overview--> | </div> <!-- /overview--> | ||
<div><a class="anchor" id="section-2"></a> | <div><a class="anchor" id="section-2"></a> | ||
<h2 class="h2">Methods</h2> | <h2 class="h2">Methods</h2> | ||
| + | |||
| + | <p> | ||
| + | Each growth experiment (for <i> Y. Lipolytica </i> and <i>S. cerevisiae</i>) is conducted according to the following: | ||
| + | </p> | ||
| + | |||
| + | <p> | ||
| + | Minimal medium is produced as stated by Mhairi Workman<sup><a href="#references">5</a></sup> using a C-source concentration of 20 g/L was used all for growth experiments. | ||
| − | + | </p> | |
| + | |||
<p> | <p> | ||
| − | + | The cells were grown overnight in YPD medium, and prepared by spinning down and washed twice. The preculture was then used as inoculum for minimal medium (substituents) to a final concentration of 0,001 (OD600). The cultivations were carried out in a cytometer (brand) shaking 900 rpm at 30 degrees celsius. Cultures were grown, shaked and measured in 48 well microtitre plates (Cellstar). Measurements was carried out by a Hamilton Robot, (cpe201, Hamilton industries) connected to a BioTek spectrophotometer (See protocols here). OD600 Measurements were taken every 2 hours until the cultures reached stationary phase, and data was analysed using R-studio. | |
</p> | </p> | ||
| + | |||
| + | <table class="table table-bordered"> | ||
| + | <thead> | ||
| + | <tr> | ||
| + | <th>Strains</th> | ||
| + | <th>Genotype</th> | ||
| + | <th>Comment/source</th> | ||
| + | </tr> | ||
| + | </thead> | ||
| + | <tbody> | ||
| + | <tr> | ||
| + | <td><i>Y. Lipolytica</i></td> | ||
| + | <td>Wildtype</td> | ||
| + | <td>Parent strain to our laboratory bug, PO1f</td> | ||
| + | </tr> | ||
| + | <tr> | ||
| + | <td><i>S. cerevisiae</i></td> | ||
| + | <td>CEN.PK113-7D</td> | ||
| + | <td>Derived from parental strains ENY.WA-1A and MC996A,<br>and is popular for use in systems biology studies</td> | ||
| + | </tr> | ||
| + | </tbody> | ||
| + | </table> | ||
| + | |||
<h3 class="h3">Section 2.1</h3> | <h3 class="h3">Section 2.1</h3> | ||
<p> | <p> | ||
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<li>(Shusta et al. 1998)</li> | <li>(Shusta et al. 1998)</li> | ||
<li>Barth 2013</li> | <li>Barth 2013</li> | ||
| − | <li></li> | + | <li>(Mhairi Workman, Philippe Holt, 2013)</li> |
<li></li> | <li></li> | ||
<li></li> | <li></li> | ||
Revision as of 09:29, 19 October 2016
Title
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Introduction
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The dimorphic, non-conventional yeast Yarrowia lipolytica, belonging to the Ascomyceta phylum, was first isolated in 1960s from lipid-rich materials, hence the name “lipolytica”. The organism was classified and reclassified a number of times, first as Candida lipolytica, then Endomycopsis lipolytica, Saccharomycopsis lipolytica and finally Yarrowia lipolytica1. The figure shows Y. lipolytica cells under a microscope. The magnification factor is 100x.
In recent years Y. Lipolytica has received increased attention from researchers, as studies have found it to possess great potential for producing industrial enzymes and pharmaceutical proteins Biotechnological applications of Yarrowia lipolytica: Past, present and future. This potential is a result of several advantages Y. Lipolytica has over the conventional yeast S. cerevisiae. Y. Lipolytica prefer secreting proteins through the co-transcription pathway and does so very efficiently2, it does not exhibit hyperglycosylation as S. cerevisiae3. Y. Lipolytica has also been shown to exhibit excellent characteristics for the production of value-added chemicals such as a long range of organic acids and polyols Biotechnological applications of Yarrowia lipolytica: Past, present and future, and the recent introduction of several genome-scale models for Y. Lipolytica will most likely lead to more processes utilizing the chassis for production. Perhaps the most important advantage for using Y. Lipolytica over S. cerevisiae, to our project at least, is the broad substrate utilization range of Y. Lipolytica. Y. Lipolytica is known to naturally utilize alcohols (especially glycerol), acetate and hydrophobic substrates (eg. alkanes, fatty acids and oils) as carbon sources4. This has naturally lead to Y. Lipolytica becoming a model organism for several metabolic pathways, especially fatty acid transport and metabolism, and single cell oil (SCO) accumulation. Y. Lipolytica has even been shown to exhibit enhanced growth on mixed substrates Yarrowia lipolytica as an oleaginous cell factory platform for production of fatty acid-based biofuel and bioproducts, which renders it ideal for utilization of industrial waste streams due to the highly diverse content of these. These findings had us believe that we had found an excellent candidate chassis for our project. The table shows a comparison of the substrate range of Y. Lipolytica W29 and S. cerevisiae CEN.PK113-7D.
| Y. Lipolytica | S. cerevisiae | |
|---|---|---|
| Sediment from canola oil production | µ = 0.31 | None |
| Glycerol from Perstop | µ = 0.27 | None |
| Glycerol from Emmelev | µ = 0.45 | None |
| Glycerol from Daka | µ = 0.31 | None |
| Molasses from Dansukker | µ = 0.42* | µ = 0.47 |
* it should be noted that the molasses was autoclaved thus degrading some of the sucrose content. This growth might not be possible to replicate with untreated molasses.
As seen in the table Y. Lipolytica is able to grow on all the waste sources we tested, while S. cerevisiae is only able to grow on molasses.
Methods
Each growth experiment (for Y. Lipolytica and S. cerevisiae) is conducted according to the following:
Minimal medium is produced as stated by Mhairi Workman5 using a C-source concentration of 20 g/L was used all for growth experiments.
The cells were grown overnight in YPD medium, and prepared by spinning down and washed twice. The preculture was then used as inoculum for minimal medium (substituents) to a final concentration of 0,001 (OD600). The cultivations were carried out in a cytometer (brand) shaking 900 rpm at 30 degrees celsius. Cultures were grown, shaked and measured in 48 well microtitre plates (Cellstar). Measurements was carried out by a Hamilton Robot, (cpe201, Hamilton industries) connected to a BioTek spectrophotometer (See protocols here). OD600 Measurements were taken every 2 hours until the cultures reached stationary phase, and data was analysed using R-studio.
| Strains | Genotype | Comment/source |
|---|---|---|
| Y. Lipolytica | Wildtype | Parent strain to our laboratory bug, PO1f |
| S. cerevisiae | CEN.PK113-7D | Derived from parental strains ENY.WA-1A and MC996A, and is popular for use in systems biology studies |
Section 2.1
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$$x = {-b \pm \sqrt{b^2-4ac} \over 2a}.$$
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Section 2.2
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Section 2.3
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Section 3
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Section 4
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Section 5
Has ut facer debitis, quo eu agam purto. In eum justo aeterno. Sea ut atqui efficiantur, mandamus deseruisse at est, erat natum cum eu. Quot numquam in vel. Salutatus euripidis moderatius qui ex, eu tempor volumus vituperatoribus has, ius ea ullum facer corrumpit.
Section 6
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