Difference between revisions of "Team:NAIT Edmonton/Desc"

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   <div id="wrap">
  
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<center><div class="top_slogan">The Project</div></center>
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 +
      <div id="nav_content">
  
<center><div class="top_slogan">Under Construction!</div></center>
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<a name="background"><h1>Background</h1></a>
 +
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<p>The structural and functional study of the proteins expressed by a genome is
  
<div class="main_content">
+
called proteomics. This relatively novel science uses different methodologies in order to
<center><img src="https://static.igem.org/mediawiki/2015/6/66/NAIT_Construction.jpg">
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<h3> Original Artist Unknown </h3>
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separate and identify specific proteins of interest. Among these techniques, SDS-PAGE
  
<style type="text/css">
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plays an essential role due to its high sensitivity, low sample volume requirement, and
.tg  {border-collapse:collapse;border-spacing:0;color:none}
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.tg td{width:280px; border-style:none;border-width:0px;overflow:hidden;word-break:normal;text-align:center;}
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.tg th{width:280px; padding:10px 5px;border-style:solid;border-width:0px;overflow:hidden;word-break:normal;text-align:center}
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high popularity. Negatively charged proteins migrate towards the positive electrode
  
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according to their size and charge. Smaller proteins migrate further in a given amount of
  
<table class="tg">
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time. As proteins are separated in this manner, users load molecular weight standards
  <tr>
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    <th class="tg-031e"><h2>Our Team</h2></th>
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    <th class="tg-031e"><h2>iGEM 2015</h2></th>
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    <th class="tg-031e"><h2>Contact Us!</h2></th>
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  </tr>
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  <tr>
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    <td class="tg-031e"><div class="roundimg"><a href="https://2015.igem.org/Team:NAIT_Edmonton/Bios" title="Team Bios"><img src="https://static.igem.org/mediawiki/2015/7/73/NAIT_Icon_clients.png" alt="" title="" /></a></div></td>
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    <td class="tg-031e"> <div class="roundimg"><a href="https://2015.igem.org" title=""><img src="https://static.igem.org/mediawiki/2015/0/05/NAIT_Icon_services.png" alt="" title="iGEM Official Site 2015" /></a></div></td>
+
    <td class="tg-031e"><div class="roundimg"><a href="https://2015.igem.org/Team:NAIT_Edmonton/ContactUs" title=""><img src="https://static.igem.org/mediawiki/2015/2/29/NAIT_Icon_contact.png" alt="" title="Contact Us" /></a></div></td>
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  </tr>
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  <tr>
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    <td class="tg-031e"><p class="centered_text">
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"When a team outgrows individual performance and learns team confidence, <strong>excellence becomes a reality</strong>." - Joe Paterno
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        </p>
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        </td>
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    <td class="tg-031e"><p class="centered_text">
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Learn about the exciting opportunities the iGEM foundation has to offer!
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        </p>
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        </td>
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    <td class="tg-031e">        <p class="centered_text">
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Please contact us if you want more information about our project or have any other questions or concerns.
+
        </p>
+
        </td>
+
  </tr>
+
  <tr>
+
    <td class="tg-031e"><a href="https://2015.igem.org/Team:NAIT_Edmonton/Bios" class="more">read more</a></td>
+
    <td class="tg-031e"><a href="https://2015.igem.org" class="more">read more</a></td>
+
    <td class="tg-031e"><a href="https://2015.igem.org/Team:NAIT_Edmonton/ContactUs" class="more">read more</a></td>
+
  </tr>
+
  
 +
to estimate the size (in kDa) of the proteins present in their sample. Once the proteins of
  
</table>
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a single sample have been isolated and are embedded in the polyacrylamide (PA) gel
     
+
 
+
  
</center>
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matrix, staining procedures are used to visualize them.</p>
  
  </div>
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<br>
  </div>
+
 
 +
<center><img src="http://upload.wikimedia.org/wikipedia/commons/4/46/SDS-PAGE_Electrophoresis.png" width="750px"></center>
 +
 
 +
<br>
 +
 
 +
<p>Organic dyes, such as Coomassie blue, can be used for this purpose;
 +
 
 +
nevertheless, their low sensitivity and a detection range that goes from 1 to 50 ng can
 +
 
 +
be a challenge for detecting low abundance proteins (Jin, Huang, Yoo, & Choi, 2006). A
 +
 
 +
higher sensitivity can be achieved by fluorescent staining techniques (from 0.1 to 10
 +
 
 +
ng.); however, UV instruments are necessary in order to read the data (Jin et al., 2006).
 +
 
 +
The most sensitive method up to date is radiolabeling, but the requirement of hazardous
 +
 
 +
isotopes and their complex management makes it a complicated procedure (Jin et al.,
 +
 
 +
2006). Silver staining is a method that offers great sensitivity and an easy to handle
 +
 
 +
protocol, thus making it one of the most commonly used staining methods. </p>
 +
 
 +
<br>
 +
 
 +
<center><img src="http://www.bio-rad.com/webroot/web/images/lsr/products/electrophoresis/product_overlay_content/global/lsr_biosafe_coomasie_gel.jpg"></center>
 +
 
 +
<br><br>
 +
 
 +
<a name="problem"><h1>The Problem </h1></a>
 +
 
 +
<p>Difficulties with silver staining arise when the molecular weight markers are re-
 +
 
 +
colored golden-brown in the staining process. Markers offer evenly distributed proteins
 +
 
 +
that show bands of equal intensity and known size. Researchers can compare these
 +
 
 +
bands with their sample and identify the protein they are looking for based on its size. A
 +
 
 +
subset of these markers has color-coded standard proteins to facilitate the identification
 +
 
 +
of each band. Post-silver staining, the users lose the ability to use the color code as a
 +
 
 +
reference.</p>
 +
 
 +
<br>
 +
 
 +
<center><img src="http://labs.mmg.pitt.edu/gjoerup/silver_stain.jpg" width="750px"></center>
 +
 
 +
<br><br>
 +
 
 +
<a name="goal"><h1>Our Goal</h1></a>
 +
 
 +
<p>Our goal is to develop a marker that, when interacting with the reagents used in
 +
 
 +
the staining protocol, will develop colour bands in specific positions so as to help in the
 +
 
 +
identification of the protein(s) of interest post-staining. In order to do so, investigation of
 +
 
 +
how specific amino acids react with silver staining reagents is underway by our team.
 +
 
 +
This will have as an outcome the creation of novel proteins that contain an excess of a
 +
 
 +
particular amino acid and/or chemical modifications that will generate a specific colour
 +
 
 +
after treating it with silver staining reagents. To obtain such proteins, the introduction of
 +
 
 +
novel nucleotide sequences into a plasmid would be done first by in vitro transcription
 +
 
 +
translation and later by transforming E. coli cells with expression vectors.</p>
 +
 
 +
<br>
 +
      </div>
 +
      <div id="nav_bar">
 +
 
 +
<li><a href="#background">Background</a><br></li>
 +
<li><a href="#problem">The Problem</a><br></li>
 +
<li><a href="#goal">Our Goal</a><br></li>
 +
 
 +
 
 +
      </div>
 +
 
 +
  </div>
  
 
   <div class="clear"></div>  
 
   <div class="clear"></div>  

Revision as of 23:17, 9 June 2015

Team NAIT 2015
The Project

Background

The structural and functional study of the proteins expressed by a genome is called proteomics. This relatively novel science uses different methodologies in order to separate and identify specific proteins of interest. Among these techniques, SDS-PAGE plays an essential role due to its high sensitivity, low sample volume requirement, and high popularity. Negatively charged proteins migrate towards the positive electrode according to their size and charge. Smaller proteins migrate further in a given amount of time. As proteins are separated in this manner, users load molecular weight standards to estimate the size (in kDa) of the proteins present in their sample. Once the proteins of a single sample have been isolated and are embedded in the polyacrylamide (PA) gel matrix, staining procedures are used to visualize them.



Organic dyes, such as Coomassie blue, can be used for this purpose; nevertheless, their low sensitivity and a detection range that goes from 1 to 50 ng can be a challenge for detecting low abundance proteins (Jin, Huang, Yoo, & Choi, 2006). A higher sensitivity can be achieved by fluorescent staining techniques (from 0.1 to 10 ng.); however, UV instruments are necessary in order to read the data (Jin et al., 2006). The most sensitive method up to date is radiolabeling, but the requirement of hazardous isotopes and their complex management makes it a complicated procedure (Jin et al., 2006). Silver staining is a method that offers great sensitivity and an easy to handle protocol, thus making it one of the most commonly used staining methods.




The Problem

Difficulties with silver staining arise when the molecular weight markers are re- colored golden-brown in the staining process. Markers offer evenly distributed proteins that show bands of equal intensity and known size. Researchers can compare these bands with their sample and identify the protein they are looking for based on its size. A subset of these markers has color-coded standard proteins to facilitate the identification of each band. Post-silver staining, the users lose the ability to use the color code as a reference.




Our Goal

Our goal is to develop a marker that, when interacting with the reagents used in the staining protocol, will develop colour bands in specific positions so as to help in the identification of the protein(s) of interest post-staining. In order to do so, investigation of how specific amino acids react with silver staining reagents is underway by our team. This will have as an outcome the creation of novel proteins that contain an excess of a particular amino acid and/or chemical modifications that will generate a specific colour after treating it with silver staining reagents. To obtain such proteins, the introduction of novel nucleotide sequences into a plasmid would be done first by in vitro transcription translation and later by transforming E. coli cells with expression vectors.