Difference between revisions of "Team:IISc Bangalore/Description"

 
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{{Template:IISc Bangalore/projectSidebar.css}}
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{{Template:IISc_Bangalore/fontawesome.css}}
{{Template:IISc Bangalore/projectSidebar.js}}
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{{Template:IISc_Bangalore/style.css}}
{{Template:IISc Bangalore/projectBoxes.css}}
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{{Template:IISc_Bangalore/sidebar.css}}
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{{Template:IISc_Bangalore/description.css}}
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{{Template:IISc_Bangalore/animate.css}}
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{{Template:IISc_Bangalore/hover.css}}
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{{Template:IISc_Bangalore/accordian.css}}
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{{Template:IISc_Bangalore/sidebar.js}}
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{{Template:IISc_Bangalore/anijs.js}}
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<html>
 
<html>
  <head>
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<head>
    <meta charset="utf-8">
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<title>Team IISc iGem</title>
  <meta name="viewport" content="width=device-width, initial-scale=1">
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  <link rel="stylesheet" href="http://maxcdn.bootstrapcdn.com/bootstrap/3.3.7/css/bootstrap.min.css">
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  <link rel="stylesheet" type="text/css" href="bootstrap-3.3.7-dist/css/bootstrap.min.css">
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  <link rel="stylesheet" type="text/css" href="bootstrap-3.3.7-dist/css/bootstrap.min.css.map">
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  <link rel="stylesheet" type="text/css" href="bootstrap-3.3.7-dist/css/bootstrap-theme.min.css.map">
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  <link rel="stylesheet" type="text/css" href="bootstrap-3.3.7-dist/css/bootstrap-theme.min.css">
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  <link rel="stylesheet" type="text/css" href="content5.css">
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  <link rel="stylesheet" type="text/css" href="sidebar5.css">
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  <link rel="stylesheet" type="text/css" href="boxes6.css">
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  <style type="text/css">
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  @font-face {
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      font-family: "Montserrat";
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      src: url(fonts/Monteserrat/Montserrat-Regular.ttf) format("truetype");
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  }
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  /*p.customfont {
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      font-family: "My Custom Font", Verdana, Tahoma;
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  }*/
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  </style>
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    <!-- <link rel="stylesheet" type="text/css" href="navbar5.css"> -->
+
  <!-- <script src="https://use.fontawesome.com/29ffc57809.js"></script> -->
+
  
 +
<link rel='stylesheet prefetch' href='http://netdna.bootstrapcdn.com/font-awesome/4.2.0/css/font-awesome.css'>
  
  <link href="http://fonts.googleapis.com/css?family=Montserrat" rel="stylesheet" type="text/css">
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<link rel="stylesheet" href="http://anijs.github.io/lib/anicollection/anicollection.css" />
  <link href="http://fonts.googleapis.com/css?family=Lato" rel="stylesheet" type="text/css">
+
  <link rel="stylesheet" type="text/css" href="bootstrap-3.3.7-dist/fonts/glyphicons-halflings-regular.woff">
+
  
 +
 +
<meta name="viewport" content="width=device-width, initial-scale=1">
 +
  <link rel="stylesheet" href="https://maxcdn.bootstrapcdn.com/bootstrap/3.3.7/css/bootstrap.min.css">
 
   <script src="https://ajax.googleapis.com/ajax/libs/jquery/1.12.4/jquery.min.js"></script>
 
   <script src="https://ajax.googleapis.com/ajax/libs/jquery/1.12.4/jquery.min.js"></script>
   <script src="http://maxcdn.bootstrapcdn.com/bootstrap/3.3.7/js/bootstrap.min.js"></script>
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   <script src="https://maxcdn.bootstrapcdn.com/bootstrap/3.3.7/js/bootstrap.min.js"></script>
  <script src="sidebar5.js"></script>
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 +
<link href="css/bootstrap.css" rel="stylesheet" type="text/css" media="all">
 +
<link rel="stylesheet" href="https://maxcdn.bootstrapcdn.com/bootstrap/3.3.7/css/bootstrap.min.css" integrity="sha384-BVYiiSIFeK1dGmJRAkycuHAHRg32OmUcww7on3RYdg4Va+PmSTsz/K68vbdEjh4u" crossorigin="anonymous">
 +
<script src="https://use.fontawesome.com/fce310c82d.js"></script>
 +
 
 +
<script src="js/jquery-1.11.0.min.js"></script>
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<script type="text/javascript" src="js/bootstrap.js"></script>
  
  </head>
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<link href="css/style.css" rel="stylesheet" type="text/css" media="all"/>
  <body data-spy="scroll" data-target="#sidebar">
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<link rel="stylesheet" href="css/flexslider.css" type="text/css" media="screen" />
  
 +
<meta name="viewport" content="width=device-width, initial-scale=1">
 +
<meta http-equiv="Content-Type" content="text/html; charset=utf-8" />
 +
<script type="application/x-javascript"> addEventListener("load", function() { setTimeout(hideURLbar, 0); }, false); function hideURLbar(){ window.scrollTo(0,1); }>
 +
</script>
 +
<meta name="keywords" content="Team IISc igem" />
 +
<!--Google Fonts-->
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<link href="css/font-awesome.min.css" rel="stylesheet" type="text/css" media="all" />
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<link href='//fonts.googleapis.com/css?family=Roboto:400,700' rel='stylesheet' type='text/css'>
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<link href="https://fonts.googleapis.com/css?family=Bitter" rel="stylesheet">
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<link href="https://fonts.googleapis.com/css?family=Varela+Round" rel="stylesheet">
 +
<!--JS for animate-->
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<link href="css/animate.css" rel="stylesheet" type="text/css" media="all">
  
  
    <!-- <span >
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<!-- here are mine -->
<svg class="panel" onclick="openBar()" enable-background="new 0 0 128 128" height="40px" id="Layer_1" version="1.1" viewBox="0 0 128 128" width="40px" xml:space="preserve" xmlns="http://www.w3.org/2000/svg" xmlns:xlink="http://www.w3.org/1999/xlink"><g><g><path d="M64,0C28.656,0,0,28.656,0,64s28.656,64,64,64s64-28.656,64-64S99.344,0,64,0z M64,120    C33.125,120,8,94.875,8,64S33.125,8,64,8s56,25.125,56,56S94.875,120,64,120z" fill="#B0BEC5"/></g></g><g><g><path d="M96,56H72V32c0-4.414-3.586-8-8-8s-8,3.586-8,8v24H32c-4.414,0-8,3.586-8,8s3.586,8,8,8h24v24    c0,4.414,3.586,8,8,8s8-3.586,8-8V72h24c4.414,0,8-3.586,8-8S100.414,56,96,56z" fill="#8BC34A"/></g></g></svg>
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<link rel="stylesheet" href="sidebar.css">
    </span> -->
+
<link rel="stylesheet" href="description.css">
      <nav class="navbar navbar-fixed-top text-center navbar-inverse">
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<link rel="stylesheet" href="hover.css" >
 +
<script src="sidebar.js"></script>
 +
</head>
 +
<body>
 +
<!--banner start here-->
 +
<!-- <div class="banner">
 +
  <div class="container"> -->
 +
<nav class="navbar navbar-fixed-top text-center navbar-inverse">
 
         <div class="container-fluid">
 
         <div class="container-fluid">
 
         <div class="navbar-header">
 
         <div class="navbar-header">
          <button type="button" class="navbar-toggle" data-toggle="collapse" data-target="#myNavbar">
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  </div>
        <span class="icon-bar"></span>
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        <span class="icon-bar"></span>
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        <span class="icon-bar"></span>
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      </button>
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          <a class="navbar-brand panel" onclick="openBar()" href="#" >On this page <span class="glyphicon glyphicon-th
+
"></span></a> </div>
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         <div class="collapse navbar-collapse" id="myNavbar">
 
         <div class="collapse navbar-collapse" id="myNavbar">
 
         <ul class="nav navbar-nav">
 
         <ul class="nav navbar-nav">
           <li class="active"><a href="#">Home</a></li>
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           <li class="hvr-underline-from-left"><a href="https://2016.igem.org/Team:IISc_Bangalore">Home</a></li>
           <li><a href="#">Team</a></li>
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           <li class="hvr-underline-from-left"><a href="https://2016.igem.org/Team:IISc_Bangalore/Team">Team</a></li>
          <li><a href="#">Project</a></li>
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           <li><a href="#">Parts</a></li>
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           <li><a href="#">Safety</a></li>
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<li class="dropdown"><a class="dropdown-toggle" data-toggle="dropdown" href="#">Project </a>
           <li><a href="#">Attributions</a></li>
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        <ul class="dropdown-menu">
          <li><a href="#">Practices</a></li>
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           <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Description">Description</a></li>
           <li><a href="#">Awards</a></li>
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           <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Experiments">Experiments</a></li>
 +
           <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Results">Results</a></li>
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Notebook">Notebook</a></li>
 +
           <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Safety">Safety</a></li>
 
         </ul>
 
         </ul>
 +
      </li>
 +
 +
 +
<li class="hvr-underline-from-left"><a href="https://2016.igem.org/Team:IISc_Bangalore/Parts">Parts</a></li>
 +
 +
                <li class="hvr-underline-from-left"><a href="https://2016.igem.org/Team:IISc_Bangalore/Collaborations">Collaborations</a></li>
 +
        <li class="hvr-underline-from-left"><a href="https://2016.igem.org/Team:IISc_Bangalore/Attributions">Attributions</a></li>
 +
       
 +
<li class="dropdown"><a class="dropdown-toggle" data-toggle="dropdown" href="#">Human Practices</a>
 +
        <ul class="dropdown-menu">
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Human_Practices">Human Practices</a></li>
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/HP/Silver">HP Silver</a></li>
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/HP/Gold">HP Gold</a></li>
 +
        </ul>
 +
      </li>
 +
 +
        <li class="hvr-underline-from-left"><a href="https://2016.igem.org/Team:IISc_Bangalore/InterLab">InterLab</a></li>
 +
<li class="dropdown"><a class="dropdown-toggle" data-toggle="dropdown" href="#">Special Prizes</a>
 +
      <ul class="dropdown-menu">
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Integrated_Practices">Integrated Human Practices</a></li>
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Engagement">Education and Public Engagement</a></li>
 +
          <li class="active"><a href="https://2016.igem.org/Team:IISc_Bangalore/Model">Model</a></li>
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Measurement">Measurement</a></li>
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Entrepreneurship">Entrepreneurship</a></li>
 +
          <li><a href="https://2016.igem.org/Team:IISc_Bangalore/Design">Applied Design</a></li>
 +
        </ul>
 +
      </li>
 +
        </ul>
 +
 
       </div>
 
       </div>
  
 
       </div>
 
       </div>
 
       </nav>
 
       </nav>
      <!-- <div class="container"> -->
 
      <div  id="sidebar" class="sidebar">
 
  
        <a href="javascript:void(0)" class="closebtn" onclick="closeBar()">&times;</a>
 
        <a class="nav" href="#overview">Contents</a>
 
        <!-- <a class="nav" href="#design">Design</a> -->
 
        <!-- <a class="nav" href="#protein">Protein</a> -->
 
        <!-- <a class="nav" href="#aggre">Aggregation</a> -->
 
        <a class="nav" href="#ref">References</a>
 
        <a class="nav" href="#top">Back to top</a>
 
  
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          <p class="whitef">With the advent of rDNA technology in the late 1970s, medicine, agriculture and several other areas underwent a quantum leap</span><br>
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      <h4>Bioreactor design</h4>
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        As stated in the introduction, our project is an attempt to modify E coli to lower capital and running costs for rDNA bioreactor systems, by automating protein over-expression induction and separation of cell from growth media.
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To learn more about the existing biotech infrastructure in India, we decided to visit some biotech parks in India and explore the feasibility and applicability of our idea.
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      <h4>Protein production module</h4>
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<div class="content">Induction synthesis of protein of interest is another important step.
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        <h1>Overview</h1>
+
      <h4>Auto-aggregation</h4>
        <p>Since the advent of rDNA technology in the late 1970s, the use of recombinant protein has been on the rise, starting from insulin and hormones all the way through to monoclonal antibodies and one hundred and fifty-one FDA approved protein based recombinant pharmaceuticals by the year 2009<a href="#bull1" onclick="closeBar()">[1]</a>. Despite being in high demand, recombinant proteins have heavy price tags, thanks to the significant manufacturing costs. One of the important steps in the manufacturing process is Centrifugation but on an industrial scale, it is an economic nightmare. <a href="#bull2" onclick="closeBar()">[2]</a> Further, existing industrial setups use complex sensors to monitor cell density to determine the point at which to begin separation of the cells from the cell culture. One can immediately see the humongous relief that would be associated with finding a way to deal with the above problems. Hence, we came up with the idea of our project, the Cellfifuge.
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     </div>
 +
<div class="content">
 +
          <p class="whitef">To achieve cellular aggregation, we use the famous auto-transporter protein, Antigen43 (Ag43).
 +
      <br><a href="#refer4" onclick="closeTab()"><span class="readm hvr-ripple-out">Read more</span></a>
 +
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        <h1>Our Bioreactor Design</h1>
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        <p>We realized that manufacturing units use expensive and energy expensive machinery <a href="#bull3" onclick="closeBar()">[3]</a>. Hence, we engineered our bacteria in such a way that it could do most of the work done by these monstrous machines so that we no longer have to buy them and pay their bills. To increase the yield of the product, we came up with the idea of separating cell growth and target protein production so that when the cells have grown up to a high enough cell density, they shuttle all their energy towards the required protein production.<a href="#bull4" onclick="closeBar()">[4]</a> Based on the above ideas, we came up with the design of our bioreactor. (Figure 1)
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<h3>Overview</h3>
 +
</div>
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<div class="row">
 +
<div class="refer col-md-6">
 +
With the advent of rDNA technology in the late 1970s, medicine, agriculture and several other areas underwent a quantum leap and from that point, progress only hastened, from one only one recombinant pharmaceutical  approved for human use (insulin) in 1982 to one hundred and fifty-one FDA approved protein based recombinant pharmaceuticals by 2009<a href="#refer" onclick="closeTab()">[1]</a>.
 +
Despite being in high demand (due to the fact that most recombinant products produced on an industrial scale are therapies for chronic diseases like cancer and diabetes), recombinant products are expensive due to several factors like long and expensive development time, high failure rate (~80%) of the products developed, manufacturing costs requiring expensive technologies and processes (bioreactors, column chromatography, sterile conditions, etc) and the involvement of skilled labor on both the manufacturing and the healthcare provider’s side<a href="#refer" onclick="closeTab()">[2]</a>. Treatments with these pharmaceuticals can cost from around 10,000 to 100,000 € per year for a single patient[2]. As scientists and engineers, it seems obvious that our contribution can be most easily and effectively be made at the level of manufacturing costs; to try to bring down the cost of these life-saving products.
 +
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 +
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 +
<div class="row">
 +
<div class="refer col-md-6">
 +
<p class="whitef leftMove"></html>[[File:Flowchart iisc.jpg|right]]<html>We realized that manufacturing units use expensive and energy expensive machinery <a href="#refer" onclick="closeTab()">[3]</a>. Hence, we engineered our bacteria in such a way that it could do most of the work done by these monstrous machines so that we no longer have to buy them and pay their bills.
 +
To increase the yield of the product, we came up with the idea of separating cell growth and target protein production so that when the cells have grown up to a high enough cell density, they shuttle all their energy towards the required protein production<a href="#refer" onclick="closeTab()"> [4]</a>. Based on the above ideas, we came up with the design of our bioreactor.<br>
 
We realized that we would not be able to work on the whole idea this summer so, we focussed on two modules of our design: the Protein production module and the auto-aggregation module leaving the arresting of cell growth for future iGEM teams as a seed for their ideas.
 
We realized that we would not be able to work on the whole idea this summer so, we focussed on two modules of our design: the Protein production module and the auto-aggregation module leaving the arresting of cell growth for future iGEM teams as a seed for their ideas.
        </p>
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        <h1>Protein Production Module</h1>
 
        <p>Induction synthesis of protein of interest is another important step. Microorganisms in bioreactors are induced at the OD, at which the protein production is maximum. <a href="#bull5" onclick="closeBar()">[5]</a> Because of this, factories install sophisticated machinery to keep track of the OD value of the culture so as to know when to induce the production. We wanted our bacteria to know when to start protein production and start it by itself. Hence, we used the lux quorum sensing system to sense this cell density. <a href="#bull6" onclick="closeBar()">[6]</a> We have expressed the gene for our protein of interest under the luxI gene so that protein of interest is produced in significant quantities only when the quorum is achieved.(Figure 2) We also wish to tune the quorum sensing system by tweaking with the strength of the promoters involved in quorum sensing.
 
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<div class="mid-content wow fadeInRight animated" data-wow-delay=".5s">
        <h1>Protein Production Module</h1>
+
<h3>Protein production</h3>
        <p>Induction synthesis of protein of interest is another important step. Microorganisms in bioreactors are induced at the OD, at which the protein production is maximum. <a href="#bull6" onclick="closeBar()">[6]</a> Because of this, factories install sophisticated machinery to keep track of the OD value of the culture so as to know when to induce the production. We wanted our bacteria to know when to start protein production and start it by itself. Hence, we used the lux quorum sensing system to sense this cell density. <a href="#bull7" onclick="closeBar()">[7]</a> We have expressed the gene for our protein of interest under the luxI gene so that protein of interest is produced in significant quantities only when the quorum is achieved.(Figure 2) We also wish to tune the quorum sensing system by tweaking with the strength of the promoters involved in quorum sensing.
+
</div>
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+
<div class="row">
      </div>
+
<div class="refer col-md-6">
      <div class="col-md-6 aggrTabcontent">
+
<p class="whitef leftMove"></html>[[File:Lux iisc.jpg|right]]<html>Induction synthesis of protein of interest is another important step. Microorganisms in bioreactors are induced at the OD, at which the protein production is maximum. <a href="#refer" onclick="closeTab()">[5]</a> Because of this, factories install sophisticated machinery to keep track of the OD value of the culture so as to know when to induce the production. We wanted our bacteria to know when to start protein production and start it by itself. Hence, we used the lux quorum sensing system to sense this cell density. <a href="#refer" onclick="closeTab()">[6]</a> We have expressed the gene for our protein of interest under the luxI gene so that protein of interest is produced in significant quantities only when the quorum is achieved.(Figure 2) We also wish to tune the quorum sensing system by tweaking with the strength of the promoters involved in quorum sensing.
        <div class="bioreactorImgwrap">
+
      <!-- <br><span class="readm hvr-ripple-out">Read more</span>  -->
        <img class="aggrImg" src="file:///media/jessica/4C84DF1584DF007E/iGem/site/14Bootstrap/tube.jpg" />
+
 
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 +
<h3>Auto-aggregation</h3>
 +
</div>
 +
<div class="row">
 +
<div class="refer col-md-6">
 +
<p class="whitef"></html>[[File:Tube iisc.jpg|right]]<html>To achieve cellular aggregation, we use the famous auto-transporter protein, Antigen43 (Ag43). <a href="#refer" onclick="closeTab()">[7]</a> It has shown to cause auto-aggregation of cells when overexpressed. (Figure 3) We plan to exploit this property of Ag43 to substitute centrifugation. We acknowledge previous iGEM teams who have worked on Ag43 (Hokkaido University, 2012; Aberdeen Scotland, 2014 and some more) as we got the BioBricks for Ag43 readily available.  We intend to express Ag43 only when the cells have made the product of interest. Hence, we use the diauxic shift in the media to act as a switch for the expression of Ag43.
 +
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<h3>References</h3>
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 +
<div class="refer col-md-6">
 +
<ol>
 +
          <li> Ferrer-Miralles N, Domingo-Espin J, Corchero JL, Vazquez E, Villaverde A. Microbial factories for recombinant pharmaceuticals, Microbial Cell Factories, 2009:8:17. </li>
 +
          <li><a href="http://lib.tkk.fi/Lic/2009/urn100121.pdf" target="_blank"> Raisa Vermasvuori,
 +
P<span class="lowert">RODUCTION OF RECOMBINANT PROTEINS AND
 +
MONOCLONAL ANTIBODIES –
 +
TECHNO-ECONOMICAL EVALUATION OF THE
 +
PRODUCTION METHODS<span></a> </li>
 +
          <li> Felo M., Christensen B., Higgins J., Process cost and facility considerations in the selection of primary cell culture clarification technology, AIChE, 2013. </li>
 +
          <li> Motoo Suzuki, Rohini Roy, Haiyan Zheng, Nancy Woychik, Masayori Inouye, Bacterial Bioreactors for High Yield Production of Recombinant Protein. The Journal of Biological Chemistry, 2006.</li>
 +
          <li> Rosano G.L., Ceccarelli E. A., Recombinant protein expression in Escherichia coli: advances and challenges, Frontiers in Microbiology, 2014.</li>
 +
          <li> Miller M.B., Bassler B.L., Quorum Sensing in Bacteria, Annual Review of Microbiology, 2001.</li>
 +
          <li> Marjan W. van der Woude, Ian R. Henderson, Regulation and Function of Ag43 (Flu), Annu. Rev. Microbiol., 2008.
 +
</li>
 +
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+
       <h1>Overview</h1><hr>
        <div class="ref">
+
      <p class="whitef">With the advent of rDNA technology in the late 1970s, medicine, agriculture and several other areas underwent a quantum leap and from that point, progress only hastened, from one only one recombinant pharmaceutical  approved for human use (insulin) in 1982 to one hundred and fifty-one FDA approved protein based recombinant pharmaceuticals by 2009<a href="#refer" onclick="closeTab()">[1]</a>.
        <li><span id="bull1" class="label label-primary">[1]</span>Ferrer-Miralles N, Domingo-Espin J, Corchero JL, Vazquez E, Villaverde A. Microbial factories for recombinant pharmaceuticals, Microbial Cell Factories, 2009:8:17.</li>
+
Despite being in high demand (due to the fact that most recombinant products produced on an industrial scale are therapies for chronic diseases like cancer and diabetes), recombinant products are expensive due to several factors like long and expensive development time, high failure rate (~80%) of the products developed, manufacturing costs requiring expensive technologies and processes (bioreactors, column chromatography, sterile conditions, etc) and the involvement of skilled labor on both the manufacturing and the healthcare provider’s side<a href="#refer" onclick="closeTab()">[2]</a>. Treatments with these pharmaceuticals can cost from around 10,000 to 100,000 € per year for a single patient[2]. As scientists and engineers, it seems obvious that our contribution can be most easily and effectively be made at the level of manufacturing costs; to try to bring down the cost of these life-saving products.
      </div>
+
       <!-- <br><span class="readm hvr-ripple-out">Read more</span>
       <div>
+
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        <li ><span id="bull2" class="label label-primary">[2]</span>Medipally S.R., Yusoff F. Md., Banerjee S., Shariff M. Microalgae as sustainable renewable energy Feedstock for Biofuel Production, BioMed Research International, 2015.</li>
+
    </div>
 
       </div>
 
       </div>
      <div class="ref">
 
        <li ><span id="bull3" class="label label-primary">[3]</span>Felo M., Christensen B., Higgins J., Process cost and facility considerations in the selection of primary cell culture clarification technology, AIChE, 2013.
 
</li>
 
        </div>
 
        <div class="ref">
 
        <li ><span id="bull4" class="label label-primary">[4]</span>Motoo Suzuki, Rohini Roy, Haiyan Zheng, Nancy Woychik, Masayori Inouye, Bacterial Bioreactors for High Yield Production of Recombinant Protein. The Journal of Biological Chemistry, 2006.</li>
 
      </div>
 
      <div class="ref">
 
        <li ><span id="bull5" class="label label-primary">[5]</span>Rosano G.L., Ceccarelli E. A., Recombinant protein expression in Escherichia coli: advances and challenges, Frontiers in Microbiology, 2014.</li>
 
      </div>
 
      <div class="ref">
 
        <li ><span id="bull6" class="label label-primary">[6]</span>Miller M.B., Bassler B.L., Quorum Sensing in Bacteria, Annual Review of Microbiology, 2001.</li>
 
      </div>
 
      <div class="ref">
 
        <li ><span id="bull7" class="label label-primary">[7]</span>Marjan W. van der Woude, Ian R. Henderson, Regulation and Function of Ag43 (Flu), Annu. Rev. Microbiol., 2008.</li>
 
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      <h1>Bioreactor design</h1><hr> </html>[[File:Flowchart iisc.jpg|right]]<html>
 +
      <p class="whitef leftMove">We realized that manufacturing units use expensive and energy expensive machinery <a href="#refer" onclick="closeTab()">[3]</a>. Hence, we engineered our bacteria in such a way that it could do most of the work done by these monstrous machines so that we no longer have to buy them and pay their bills.
 +
To increase the yield of the product, we came up with the idea of separating cell growth and target protein production so that when the cells have grown up to a high enough cell density, they shuttle all their energy towards the required protein production<a href="#refer" onclick="closeTab()"> [4]</a>. Based on the above ideas, we came up with the design of our bioreactor.<br>
 +
We realized that we would not be able to work on the whole idea this summer so, we focussed on two modules of our design: the Protein production module and the auto-aggregation module leaving the arresting of cell growth for future iGEM teams as a seed for their ideas.
 +
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 +
 
 +
      <p class="whitef leftMove">Induction synthesis of protein of interest is another important step. Microorganisms in bioreactors are induced at the OD, at which the protein production is maximum. <a href="#refer" onclick="closeTab()">[5]</a> Because of this, factories install sophisticated machinery to keep track of the OD value of the culture so as to know when to induce the production. We wanted our bacteria to know when to start protein production and start it by itself. Hence, we used the lux quorum sensing system to sense this cell density. <a href="#refer" onclick="closeTab()">[6]</a> We have expressed the gene for our protein of interest under the luxI gene so that protein of interest is produced in significant quantities only when the quorum is achieved.(Figure 2) We also wish to tune the quorum sensing system by tweaking with the strength of the promoters involved in quorum sensing.
 +
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 +
 
 +
      <p class="whitef">To achieve cellular aggregation, we use the famous auto-transporter protein, Antigen43 (Ag43). <a href="#refer" onclick="closeTab()">[7]</a> It has shown to cause auto-aggregation of cells when overexpressed. (Figure 3) We plan to exploit this property of Ag43 to substitute centrifugation. We acknowledge previous iGEM teams who have worked on Ag43 (Hokkaido University, 2012; Aberdeen Scotland, 2014 and some more) as we got the BioBricks for Ag43 readily available.  We intend to express Ag43 only when the cells have made the product of interest. Hence, we use the diauxic shift in the media to act as a switch for the expression of Ag43.
 +
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Latest revision as of 01:06, 20 October 2016

Team IISc iGem

Overview

With the advent of rDNA technology in the late 1970s, medicine, agriculture and several other areas underwent a quantum leap
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Bioreactor design

As stated in the introduction, our project is an attempt to modify E coli to lower capital and running costs for rDNA bioreactor systems, by automating protein over-expression induction and separation of cell from growth media. To learn more about the existing biotech infrastructure in India, we decided to visit some biotech parks in India and explore the feasibility and applicability of our idea.
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Protein production module

Induction synthesis of protein of interest is another important step.
Read rest

Auto-aggregation

To achieve cellular aggregation, we use the famous auto-transporter protein, Antigen43 (Ag43).
Read more

Overview

With the advent of rDNA technology in the late 1970s, medicine, agriculture and several other areas underwent a quantum leap and from that point, progress only hastened, from one only one recombinant pharmaceutical approved for human use (insulin) in 1982 to one hundred and fifty-one FDA approved protein based recombinant pharmaceuticals by 2009[1]. Despite being in high demand (due to the fact that most recombinant products produced on an industrial scale are therapies for chronic diseases like cancer and diabetes), recombinant products are expensive due to several factors like long and expensive development time, high failure rate (~80%) of the products developed, manufacturing costs requiring expensive technologies and processes (bioreactors, column chromatography, sterile conditions, etc) and the involvement of skilled labor on both the manufacturing and the healthcare provider’s side[2]. Treatments with these pharmaceuticals can cost from around 10,000 to 100,000 € per year for a single patient[2]. As scientists and engineers, it seems obvious that our contribution can be most easily and effectively be made at the level of manufacturing costs; to try to bring down the cost of these life-saving products.

Bioreactor design

Flowchart iisc.jpg
We realized that manufacturing units use expensive and energy expensive machinery [3]. Hence, we engineered our bacteria in such a way that it could do most of the work done by these monstrous machines so that we no longer have to buy them and pay their bills. To increase the yield of the product, we came up with the idea of separating cell growth and target protein production so that when the cells have grown up to a high enough cell density, they shuttle all their energy towards the required protein production [4]. Based on the above ideas, we came up with the design of our bioreactor.
We realized that we would not be able to work on the whole idea this summer so, we focussed on two modules of our design: the Protein production module and the auto-aggregation module leaving the arresting of cell growth for future iGEM teams as a seed for their ideas.

Protein production

Lux iisc.jpg
Induction synthesis of protein of interest is another important step. Microorganisms in bioreactors are induced at the OD, at which the protein production is maximum. [5] Because of this, factories install sophisticated machinery to keep track of the OD value of the culture so as to know when to induce the production. We wanted our bacteria to know when to start protein production and start it by itself. Hence, we used the lux quorum sensing system to sense this cell density. [6] We have expressed the gene for our protein of interest under the luxI gene so that protein of interest is produced in significant quantities only when the quorum is achieved.(Figure 2) We also wish to tune the quorum sensing system by tweaking with the strength of the promoters involved in quorum sensing.

Auto-aggregation

Tube iisc.jpg
To achieve cellular aggregation, we use the famous auto-transporter protein, Antigen43 (Ag43). [7] It has shown to cause auto-aggregation of cells when overexpressed. (Figure 3) We plan to exploit this property of Ag43 to substitute centrifugation. We acknowledge previous iGEM teams who have worked on Ag43 (Hokkaido University, 2012; Aberdeen Scotland, 2014 and some more) as we got the BioBricks for Ag43 readily available. We intend to express Ag43 only when the cells have made the product of interest. Hence, we use the diauxic shift in the media to act as a switch for the expression of Ag43.

References

  1. Ferrer-Miralles N, Domingo-Espin J, Corchero JL, Vazquez E, Villaverde A. Microbial factories for recombinant pharmaceuticals, Microbial Cell Factories, 2009:8:17.
  2. Raisa Vermasvuori, PRODUCTION OF RECOMBINANT PROTEINS AND MONOCLONAL ANTIBODIES – TECHNO-ECONOMICAL EVALUATION OF THE PRODUCTION METHODS
  3. Felo M., Christensen B., Higgins J., Process cost and facility considerations in the selection of primary cell culture clarification technology, AIChE, 2013.
  4. Motoo Suzuki, Rohini Roy, Haiyan Zheng, Nancy Woychik, Masayori Inouye, Bacterial Bioreactors for High Yield Production of Recombinant Protein. The Journal of Biological Chemistry, 2006.
  5. Rosano G.L., Ceccarelli E. A., Recombinant protein expression in Escherichia coli: advances and challenges, Frontiers in Microbiology, 2014.
  6. Miller M.B., Bassler B.L., Quorum Sensing in Bacteria, Annual Review of Microbiology, 2001.
  7. Marjan W. van der Woude, Ian R. Henderson, Regulation and Function of Ag43 (Flu), Annu. Rev. Microbiol., 2008.
×

Overview


With the advent of rDNA technology in the late 1970s, medicine, agriculture and several other areas underwent a quantum leap and from that point, progress only hastened, from one only one recombinant pharmaceutical approved for human use (insulin) in 1982 to one hundred and fifty-one FDA approved protein based recombinant pharmaceuticals by 2009[1]. Despite being in high demand (due to the fact that most recombinant products produced on an industrial scale are therapies for chronic diseases like cancer and diabetes), recombinant products are expensive due to several factors like long and expensive development time, high failure rate (~80%) of the products developed, manufacturing costs requiring expensive technologies and processes (bioreactors, column chromatography, sterile conditions, etc) and the involvement of skilled labor on both the manufacturing and the healthcare provider’s side[2]. Treatments with these pharmaceuticals can cost from around 10,000 to 100,000 € per year for a single patient[2]. As scientists and engineers, it seems obvious that our contribution can be most easily and effectively be made at the level of manufacturing costs; to try to bring down the cost of these life-saving products.

×

Bioreactor design


Flowchart iisc.jpg

We realized that manufacturing units use expensive and energy expensive machinery [3]. Hence, we engineered our bacteria in such a way that it could do most of the work done by these monstrous machines so that we no longer have to buy them and pay their bills. To increase the yield of the product, we came up with the idea of separating cell growth and target protein production so that when the cells have grown up to a high enough cell density, they shuttle all their energy towards the required protein production [4]. Based on the above ideas, we came up with the design of our bioreactor.
We realized that we would not be able to work on the whole idea this summer so, we focussed on two modules of our design: the Protein production module and the auto-aggregation module leaving the arresting of cell growth for future iGEM teams as a seed for their ideas.

×

Protein production


Lux iisc.jpg

Induction synthesis of protein of interest is another important step. Microorganisms in bioreactors are induced at the OD, at which the protein production is maximum. [5] Because of this, factories install sophisticated machinery to keep track of the OD value of the culture so as to know when to induce the production. We wanted our bacteria to know when to start protein production and start it by itself. Hence, we used the lux quorum sensing system to sense this cell density. [6] We have expressed the gene for our protein of interest under the luxI gene so that protein of interest is produced in significant quantities only when the quorum is achieved.(Figure 2) We also wish to tune the quorum sensing system by tweaking with the strength of the promoters involved in quorum sensing.

×

Auto-aggregation


Tube iisc.jpg

To achieve cellular aggregation, we use the famous auto-transporter protein, Antigen43 (Ag43). [7] It has shown to cause auto-aggregation of cells when overexpressed. (Figure 3) We plan to exploit this property of Ag43 to substitute centrifugation. We acknowledge previous iGEM teams who have worked on Ag43 (Hokkaido University, 2012; Aberdeen Scotland, 2014 and some more) as we got the BioBricks for Ag43 readily available. We intend to express Ag43 only when the cells have made the product of interest. Hence, we use the diauxic shift in the media to act as a switch for the expression of Ag43.