Difference between revisions of "Team:ColumbiaNYC/HP/Silver"

 
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   <!-- SafetyStyle CSS -->
 
   <!-- SafetyStyle CSS -->
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     <div class="container">
 
     <div class="container">
 
       <h1>Safety - HP Silver</h1>
 
       <h1>Safety - HP Silver</h1>
       <p>Lorem ipsum dolor sit amet, consectetur adipisicing elit. Sint, explicabo dolores ipsam aliquam inventore corrupti.</p>
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<!-- Page Content -->
  <body>
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<body>
  
 
   <div class="container gallery-container">
 
   <div class="container gallery-container">
      <div class="tz-gallery">
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    <div class="tz-gallery">
  
        <div class="row">
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      <div class="row">
 +
        <div class="col-lg-12">
 +
          <h2>Listeria monocytogenes (hlyA gene)</h2>
 +
          <br>
 +
          <p>The hlyA gene codes for Listeriolysin O. When human cells have engulfed Listeria cells by phagocytosis, Listeriolysin
 +
            O becomes active and breaks open the phagosome, allowing the bacteria to live in the cytoplasm. Bacteria transformed
 +
            with Listeriolysin O are invasive microorganisms with the ability to hide from the immune system. With Listeriolysin,
 +
            bacteria can invade macrophages and then break open the phagosome, and the bacteria are free to live inside the
 +
            cytoplasm. Genetically engineered bacteria that express both listeriolysin and invasin are able to invade any
 +
            beta-1-integrin expressing cell type, and they can penetrate to the cytoplasm at high efficiencies.</p>
 +
          <br>
 +
          <p>
 +
            The hlyA gene (coding for Listerolysin O) will be part of the transkingdom RNAi plasmid (TRIP) that the team will use to
 +
            determine how well transkingdom RNA interference will work on different types of cancer cells and different oncogenes.
 +
            We aim to design the bacteria so that it only targets cancer cells.
 +
          </p>
  
           <div class="col-sm-6 col-md-4">
+
        </div>
            <div class="thumbnail">
+
        <div class="col-lg-12">
              <a class="lightbox" href="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg">
+
           <h2>Yersinia enterocolitica (Inv gene)</h2>
                <img src="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg" alt="1">
+
          <br>
              </a>
+
          <p>The inv gene codes for the invasin protein. The invasin protein on the surface of a Yersinia cell interacts with
              <div class="caption">
+
            beta-1-integrin receptors on the surface of eukaryotic cells. This triggers a signal transduction pathway, leading
                <h3>Thumbnail label</h3>
+
            to endocytosis of the whole bacterium. Bacteria transformed with invasin are invasive microorganisms with the
                 <p>This is where we do polymerase chain reaction</p>
+
            ability to hide from the immune system. Genetically engineered bacteria that express both listeriolysin and invasin
 +
            are able to invade any beta-1-integrin expressing cell type, and they can penetrate to the cytoplasm at high
 +
            efficiencies.
 +
          </p>
 +
          <br>
 +
          <p>
 +
            The inv gene (coding for invasin) will be part of the transkingdom RNAi plasmid (TRIP) that the team will use to determine
 +
            how well transkingdom RNA interference will work on different types of cancer cells and different oncogenes.
 +
            We aim to design the bacteria so that it only targets cancer cells.
 +
          </p>
 +
 
 +
        </div>
 +
        <div class="col-lg-12">
 +
            <h2>Precautions taken with hlyA and Inv genes</h2>
 +
          <div class="row">
 +
            <div class="col-sm-6 col-md-4">
 +
              <div class="thumbnail">
 +
                <a class="lightbox" href="https://static.igem.org/mediawiki/2017/9/9f/T--ColumbiaNYC--LabSafetyPic1.jpg">
 +
                  <img src="https://static.igem.org/mediawiki/2017/9/9f/T--ColumbiaNYC--LabSafetyPic1.jpg" alt="1">
 +
                </a>
 +
                <div class="caption">
 +
                  <h3>Incubators, PCR, Thermocycler Station</h3>
 +
                 </div>
 
               </div>
 
               </div>
 
             </div>
 
             </div>
          </div>
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            <div class="col-sm-6 col-md-4">
          <div class="col-sm-6 col-md-4">
+
              <div class="thumbnail">
            <div class="thumbnail">
+
                <a class="lightbox" href="https://static.igem.org/mediawiki/2017/e/ef/T--ColumbiaNYC--LabSafetyPic2.jpg">
              <a class="lightbox" href="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg">
+
                  <img src="https://static.igem.org/mediawiki/2017/e/ef/T--ColumbiaNYC--LabSafetyPic2.jpg" alt="1">
                <img src="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg" alt="1">
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                </a>
              </a>
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                <div class="caption">
              <div class="caption">
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                  <h3>Tissue culture hood/Biosafety cabinet</h3>
                <h3>Thumbnail label</h3>
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                 </div>
                 <p>This is where we do polymerase chain reaction</p>
+
 
               </div>
 
               </div>
 
             </div>
 
             </div>
          </div>
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            <div class="col-sm-6 col-md-4">
          <div class="col-sm-6 col-md-4">
+
              <div class="thumbnail">
            <div class="thumbnail">
+
                <a class="lightbox" href="https://static.igem.org/mediawiki/2017/9/93/T--ColumbiaNYC--LabSafetyPic3.jpg">
              <a class="lightbox" href="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg">
+
                  <img src="https://static.igem.org/mediawiki/2017/9/93/T--ColumbiaNYC--LabSafetyPic3.jpg" alt="1">
                <img src="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg" alt="1">
+
                </a>
              </a>
+
                <div class="caption">
              <div class="caption">
+
                  <h3>Open bench</h3>
                <h3>Thumbnail label</h3>
+
                 </div>
                 <p>This is where we do polymerase chain reaction</p>
+
 
               </div>
 
               </div>
 
             </div>
 
             </div>
          </div>
+
            <div class="col-lg-12">
          <div class="col-sm-6 col-md-4">
+
 
            <div class="thumbnail">
+
               <p>The host strain is auxotrophic nonpathegenic E. coli, the DapA- mutant, whose growth is inhibited in the absence
               <a class="lightbox" href="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg">
+
                 of lysine. We wore full personal protective equipment and worked only in specific areas designated only for
                 <img src="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg" alt="1">
+
                 handling these specimen. We were under the supervision of researchers who are experienced and qualified in
              </a>
+
                 working with BSL2 organisms.</p>
              <div class="caption">
+
               <br>
                 <h3>Thumbnail label</h3>
+
              <p>
                 <p>This is where we do polymerase chain reaction</p>
+
                All team members received lab safety training prior to lab work. Research compliance and administration is coordinated through
               </div>
+
                Columbia University's RASCAL web-based application and through Columbia University's Office of Research Compliance
            </div>
+
                and Training. Each member of the 2017 Columbia University iGEM team has undergone extensive training and
          </div>
+
                attained certification in the use of recombinant DNA, biological safety and bloodborne pathogen precautions,
          <div class="col-sm-6 col-md-4">
+
                and lab safety, chemical hygiene, and hazardous waste management. More information and resources about specific
            <div class="thumbnail">
+
                 guidelines for safety can be found on the <a href="http://www.columbia.edu/cu/compliance/index.html."> Office of Research Compliance and Training website </a> at
              <a class="lightbox" href="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg">
+
                At Columbia University, the Environmental Health and Safety Department is responsible for the safety of biology
                 <img src="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg" alt="1">
+
                 labs. The department follows the guidelines set by the National Institute of Health (NIH) and does so through
              </a>
+
                 the "application of materials substitution, engineering controls, administrative controls and the use of
              <div class="caption">
+
                personal protective equipment." A link to their guidelines can be found <a href= "http://www.ehs.columbia.edu/bs.html"> here. </a>
                 <h3>Thumbnail label</h3>
+
                 Safety topics discussed include lab access and rules, biosafety levels, biosafety equipment, good microbial
                 <p>This is where we do polymerase chain reaction</p>
+
                technique, disinfection and sterilzation, emergency procedures, transport rules, chemicals, fires, and electrical
              </div>
+
                safety specific to the lab space. Training was provided by the University biosafety office and by our PI's
            </div>
+
                and Instructors. Recommendations as well as descriptions of mandatory safety and health standards are contained
          </div>
+
                in the Occupational Safety and Health Administration (OSHA) Laboratory Safety Guidelines found <a href="https://www.osha.gov/Publications/laboratory/OSHA3404laboratory-safety-guidance.pdf"> here. </a>
          <div class="col-sm-6 col-md-4">
+
               </p>
            <div class="thumbnail">
+
              <a class="lightbox" href="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg">
+
                 <img src="https://static.igem.org/mediawiki/2017/3/3d/T--ColumbiaNYC--LabPic1.jpg" alt="1">
+
              </a>
+
               <div class="caption">
+
                <h3>Thumbnail label</h3>
+
                <p>This is where we do polymerase chain reaction</p>
+
              </div>
+
 
             </div>
 
             </div>
 
           </div>
 
           </div>
 +
 +
        </div>
 +
 +
        <div class="col-lg-12">
 +
          <h2>Ethical Risks and Safety Considerations</h2>
 +
          <br>
 +
          <p>There are safety considerations when engineering a non-pathogenic strain of bacteria to possess such virulence
 +
            factors as invasin and listeriolysin from yersinia and listeria, respectively. By engineering otherwise attenuated
 +
            bacteria to possess these virulence factors, the bacteria can become pathogenic. Containment precautions must
 +
            be taken to ensure the virulence factors do not proliferate through horizontal gene transfer. Additionally, though
 +
            our project is a proposed treatment for aberrant gene expression at the post-transcriptional level for conditions
 +
            such as cancer, it could also be used to induce such disease states. For example, if the shRNA released from
 +
            the invading bacteria was to interfere with a tumor-suppressor gene rather than an oncogene, cancer could be
 +
            induced.
 +
          </p>
 +
 
         </div>
 
         </div>
  
 
       </div>
 
       </div>
 +
 +
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Latest revision as of 22:49, 1 November 2017

Safety - HP Silver

Listeria monocytogenes (hlyA gene)


The hlyA gene codes for Listeriolysin O. When human cells have engulfed Listeria cells by phagocytosis, Listeriolysin O becomes active and breaks open the phagosome, allowing the bacteria to live in the cytoplasm. Bacteria transformed with Listeriolysin O are invasive microorganisms with the ability to hide from the immune system. With Listeriolysin, bacteria can invade macrophages and then break open the phagosome, and the bacteria are free to live inside the cytoplasm. Genetically engineered bacteria that express both listeriolysin and invasin are able to invade any beta-1-integrin expressing cell type, and they can penetrate to the cytoplasm at high efficiencies.


The hlyA gene (coding for Listerolysin O) will be part of the transkingdom RNAi plasmid (TRIP) that the team will use to determine how well transkingdom RNA interference will work on different types of cancer cells and different oncogenes. We aim to design the bacteria so that it only targets cancer cells.

Yersinia enterocolitica (Inv gene)


The inv gene codes for the invasin protein. The invasin protein on the surface of a Yersinia cell interacts with beta-1-integrin receptors on the surface of eukaryotic cells. This triggers a signal transduction pathway, leading to endocytosis of the whole bacterium. Bacteria transformed with invasin are invasive microorganisms with the ability to hide from the immune system. Genetically engineered bacteria that express both listeriolysin and invasin are able to invade any beta-1-integrin expressing cell type, and they can penetrate to the cytoplasm at high efficiencies.


The inv gene (coding for invasin) will be part of the transkingdom RNAi plasmid (TRIP) that the team will use to determine how well transkingdom RNA interference will work on different types of cancer cells and different oncogenes. We aim to design the bacteria so that it only targets cancer cells.

Precautions taken with hlyA and Inv genes

1

Incubators, PCR, Thermocycler Station

1

Tissue culture hood/Biosafety cabinet

1

Open bench

The host strain is auxotrophic nonpathegenic E. coli, the DapA- mutant, whose growth is inhibited in the absence of lysine. We wore full personal protective equipment and worked only in specific areas designated only for handling these specimen. We were under the supervision of researchers who are experienced and qualified in working with BSL2 organisms.


All team members received lab safety training prior to lab work. Research compliance and administration is coordinated through Columbia University's RASCAL web-based application and through Columbia University's Office of Research Compliance and Training. Each member of the 2017 Columbia University iGEM team has undergone extensive training and attained certification in the use of recombinant DNA, biological safety and bloodborne pathogen precautions, and lab safety, chemical hygiene, and hazardous waste management. More information and resources about specific guidelines for safety can be found on the Office of Research Compliance and Training website at At Columbia University, the Environmental Health and Safety Department is responsible for the safety of biology labs. The department follows the guidelines set by the National Institute of Health (NIH) and does so through the "application of materials substitution, engineering controls, administrative controls and the use of personal protective equipment." A link to their guidelines can be found here. Safety topics discussed include lab access and rules, biosafety levels, biosafety equipment, good microbial technique, disinfection and sterilzation, emergency procedures, transport rules, chemicals, fires, and electrical safety specific to the lab space. Training was provided by the University biosafety office and by our PI's and Instructors. Recommendations as well as descriptions of mandatory safety and health standards are contained in the Occupational Safety and Health Administration (OSHA) Laboratory Safety Guidelines found here.

Ethical Risks and Safety Considerations


There are safety considerations when engineering a non-pathogenic strain of bacteria to possess such virulence factors as invasin and listeriolysin from yersinia and listeria, respectively. By engineering otherwise attenuated bacteria to possess these virulence factors, the bacteria can become pathogenic. Containment precautions must be taken to ensure the virulence factors do not proliferate through horizontal gene transfer. Additionally, though our project is a proposed treatment for aberrant gene expression at the post-transcriptional level for conditions such as cancer, it could also be used to induce such disease states. For example, if the shRNA released from the invading bacteria was to interfere with a tumor-suppressor gene rather than an oncogene, cancer could be induced.