Team:IvyTech SouthBend IN

From 2014.igem.org

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<h3>What is your project about?</h3>
<h3>What is your project about?</h3>
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<p>Our project Idea is based on the need for for a preemptive approach to fecal matter bacteriophage disease causing viruses, not the post disease acquiring reaction that is now in effect.Currently those in charge of the swimming areas wait until they are notified that someone has come down with an unknown sickness and only know they swam in the area the day before. Two to three people may have symptoms and the common denominator is swimming at the same beach or drinking the same water. A water sample is then taken, sent to a local laboratory and grown up on petri  dishes. When a beach is closed due to bacteria it is usually three days after the current full of bacteria-phages was present. Given the amount of swimming areas, beaches and public access sites, along with the number of people who frequent them, we feel that there is a need for a rapid, handheld bio-sensor that can immediately get results.  </p>
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<p>The American Public Health Assay (APHA) for human waste contaminated water is hampered by a dependency on culturing coliform bacteria with a turn-around time exceeding one day.  An assay for coliphage detection, as surrogate for coliforms, has been developed which employs the release of the host indicator cell β-galactosidase enzyme (β-gal) activity by lytic coliphage and the conversion of a colorimetric substrate.  While significantly shortening the APHA time to 3 hrs.,  this assay requires a laboratory equipment to separate phage-induced released β-gal enzyme from intact cells before addition of the substrate.  To optimize this assay we have taken advantage of the α-complementation feature of β-gal. We are engineering cell lines containing either the gene fragments of LacZα or LacZΩ of β-gal on separate plasmids. We predict upon lysis of a mix population of cells by coliphage in the presence of substrate, the gene products will complement in trans reconstituting the β-gal activity thus eliminating a separation step in the assay. In addition we are testing the introduction of a cassette of coliphage cell lysis genes on both plasmids under the control of a coliphage promoter to accelerate the enzyme fragment release thus further reducing test time.  Our goal is to design a fast-acting hand-held coliphage biosensor device that can be used by someone without any special technical expertise.  We anticipate our device being useful in rapidly reporting the contamination of recreational waters in the U.S. or assuring potable water in the water sources in the developing World.  </p>
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<h3> How does your project work?</h3>
<h3> How does your project work?</h3>
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<p> Our project uses a lytic coliphage release of the bacterial beta-galactosidase enzyme activity and the conversion of a colorimetric substrate. In the presence of lacZ alpha fragments, the LacZ omega fragments will bind to the alpha fragments creating change in either pH or electrolyte-resistivity.</p>
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<p>The human pathogens in contaminated water are too varied to reasonably test for their presence. The presence of the normal human enteric bacteria E.coli has been used as a marker for contamination but their are conscerns that it might not persist in the environment as long as the human pathogenic virus will.  Another dependable marker of water contaminated by human is, however, the presence of bacteriophage of the human intestines or so-called "coliphage."  These have been found to be more stable under various environmental conditions and because the lyse E.coli can be used to detect the presence of human waste in the water.  Our biosensor is designed to report the lysis of target cells by coliphage by the release of one of two fragments of the enzyme beta-galactosidase (Omega fragment).  Upon release the beta-galactosidase omega fragment joins beta-galactosidase alpha fragments that are suspended by the added contaminated water.  After the two fragments join, beta-galactosidase enzyme activity is formed and an enzyme substrate present is converted to its colorimetric form.  The amount of color development will be quantified by comparison with a parallel test with known amount of coliphage present. </p>
<a href="http://ckmnye.wix.com/2014ivytechsouthbend/">Visit to Learn More</a>  
<a href="http://ckmnye.wix.com/2014ivytechsouthbend/">Visit to Learn More</a>  
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<h3> Who will your project help?</h3>
<h3> Who will your project help?</h3>
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<p> Our project will not only safeguard lakes,rivers,streams,swimming areas, beaches and public access sites, but potentially safeguard municipalities or anywhere clean uncontaminated water is preferred. The rapid detection and the low cost prediction of the device would have a positive impact on developing countries as well as developed nations where contamination can be a concern.</p>
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<p> Our proposed device could not only be used to safeguard lakes,rivers,streams,swimming areas, beaches and public access sites, but potentially municipalities or anywhere clean uncontaminated water is preferred. The rapid detection and the potential low cost of the device would have a positive impact on developing countries as well as developed nations where drinking water safety is a concern.</p>
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Revision as of 03:48, 29 August 2014

Team:IvyTech SouthBend IN/Templates/Navigationbar

Welcome!
We are Team Ivy Tech Community College of Indiana-South Bend!

Please click on banner links to learn more about our team and project!

What is your project about?

The American Public Health Assay (APHA) for human waste contaminated water is hampered by a dependency on culturing coliform bacteria with a turn-around time exceeding one day. An assay for coliphage detection, as surrogate for coliforms, has been developed which employs the release of the host indicator cell β-galactosidase enzyme (β-gal) activity by lytic coliphage and the conversion of a colorimetric substrate. While significantly shortening the APHA time to 3 hrs., this assay requires a laboratory equipment to separate phage-induced released β-gal enzyme from intact cells before addition of the substrate. To optimize this assay we have taken advantage of the α-complementation feature of β-gal. We are engineering cell lines containing either the gene fragments of LacZα or LacZΩ of β-gal on separate plasmids. We predict upon lysis of a mix population of cells by coliphage in the presence of substrate, the gene products will complement in trans reconstituting the β-gal activity thus eliminating a separation step in the assay. In addition we are testing the introduction of a cassette of coliphage cell lysis genes on both plasmids under the control of a coliphage promoter to accelerate the enzyme fragment release thus further reducing test time. Our goal is to design a fast-acting hand-held coliphage biosensor device that can be used by someone without any special technical expertise. We anticipate our device being useful in rapidly reporting the contamination of recreational waters in the U.S. or assuring potable water in the water sources in the developing World.

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How does your project work?

The human pathogens in contaminated water are too varied to reasonably test for their presence. The presence of the normal human enteric bacteria E.coli has been used as a marker for contamination but their are conscerns that it might not persist in the environment as long as the human pathogenic virus will. Another dependable marker of water contaminated by human is, however, the presence of bacteriophage of the human intestines or so-called "coliphage." These have been found to be more stable under various environmental conditions and because the lyse E.coli can be used to detect the presence of human waste in the water. Our biosensor is designed to report the lysis of target cells by coliphage by the release of one of two fragments of the enzyme beta-galactosidase (Omega fragment). Upon release the beta-galactosidase omega fragment joins beta-galactosidase alpha fragments that are suspended by the added contaminated water. After the two fragments join, beta-galactosidase enzyme activity is formed and an enzyme substrate present is converted to its colorimetric form. The amount of color development will be quantified by comparison with a parallel test with known amount of coliphage present.

Visit to Learn More
Top

Who will your project help?

Our proposed device could not only be used to safeguard lakes,rivers,streams,swimming areas, beaches and public access sites, but potentially municipalities or anywhere clean uncontaminated water is preferred. The rapid detection and the potential low cost of the device would have a positive impact on developing countries as well as developed nations where drinking water safety is a concern.

Top

Why did you choose this project?

The thought of creating something from the ground up as well as applying education to overcome obstacles that occur in everyday life has been a tremendous motivator. Being able to use science and engineering to make the lives of others more safe is our main goal and why we chose this project.

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