Team:Carnegie Mellon/Our Sensor

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<p>In order decrease time and increase sensitivity, our approach was to use the robust T7 RNA Polymerase (T7 RNAP) and a fluorescent reporter. T7 RNAP had been used with a temperature sensitive intein (Liang et al. 2007). At the permissive temperature the intein was spliced out to form functional T7 RNAP resulting in transcription from the T7 promoter to the terminator only at the permissive temperature of 18 &deg;C, but not at the restrictive temperature of 37 &deg;C. The <i>S. cerevisiae</i> VMA intein was inserted in between the Ala491 and Cys492 residues of the T7 RNAP. The T7 promoter was placed upstream of the <i>lacZ</i> gene, and was transcribed and translated resulting in blue colonies upon the production of functional T7 RNAP.</p>
<p>In order decrease time and increase sensitivity, our approach was to use the robust T7 RNA Polymerase (T7 RNAP) and a fluorescent reporter. T7 RNAP had been used with a temperature sensitive intein (Liang et al. 2007). At the permissive temperature the intein was spliced out to form functional T7 RNAP resulting in transcription from the T7 promoter to the terminator only at the permissive temperature of 18 &deg;C, but not at the restrictive temperature of 37 &deg;C. The <i>S. cerevisiae</i> VMA intein was inserted in between the Ala491 and Cys492 residues of the T7 RNAP. The T7 promoter was placed upstream of the <i>lacZ</i> gene, and was transcribed and translated resulting in blue colonies upon the production of functional T7 RNAP.</p>
<p>In order to construct a sensitive assay, a system to amplify the estrogen signal was required. We designed a system that inserted an estrogen responsive intein inside T7 RNAP at the 491 and 492 residues. T7 RNAP is a strong viral polymerase requiring no additional factors, making its expression straightforward. In the presence of estrogen, functional T7 RNAP would be produced, and readily bind to the T7 promoter, resulting in signal amplification in the presence of estrogen. The level of the estrogen-responsive intein sensor is reported using a yellow fluorescent protein and the level of estrogen, measured by the production of functional T7 RNAP, would be reported using a red fluorescent protein.</p>
<p>In order to construct a sensitive assay, a system to amplify the estrogen signal was required. We designed a system that inserted an estrogen responsive intein inside T7 RNAP at the 491 and 492 residues. T7 RNAP is a strong viral polymerase requiring no additional factors, making its expression straightforward. In the presence of estrogen, functional T7 RNAP would be produced, and readily bind to the T7 promoter, resulting in signal amplification in the presence of estrogen. The level of the estrogen-responsive intein sensor is reported using a yellow fluorescent protein and the level of estrogen, measured by the production of functional T7 RNAP, would be reported using a red fluorescent protein.</p>
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<center><p><img src ="https://static.igem.org/mediawiki/2014/1/11/Sensor.png" alt="ER sensor"</p></center>
<p><b>References:</b></p>
<p><b>References:</b></p>
<p>Routledge EJ, Sumpter JP. 1996. Estrogenic activity of surfactants and some of their degradation products assessed using a recombinant yeast screen.  Environ. Toxicol. Chem. 15, 241–248.</p>
<p>Routledge EJ, Sumpter JP. 1996. Estrogenic activity of surfactants and some of their degradation products assessed using a recombinant yeast screen.  Environ. Toxicol. Chem. 15, 241–248.</p>

Revision as of 18:46, 17 October 2014

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