Team:Lethbridge/Project/Compartamentalization
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To characterize the means of targeting the tagged protein we will be using another expression construct as shown in Figure 1 that contains the IPTG inducible LS that also has two fluorescent proteins – cyan fluorescent protein (CFP) and yellow fluorescent protein (YFP) – that are controlled by an arabinose induced inverter. This would allow us to selectively express the LS by adding IPTG and repressing the fluorescent protein expression by adding arabinose. We have chosen to work with CFP and YFP due their ability to undergo fluorescence resonance energy transfer (FRET) that will allow us to observe their colocalization within the LS microcompartment (for a general overview of FRET visit <html><a href="http://en.wikipedia.org/wiki/Förster_resonance_energy_transfer" target="new"><font color="green">Wikipedia </font></a></html>or <html><a href="https://2009.igem.org/Team:Lethbridge/Project#The_Experiments" target="new"><font color="green">Lethbridge 2009 FRET</font></a></html>). By observing FRET within the microcompartment it will demonstrate our ability to selectively localize multiple proteins within it. | To characterize the means of targeting the tagged protein we will be using another expression construct as shown in Figure 1 that contains the IPTG inducible LS that also has two fluorescent proteins – cyan fluorescent protein (CFP) and yellow fluorescent protein (YFP) – that are controlled by an arabinose induced inverter. This would allow us to selectively express the LS by adding IPTG and repressing the fluorescent protein expression by adding arabinose. We have chosen to work with CFP and YFP due their ability to undergo fluorescence resonance energy transfer (FRET) that will allow us to observe their colocalization within the LS microcompartment (for a general overview of FRET visit <html><a href="http://en.wikipedia.org/wiki/Förster_resonance_energy_transfer" target="new"><font color="green">Wikipedia </font></a></html>or <html><a href="https://2009.igem.org/Team:Lethbridge/Project#The_Experiments" target="new"><font color="green">Lethbridge 2009 FRET</font></a></html>). By observing FRET within the microcompartment it will demonstrate our ability to selectively localize multiple proteins within it. | ||
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With our ability to control the production of LS and the florescent proteins separately we will be able to determine the optimal conditions that will allow the colocalization of the proteins. By varying both the concentrations of arabinose and IPTG as well as the times of induction we will be able to determine the optimal conditions. Examples of conditions we will attempt in the future are shown in Figure 2. This will allow us to determine if the microcompartments form before entry of the proteins, after or simultaneously for a better understanding of the system. | With our ability to control the production of LS and the florescent proteins separately we will be able to determine the optimal conditions that will allow the colocalization of the proteins. By varying both the concentrations of arabinose and IPTG as well as the times of induction we will be able to determine the optimal conditions. Examples of conditions we will attempt in the future are shown in Figure 2. This will allow us to determine if the microcompartments form before entry of the proteins, after or simultaneously for a better understanding of the system. | ||
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