IGEM:Cambridge/2008/Notebook/Voltage
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*The mechanism we have designed is similar to that used in the brain – relying on ion movement across the membrane, and gated ion channels. | *The mechanism we have designed is similar to that used in the brain – relying on ion movement across the membrane, and gated ion channels. | ||
*To simplify the concept, we are only regulating and measuring the flux of potassium (K+) ions, and we are using a directly glutamate-gated K+ ion channel. | *To simplify the concept, we are only regulating and measuring the flux of potassium (K+) ions, and we are using a directly glutamate-gated K+ ion channel. | ||
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*This means that on the binding of glutamate, the channels will open, allowing a K+ flux, which will change the voltage of the medium enough to be detected with a very sensitive electrode. | *This means that on the binding of glutamate, the channels will open, allowing a K+ flux, which will change the voltage of the medium enough to be detected with a very sensitive electrode. | ||
| - | *In order to set up a large enough K+ concentration gradient across the membrane for ions to flow down when the channels open, | + | *In order to set up a large enough K+ concentration gradient across the membrane for ions to flow down when the channels open, cells are grown in high K+ medium (100mM) and resuspended in low K+ medium. |
| - | *However, E.coli also has a number of osmoregulatory systems which use relative K+ ion concentrations to control turgor. There are K+ leak channels (Kch and Kef) in the membrane, so we have | + | *However, E.coli also has a number of osmoregulatory systems which use relative K+ ion concentrations to control turgor. There are K+ leak channels (Kch and Kef) in the membrane, so we have chosen E.coli strains with mutations in these genes as our chassis. |
[[Media:Voltage_project.ppt |Presentation]] | [[Media:Voltage_project.ppt |Presentation]] | ||
Revision as of 06:26, 28 October 2008
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