Team:UCSF/Data
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+ | <h2red>(For images of strains expressing Hwp1, Cadherin, and Mgfp-5 please see the individual Parts pages.) </h2red><p> | ||
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<h3red>EBY100 (-)control </h3red> <p> | <h3red>EBY100 (-)control </h3red> <p> | ||
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<h3red>Mgfp5</h3red> <p> | <h3red>Mgfp5</h3red> <p> | ||
- | <regulartext><p> </regulartext> | + | <regulartext>Since Mgfp5 is an adhesive protein from mussel, we believed that if we added more salt to the liquid cultures, the cells expressing the proteins would have a higher chance of adhering. We discovered that an increase of salt in the liquid cultures caused larger clumps. <p> </regulartext> |
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<h3red>Other Proteins</h3red> <p> | <h3red>Other Proteins</h3red> <p> | ||
- | <regulartext>We did not | + | <regulartext>We also tried to express many other proteins but they did not function the way we expected them to when we observed the cells under the microscope. Eap1 was supposed to bind itself, but it didn’t. We thought that ZipRR and ZipEE, both leucine zippers, would to bind to one another, but they didn’t. ALS3 was believed to bind to itself and mammalian proteins, but it wasn’t show to bind to itself under the microscope. Cul3 is a hydrophobic protein but we were unable to determine if the cells expressing Cul3 were floating in our microscopy tests. BCL2 and BIM were supposed to adhere to each other but they were unsuccessful from what we observed under the microscope. <p> </regulartext> |
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Latest revision as of 03:43, 29 September 2011