Igem2010/Main/Homology Based/October
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==08/10/2010== | ==08/10/2010== | ||
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+ | - A non-ITR AAV helper vector was obtained and maxi-preped to clone into it the cap genes from the 50 single clones picked. | ||
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+ | ==09/10/2010== | ||
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+ | - The non-ITR vector was cut with AscI and PacI, and so was the pTR-UF3 containg cap genes from the 50 clones. The bands were purified from the gel. | ||
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+ | ==10/10/2010== | ||
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+ | * The cap genes were ligated into the non-ITR vector, and Hek 293 cells were prepared in 24-well plates for transfection. | ||
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+ | * The first selection round Huh-7 cells infect with AAV library and Adeno-virus 5 were monitored under the microscope, and the typical cytopathic effect caused by Adeno-5 infection (roundening of cells) was observed. Cells were harvested by washing the wells with the media (in this case, one well of the 6-well plate was used). | ||
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+ | ==11/10/2010== | ||
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+ | * The harvested cells from the previous day were incubated at 56 ͦC for 20 min to inactivate adeno virus 5. Then, freeze-thaw cycles (between liquid nitrogen and 37ͦC, see above) were carried out to lyse the cells and get the AAVs out. A 5-minute centrifugation at full speed was then done, and the supernatant containing the 1st selection round AAVs was collected and aliqueted and stored at -20ͦC (initial freezing with liquid nitrogen), or used immediately to infect the 2nd-selection-round Huh-7 cells as follows: | ||
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Latest revision as of 18:24, 26 October 2010
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