Team:Heidelberg/Project/Mouse Infection
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(4) The on-targeting construct consisted of two independent viruses which were co-infected into mice, as well. One of these viruses packaged the Tet Repressor (TetR) driven by an SV40 promoter. The expression of TetR is under the control of miR-122 as four binding sites of this miRNA were cloned into the 3’UTR of the gene. The second virus was composed of an sv40 promoter driving the Tet operator (TetO2) which monitors the expression of luc2. With this setup, luc2 expression should be inhibited by the TetR in all mice tissues except for liver cells, where TetR is downregulated by miRNA 122. | (4) The on-targeting construct consisted of two independent viruses which were co-infected into mice, as well. One of these viruses packaged the Tet Repressor (TetR) driven by an SV40 promoter. The expression of TetR is under the control of miR-122 as four binding sites of this miRNA were cloned into the 3’UTR of the gene. The second virus was composed of an sv40 promoter driving the Tet operator (TetO2) which monitors the expression of luc2. With this setup, luc2 expression should be inhibited by the TetR in all mice tissues except for liver cells, where TetR is downregulated by miRNA 122. | ||
- | === | + | ===Virus Production=== |
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+ | The viruses were produced on HEK 293-T cells and purified on an iodixanol gradient according to [https://2010.igem.org/Team:Heidelberg/Notebook/Methods#Virus_Production protocol]. | ||
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+ | Before infection, the titer of the viruses was quantified using .[https://2010.igem.org/Team:Heidelberg/Notebook/Methods#Quantitative_Realtime_PCR quantitative realtime PCR] | ||
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===mice injection=== | ===mice injection=== | ||
In order to assess tissue tropism of the The TVroute was chosen so as to assess AAV serotype tissue tropism; | In order to assess tissue tropism of the The TVroute was chosen so as to assess AAV serotype tissue tropism; |
Revision as of 13:52, 25 October 2010
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