Team:UCSF/Project/Conjugation/Data1
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<span>CRISPRi Conjugation</span> | <span>CRISPRi Conjugation</span> | ||
- | <a href="https://2013.igem.org/Team:UCSF/Project/Conjugation/Design1">Design</a> | + | <a href="https://2013.igem.org/Team:UCSF/Project/Conjugation/Design1">Project Design</a> |
<a href="https://2013.igem.org/Team:UCSF/Project/Conjugation/Data1">Data</a> | <a href="https://2013.igem.org/Team:UCSF/Project/Conjugation/Data1">Data</a> | ||
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<span>CRISPRi Circuit</span> | <span>CRISPRi Circuit</span> | ||
- | <a href="/Team:UCSF/Project/Circuit/Design">Design</a> | + | <a href="/Team:UCSF/Project/Circuit/Design">Circuit Design</a> |
+ | <a href="/Team:UCSF/Project/Circuit/Design">Promoter Engineering</a> | ||
<a href="/Team:UCSF/Project/Circuit/Data">Data</a> | <a href="/Team:UCSF/Project/Circuit/Data">Data</a> | ||
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<p2>After the transfer of the conjugative plasmid, there is a decrease in RFP expression in strains that have received the CRISPRi system compared to the control (pARO190 backbone), which shows no significant change. Our data in the second trial seem to suggest that dCas9 expression is somewhat leaky behind our pTET promoter, for there is expression of dCas9 without induction. Since our guideRNA is constitutively expressed, this results in a small amount of specific targeting, and therefore RFP repression, without induction. It also appears that overexpression of the dCas9 protein could be somewhat toxic to the cells, so we are currently working on modifying the promoter to achieve a tighter regulation of dCas9 expression.</p2> | <p2>After the transfer of the conjugative plasmid, there is a decrease in RFP expression in strains that have received the CRISPRi system compared to the control (pARO190 backbone), which shows no significant change. Our data in the second trial seem to suggest that dCas9 expression is somewhat leaky behind our pTET promoter, for there is expression of dCas9 without induction. Since our guideRNA is constitutively expressed, this results in a small amount of specific targeting, and therefore RFP repression, without induction. It also appears that overexpression of the dCas9 protein could be somewhat toxic to the cells, so we are currently working on modifying the promoter to achieve a tighter regulation of dCas9 expression.</p2> | ||
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Latest revision as of 03:32, 29 October 2013
CRISPR Conjugation - Experiments and Results
Confirming Conjugation:
We first needed to confirm that conjugation was possible in our experimental setup. To test this, we co-cultured the donor strain (spectinomycin resistance) containing our empty pARO190 plasmid (carbenicillin resistance) with our target strain, which has RFP and chloramphenicol resistance intergrated into its chromosome (JM109-RFP). At certain time points, we took a sample of the co-cultures and selected for target strain cells that have received the conjugative plasmid, which we call “transconjugates”. On average, we obtained a conjugation efficiency of 0.4%.