Team:EPF Lausanne
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We are now in our first week in the wet lab. Apart from training basic lab skills like making a PCR and running a gel we are growing Asaia and studying its properties. Furthermore we finished our first biobrick containing an origin of replication for Asaia. | We are now in our first week in the wet lab. Apart from training basic lab skills like making a PCR and running a gel we are growing Asaia and studying its properties. Furthermore we finished our first biobrick containing an origin of replication for Asaia. | ||
Within the next week we also plan to test the propagation of Asaia within Drosophila.<br><br> | Within the next week we also plan to test the propagation of Asaia within Drosophila.<br><br> | ||
- | ''' | + | '''Our plan:'''<br> |
The bacterium Asaia was chosen as a chassis mainly since it is naturally present in the mosquitoes gut. Furthermore it is transmitted vertically (to the offspring) and horizontally (during reproduction) which enables the engineered Asaia to propagate within a mosquito population. | The bacterium Asaia was chosen as a chassis mainly since it is naturally present in the mosquitoes gut. Furthermore it is transmitted vertically (to the offspring) and horizontally (during reproduction) which enables the engineered Asaia to propagate within a mosquito population. | ||
We have discussed several ways of blocking the Plasmodium in the gut of the mosquito. We plan to test the following two approaches: | We have discussed several ways of blocking the Plasmodium in the gut of the mosquito. We plan to test the following two approaches: | ||
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* p25 p28 are ookinete (a specific form of the plasmodium) surface proteins. It has been shown [2] that if these proteins are missing the formation of ookinetes and the transformation of plasmodium to the next stage are inhibited. We therefore want to engineer Asaia to inhibit these proteins. <br> | * p25 p28 are ookinete (a specific form of the plasmodium) surface proteins. It has been shown [2] that if these proteins are missing the formation of ookinetes and the transformation of plasmodium to the next stage are inhibited. We therefore want to engineer Asaia to inhibit these proteins. <br> | ||
The next step is to achieve a release of the toxin or the receptors into the gut of the mosquito. This could be done by lysis of the cells or ideally by secretion. | The next step is to achieve a release of the toxin or the receptors into the gut of the mosquito. This could be done by lysis of the cells or ideally by secretion. | ||
- | As a last and very challenging step we consider the option of a blood sensor, which triggers lysis or secretion. This would greatly increase the probability that there is a sufficient amount of immunotoxin to stop the plasmodium from being able to travel to the salivary gland and hence being transmitted to the next victim. | + | As a last and very challenging step we consider the option of a blood sensor, which triggers lysis or secretion. This would greatly increase the probability that there is a sufficient amount of immunotoxin to stop the plasmodium from being able to travel to the salivary gland and hence being transmitted to the next victim.<br> <br> |
+ | <font size="1.5"> | ||
+ | [1] http://www.ncbi.nlm.nih.gov/pmc/articles/PMC1885625/ <br> | ||
+ | [2] http://www.nature.com/emboj/journal/v20/n15/full/7593895a.html </font> | ||
Revision as of 13:41, 15 July 2010
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Our project:
The next step is to achieve a release of the toxin or the receptors into the gut of the mosquito. This could be done by lysis of the cells or ideally by secretion.
As a last and very challenging step we consider the option of a blood sensor, which triggers lysis or secretion. This would greatly increase the probability that there is a sufficient amount of immunotoxin to stop the plasmodium from being able to travel to the salivary gland and hence being transmitted to the next victim.
[1] http://www.ncbi.nlm.nih.gov/pmc/articles/PMC1885625/
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