Difference between revisions of "Team:Munich/Parts"
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| − | <h3>Lwa Cas13a</ | + | <h3>Lwa Cas13a</h3> |
<p>To express the core piece of our project, Cas13a, we cloned the protein sequence - in this set of biobricks for the version of Leptotrichia Wadei- into a psB1C3-backbone and fused it with several elements of our part collection. | <p>To express the core piece of our project, Cas13a, we cloned the protein sequence - in this set of biobricks for the version of Leptotrichia Wadei- into a psB1C3-backbone and fused it with several elements of our part collection. | ||
By equipping the Cas13a with a T7-promoter, a Tphi-Terminator , N-terminal 6xHis/Twin-strep tag for affinity-chromatography and Sumo tag for increased solubility, we created our favorite Biobrick: BBa_K2323001, customized for expression and purification of Lwa Cas13a. | By equipping the Cas13a with a T7-promoter, a Tphi-Terminator , N-terminal 6xHis/Twin-strep tag for affinity-chromatography and Sumo tag for increased solubility, we created our favorite Biobrick: BBa_K2323001, customized for expression and purification of Lwa Cas13a. | ||
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| − | <tr><td>< | + | <tr><td><h3>Tev protease</h3> |
<p> To independently provide a tool for the removal of the affinity tag for our other Cas13a versions from Lsh and Lbu, we improved BBa_K1319004, submitted by the Aachen team 2014, coding for Tobacco Etch Virus-(TEV) protease by inserting the sequence for an N-termianl 6xHis Tag, creating BBa_K2323002 . This way we were able to express and purify the protease ourselves and could also show that it posesses high cleavage activity (https://2017.igem.org/Team:Munich/Improve). | <p> To independently provide a tool for the removal of the affinity tag for our other Cas13a versions from Lsh and Lbu, we improved BBa_K1319004, submitted by the Aachen team 2014, coding for Tobacco Etch Virus-(TEV) protease by inserting the sequence for an N-termianl 6xHis Tag, creating BBa_K2323002 . This way we were able to express and purify the protease ourselves and could also show that it posesses high cleavage activity (https://2017.igem.org/Team:Munich/Improve). | ||
This BioBrick will be useful for any future iGEM using proteins in a cell-free system. </p> | This BioBrick will be useful for any future iGEM using proteins in a cell-free system. </p> | ||
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| − | <tr><td>< | + | <tr><td><h3>Degradation Tag</h3> |
<p>We created a library of GFP-containing constructs fused to different degradation tags which are targeted by the ClpP machinery of E.coli. The degradation tags for BBa_K2323003, BBa_K2323003, BBa_K2323006, BBa_K2323007, BBa_K2323008, and BBa_K2323009 were pdt2E, ASV, LAA, LVA, and pdt2B, respectively. | <p>We created a library of GFP-containing constructs fused to different degradation tags which are targeted by the ClpP machinery of E.coli. The degradation tags for BBa_K2323003, BBa_K2323003, BBa_K2323006, BBa_K2323007, BBa_K2323008, and BBa_K2323009 were pdt2E, ASV, LAA, LVA, and pdt2B, respectively. | ||
Further, the constructs were put under control of a pTet promoter to make them inducable by aTc. | Further, the constructs were put under control of a pTet promoter to make them inducable by aTc. | ||
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| − | http://parts.igem.org/File:17-10-30_overview.png | + | <img width=900 src="http://parts.igem.org/File:17-10-30_overview.png"> |
Revision as of 23:09, 1 November 2017
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Since these tags promote degradation at different rates which are described here and in more detail on the respective registry page (http://parts.igem.org/wiki/index.php?title=Part:BBa_K2323003), this degradation tag library can be used by future teams for creation and fine-tuning of bacterial systems.
