Team:TU-Eindhoven/LEC/Lab

From 2012.igem.org

(Difference between revisions)
Line 15: Line 15:
<p>To reach the aim of this project and prepare a multi-colored screen, three kind of cells, each with a different color, are needed. Therefore, one single plasmid strain would have to consist of both calcium channel parts MID1 and CCH1 sequences and one of the fluorescent GECO protein sequence. Each of these DNA sequences, coding for the three different parts, is transformed into a yeast plasmid (InvSC1). Moreover, each of these sequences contain a small sequence coding for an amino acid, causing the yeast strain to be able to synthesize this specific amino acid. The synthesis of this specific amino acid will allow strain selection by retaining this amino acid from the culture media. Cells containing the  coding CCH1, MID1 and GECO sequence are able to synthesize leucine, uracil and tryptophan respectively. </p>
<p>To reach the aim of this project and prepare a multi-colored screen, three kind of cells, each with a different color, are needed. Therefore, one single plasmid strain would have to consist of both calcium channel parts MID1 and CCH1 sequences and one of the fluorescent GECO protein sequence. Each of these DNA sequences, coding for the three different parts, is transformed into a yeast plasmid (InvSC1). Moreover, each of these sequences contain a small sequence coding for an amino acid, causing the yeast strain to be able to synthesize this specific amino acid. The synthesis of this specific amino acid will allow strain selection by retaining this amino acid from the culture media. Cells containing the  coding CCH1, MID1 and GECO sequence are able to synthesize leucine, uracil and tryptophan respectively. </p>
<p>Looking at Scheme 1, which represents the transformations needed to come to the desired yeast strain, it seems and is logical to start with the MID1 or CCH1 vectors. By doing so, less transformations can be performed due to the transformation intensive introduction of the three different GECO proteins at last. To make sure that the transformations would lead to the desired strain, it was decided to start the first step with transforming all possibilities. When step one was transformed successfully, visualized by the arrows in Scheme 1, the transformation of step two was performed and so on.</p>
<p>Looking at Scheme 1, which represents the transformations needed to come to the desired yeast strain, it seems and is logical to start with the MID1 or CCH1 vectors. By doing so, less transformations can be performed due to the transformation intensive introduction of the three different GECO proteins at last. To make sure that the transformations would lead to the desired strain, it was decided to start the first step with transforming all possibilities. When step one was transformed successfully, visualized by the arrows in Scheme 1, the transformation of step two was performed and so on.</p>
-
[[File:Transformation chart.png|500px|link=]]
+
[[File:Transformation chart.png|700px|link=]]
<p>The several transformation steps are clarified in Scheme 1. The arrows represent a successful transformation as at the same time the lack of an arrow represents a transformation failure. Of course, not every transformation was needed to obtain the desired strain. E.g. in step one the transformation of the R-GECO failed, however, the strain containing the R-GECO was obtained in step two due to other successful transformations.  
<p>The several transformation steps are clarified in Scheme 1. The arrows represent a successful transformation as at the same time the lack of an arrow represents a transformation failure. Of course, not every transformation was needed to obtain the desired strain. E.g. in step one the transformation of the R-GECO failed, however, the strain containing the R-GECO was obtained in step two due to other successful transformations.  
<p>As can be seen, in step 2 the first co-transformation are performed. This brought some complications because the regular transformation protocol did not work for these co-transformations. For the co- and co-co-transformations (performed in step 3) we used another high-efficiency transformation [[Team:TU-Eindhoven/Protocols|protocol]] which worked out successfully. After 3 steps of transformations, a couple of different transformation paths reached the three desired strains a complete calcium channel and one of the three GECO proteins.</p>
<p>As can be seen, in step 2 the first co-transformation are performed. This brought some complications because the regular transformation protocol did not work for these co-transformations. For the co- and co-co-transformations (performed in step 3) we used another high-efficiency transformation [[Team:TU-Eindhoven/Protocols|protocol]] which worked out successfully. After 3 steps of transformations, a couple of different transformation paths reached the three desired strains a complete calcium channel and one of the three GECO proteins.</p>

Revision as of 01:02, 27 September 2012