Team:ETH Zurich/Design

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Contents

Design of the single parts

UVR8

Three different fusion strategies were carried out to verify the best UVR8 dTetR fusion. Tet DBD stands for TetR DNA binding domain.

1. Full length UVR8 without a linker

Ethuvr81.jpg


2. Full length UVR8 + [GGS]x2 linker (+6 aa)

Uvr83rdeth.jpg


3. Truncated UVR8 (-13 aa which are not seen in the 3d structure)

Uvr82ndeth.jpg
Uvr8uv.jpg



p-ABA generator

We constructed one operon consisting of the pabA and pabB/C gene from Lactococcus Lactis to overexpress p-ABA. Therefore we used the biobrick parts K137055 and S04039 as a template. In a second step the pab operon was cloned downstream to the Tet promoter so that derepression of UVR8 leads to p-ABA expression as a response to UV radiation.


Dual input promoters

In our case we want the [decoder][1] to have AND logics. Therefore we designed 3 different promoters, all of them derived from the Lambda-phage promoters PR and PL.

Promoterr.jpg

UVR8

UVR8


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