From 2009.igem.org

Revision as of 16:36, 21 October 2009 by Francesca ceroni (Talk | contribs)

(diff) ← Older revision | Latest revision (diff) | Newer revision → (diff)

HOME	TEAM	PROJECT	SOFTWARE	MODELING	WET LAB	PARTS	HUMAN PRACTICE	JUDGING CRITERIA

Project Summary

Which is our idea?

The project aims to design a new device to control the synthesis of a protein in Escherichia coli regardless of the protein to be controlled. This "general-purpose" standard device acts on translation to allow a faster silencing of protein expression if compared to standard regulated promoters. We named this device T-Rex (Trans Repressor of Expression).

How does T-Rex work?

The device consists of two new BioBricks (see Fig.1):

CIS-repressing, to be assembled upstream of the target coding sequence.

TRANS-repressor, complementary to the CIS-repressing and placed under the control of a different promoter.

CIS-repressing and TRANS-repressor were designed using our [[Team:Bologna/Software#1|BASER]] tool.

Fig.1

Transcription of the target gene produces a mRNA strand, starting with the Cis element, which is translated into proteins by ribosome. Trans’ promoter induction produces a transcript that binds with the Cis part. The RNA duplex prevents ribosome from binding to RBS, repressing protein synthesis. Thus, the TRANS-repressor amount regulates the gene mRNA translation rate. </font> How can we test the device?

In order to test and characterize our T-REX device, we developed the following genetic circuit:

The T-REX device is proposed as a universal and fast switch in synthetic gene circuits.

More details about our work in the Project section.

Acknowledgements

University of Bologna

Ser.In.Ar. Cesena

Cultural Association San Sebastiano

Up