Part:BBa_I739102

Double Promoter (cI, negative / TetR, negative)

Part Structure

The Biobrick consists of the whole non-constitutive promoter BBa_R051 linked to twice the first operator sequence of BBa_R0040 (TetR 1).

The -35 and -10 regions, which are responsible for the binding of RNA-polymerase to DNA via sigma factors, are included in the BBa_R0051 promoter region (first part of the double promoter). No further functional -10 and -35 regions were included in the second part of the double promoter. Instead, two operator sequences of the same type were included in the second part. The reason for this is that the probability of a binding event (and hence regulation strength) is increased if a multiple of identical operator sequences is included in the regulatory sequence.

Summarized:
There are four operator sequences: 1xBBa_R0051 (OR 2), 1xBBa_R0051 (OR 1), 2xBBa_R0040 (TetR 1).

Mode of Action

Regulation of the first part: When lambda cI binds to the cI operator sequences, it represses transcription. There is no inducer which derepresses the promoter upon addition.

Regulation of the second part: When TetR binds to the TetR operator sequences, it represses transcription. If the inducer [http://openwetware.org/wiki/ATc anhydrotetracycline (ATc)] is added, TetR action is inhibited and the promoter gets derepressed.

Purpose

This Biobrick was designed for the [http://2007.igem.org/ETHZ ETHZ iGEM 2007 project] and belongs to a first generation of double promoters. BBa_I739102 is part of biobrick BBa_I739004.

Testing

Checked for uniqueness of restriction enzyme cleavage sites:
Eco: ok
Xba: ok
Spe: ok
Pst: ok

Sequence and Features