Difference between revisions of "Part:BBa K911004"
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This part was designed as a ratiometric luciferase reporter. The first promoter, hyperSpank, is LacI - repressed and controls the transcription of a (vibrio harveyi) luxA gene that has been fused at the N-terminus to an mOrange gene via a flexible linker. This was described by Dachuan Ke and Shiao-Chun Tu (2011) as having an additional peak in its emission spectrum at 560 nm, whereas the normal peak is at 490 nm. This is terminated by b0015. Downstream, pVEG controls the translation of the entire normal lux operon, which is again terminated by b0015. | This part was designed as a ratiometric luciferase reporter. The first promoter, hyperSpank, is LacI - repressed and controls the transcription of a (vibrio harveyi) luxA gene that has been fused at the N-terminus to an mOrange gene via a flexible linker. This was described by Dachuan Ke and Shiao-Chun Tu (2011) as having an additional peak in its emission spectrum at 560 nm, whereas the normal peak is at 490 nm. This is terminated by b0015. Downstream, pVEG controls the translation of the entire normal lux operon, which is again terminated by b0015. | ||
− | + | This part was designed so that the 490nm luciferase output acts as an internal control signal, to which the intensity output of the induced luciferase with the spectral shift can be normalised. The luxA which does not produce a spectral shift will compete with the luxA which does for binding to luxB, and thus a induction-dependent ratio of 490nm to 560nm intensity produced. | |
This contruct has been designed to work in bacillus and E.coli, so all the RBSes are at the bacillus consensus. | This contruct has been designed to work in bacillus and E.coli, so all the RBSes are at the bacillus consensus. | ||
+ | Users looking for a lux operon optimised for B.subtilus may wish to use the one included within this construct, which is functional (see experience). | ||
− | There are some issues with the stability and function of this part, see experience for further details. | + | There are some issues with the stability and function of this as a whole part necessitating its submission to the registry in a non-standard backbone (BBa_k911006), see experience for further details and characterisation. We contacted the registry about this and were granted exemption from the pSB1C3 standard for this part. |
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Latest revision as of 18:13, 25 September 2012
Synthesised Ratiometric Luciferase construct in non-standard plasmid
This part was designed as a ratiometric luciferase reporter. The first promoter, hyperSpank, is LacI - repressed and controls the transcription of a (vibrio harveyi) luxA gene that has been fused at the N-terminus to an mOrange gene via a flexible linker. This was described by Dachuan Ke and Shiao-Chun Tu (2011) as having an additional peak in its emission spectrum at 560 nm, whereas the normal peak is at 490 nm. This is terminated by b0015. Downstream, pVEG controls the translation of the entire normal lux operon, which is again terminated by b0015.
This part was designed so that the 490nm luciferase output acts as an internal control signal, to which the intensity output of the induced luciferase with the spectral shift can be normalised. The luxA which does not produce a spectral shift will compete with the luxA which does for binding to luxB, and thus a induction-dependent ratio of 490nm to 560nm intensity produced.
This contruct has been designed to work in bacillus and E.coli, so all the RBSes are at the bacillus consensus. Users looking for a lux operon optimised for B.subtilus may wish to use the one included within this construct, which is functional (see experience).
There are some issues with the stability and function of this as a whole part necessitating its submission to the registry in a non-standard backbone (BBa_k911006), see experience for further details and characterisation. We contacted the registry about this and were granted exemption from the pSB1C3 standard for this part.
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12INCOMPATIBLE WITH RFC[12]Illegal NheI site found at 3988
Illegal NheI site found at 7654 - 21INCOMPATIBLE WITH RFC[21]Illegal BglII site found at 1479
Illegal BglII site found at 4330
Illegal BglII site found at 6912
Illegal BglII site found at 8389
Illegal BamHI site found at 7593 - 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 6308
- 1000COMPATIBLE WITH RFC[1000]