Team:Edinburgh/Bacterial/Blue light producer

From 2010.igem.org

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<p>The LuxAB which last year's team made and stored is failing to transform correctly. Colonies that ought to be growing white are growing blue (LuxAB should have replaced the <i>lacZ'</i> in the vector, EdinbrickI). A similar thing is happening with LumP and RFP, where cells are still growing red, despite the fact that the RFP ought to have been removed when LumP was inserted last year.</p>
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<p>Last year’s LuxAB and LumP parts were having some problems (blue and red colonies were growing when they should not be. This was part of the reason for resubmitting them, as the parts in the registry may have the same problems. </p>
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<p>We have come across several PCR products not yet inserted into vectors with which we are hoping to start this part of the project (i.e. the bit which should already have been done by last year according to their lab notes) again.</p>
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<p>We have also had issues with the instrument used to measure the spectral output. It could not pick up a signal from the tubes despite visible bioluminescence. Hopefully we will be able to characterise these parts more fully before the Jamboree.
<p>We have also had issues with the instrument used to measure the spectral output. It could not pick up a signal from the tubes despite visible bioluminescence. Hopefully we will be able to characterise these parts more fully before the Jamboree.

Revision as of 17:53, 27 October 2010







Overview: The blue light producer


To produce blue light, we used two systems using the bacterial luciferase from Xenorhabdus luminescens (LuxAB). The standalone LuxAB has an emission peak of 495nm. (Figure 1). According to O'Kane and Lee (1985) and others, the addition of lumazine protein shifts the wavelength towards blue (478 nm), to be in the correct region to activate the blue light sensor.




Figure 1: Emission spectra of LuxAB (in solid black line). The LuxAB depicted is that from Vibrio campbellii, but sources confirm that other bacterial luciferases produce similar spectral graphs.

Image: Suadee et al. (2008)



Strategy


Last year's Edinburgh team already made both of these parts individually, so all we had to do was fuse them together and add a promoter before. Individual parts were resubmitted in pSB1C3.



Problems


Last year’s LuxAB and LumP parts were having some problems (blue and red colonies were growing when they should not be. This was part of the reason for resubmitting them, as the parts in the registry may have the same problems.

We have also had issues with the instrument used to measure the spectral output. It could not pick up a signal from the tubes despite visible bioluminescence. Hopefully we will be able to characterise these parts more fully before the Jamboree.



BioBricks


Both lumP and luxAB have already been submitted as BioBricks in pSB1A3 by last year's Edinburgh team, but we are re-submitting corrected variants in pSB1C3.

We are also submitting a luxAB-lumP fusion construct in pSB1C3 with a constitutive promoter which can be used for blue light production. We have confirmation of working luxAB with the promoter in question.


BBa_K322139: bacterial luciferase luxAB, updated version of BBa_K216008.

BBa_K322312: luxCDE (required for luxAB expression), updated version of BBa_K216017.

BBa_K322007: lumP (shifts luxAB to blue), updated version of BBa_K216007.

BBa_K322140: luxAB under lac promoter.

BBa_K322141: luxAB and luxCDE under lac promoter.

BBa_K322149: luxAB and lumP composite part.

BBa_K322150: luxAB and lumP under lac promoter.



Characterisation


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References


O'Kane, D. J. & Lee, J. (1985). Chemical characterization of lumazine protein from Photobacterium leiognathi: comparison with lumazine protein from Photobacterium phosphoreum. Biochemistry 24, 1467-1475.

Suadee, C., Nijvipakul, S., et al. (2008). LuxG Is a Functioning Flavin Reductase for Bacterial Luminescence. J. Bacteriol. 190(5): 1531-1538

Edinburgh 2009 team wiki, https://2009.igem.org/Team:Edinburgh.




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