Team:WITS-South Africa/Machine Design

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===Machine Testing===
===Machine Testing===
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A culture of 2ml of ''E. coli''-containing Lacto-detect was grown overnight at 37^{o}C and then transfered to 25 ml of ampicillin LB broth. This innoculent was grown at 37^{0}C in a shaking incubator for 2.5 hours so as to ensure that the bacteria were in their exponential growth phase. A baseline reading was taken at this point (tile A), after which 10% 1mM IPTG was added and then returned to the shaking incubator. An aliquot was then imaged after 30min (tile B) and again after 1 hour (tile C). All aliquots used in imaging were 100 ul. <br /> <br />
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Once the induction of Lacto-detect had reached an appreciable level, it was added to an aliquot of ''B. subtilis'' containing a construct driven by the PlcR promoter. Baseline images of both Lacto-detect (tile A) and the ''B. subtilis'' population (tile B) are given as well as a combined baseline image (tile C). <br /> <br />
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Revision as of 14:19, 27 October 2010


Contents

Lacto-detect

Purpose:

a) To act as the ‘Detector’ Machine within the population and produce the quorum signalling peptide in response to an input signal


Wits Machine 1 wiki.jpg


So how did we end up selecting the final parts of our Machines? Each one was chosen after much consideration and scouring of the literature to select the most suitable biological system. For a design rationale of why we selected the parts that we did to create this machine, click here

For an account of how we assemblied and verified Lacto-detect, click here

Lacto-report

Wits Machine 2.jpg

For a design rationale of why we selected the parts that we did to create this machine, click here

We were not able to finish constructing Lacto-report in it's entirety, due to time constraints and issues with the E.chromi Biobrick parts. (For more details, click here.)

For testing and characterising the behaviour of the quorum sensing mechanism in a model Gram-positive bacillus, we used an intermediate machine construct we dubbed Lacto-

Lacto-test

Purpose:

a) To show that the PlcR promoter is activated in L. gasseri by measuring fluorescence after the addition of exogenous PlcR and PapR proteins

Wits Lacto-test.jpg


Machine Testing


A culture of 2ml of E. coli-containing Lacto-detect was grown overnight at 37^{o}C and then transfered to 25 ml of ampicillin LB broth. This innoculent was grown at 37^{0}C in a shaking incubator for 2.5 hours so as to ensure that the bacteria were in their exponential growth phase. A baseline reading was taken at this point (tile A), after which 10% 1mM IPTG was added and then returned to the shaking incubator. An aliquot was then imaged after 30min (tile B) and again after 1 hour (tile C). All aliquots used in imaging were 100 ul.

Montage of M1I d.jpg



Once the induction of Lacto-detect had reached an appreciable level, it was added to an aliquot of B. subtilis containing a construct driven by the PlcR promoter. Baseline images of both Lacto-detect (tile A) and the B. subtilis population (tile B) are given as well as a combined baseline image (tile C).

Montage of Mixed.jpg