Team:NTU-Singapore/Wetlab/Materials and Equipment

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- Victor 3 multilabel reader was used to measure RFU value of yellow fluorescent protein (YFP) using excitation filter of 490 nm and emission filter of 535 nm.
- Victor 3 multilabel reader was used to measure RFU value of yellow fluorescent protein (YFP) using excitation filter of 490 nm and emission filter of 535 nm.
- Absorbance-meter was used to measure OD600 values.
- Absorbance-meter was used to measure OD600 values.

Revision as of 07:33, 26 October 2008



Contents

Materials

Preparation of AI-2

Pure AI-2 is very difficult to harvest or synthesize. However, as a quorum sensing messenger, AI-2 is present in intercellular medium in considerable amount. In this project, AI-2 was indirectly harvested by obtaining cell supernatants at different time points of cell growth. Glucose was added to the growth medium as it promotes AI-2 production significantly (Liang Wang, 2005).

A colony of E. coli W3110 was grown overnight in LB for 16 hours at 37°C . The overnight culture was then diluted in LB plus 0.8% glucose to an optical density at 600 nm (OD600) of 0.02. The cells were incubated at 37°C with shaking at 225 rpm in 500ml Erlenmeyer flask. Cell aliquots were removed at each time point for measurement of the OD600. The measured values were shown in the following table:

Time (hrs) OD of W3110
0 0.002
1 0.047
2 0.112
3 0.341
4 0.628
5 0.921
6 1.032
7 1.172
8 1.252

Based on the data, a graph of OD600 versus time was constructed as below:

OD of W3110 vs time

Maximal AI-2 production activity is typically observed during mid- to late exponential phase (Surette, 1998). Therefore, 4ml of samples corresponding to 2, 3, 3.333, 3.667, 4, 6 time points were collected and centrifuged at 13,200 rpm for 10 min in a microcentrifuge to separate cell pellets from supernatants. Cleared supernatants were filtered using 0.2 µm pore size filters to remove unwanted big proteins. Supernatants were stored at -20°C.

Bacteria strains and media

Bacteria used in all the experiments were LuxS mutants derived from the wild type E coli strain W3110. By knocking out LuxS gene, the cells were unable to synthesize AI-2. As a result, lsrA promoter could only be induced in the presence of external AI-2 produced by other bacteria rather than the host cells. LuxS mutants were first made chemically competent in order to be able to take in biobrick plasmids during transformation. The media used for overnight growth of cells were Luria-Bertani broth (LB). Cells were diluted in M9 media to an OD600 of 1 before ready to be read under Fluorescence Microplate Reader or Absorbance reader.

Plasmid construction

All the plasmids used were in the standard biobrick form as regulated by the Biobricks Registry at MIT. The plasmid containing plsrA-YFP was used for characterization of lsrA promoter, while plsrA-celE7-Terminator plasmid (detection system) aimed to show the lysis of cells when exposed to AI-2.

Insert Vector Subparts Name in Registry
pLsrA-YFP pSB1A3 BBa_K117002
BBa_E0430
BBa_K117008
plsrA-celE7-Terminator pSB1A3 BBa_K117002
BBa_K117006
BBa_K117010

Equipments

- Victor 3 multilabel reader was used to measure RFU value of yellow fluorescent protein (YFP) using excitation filter of 490 nm and emission filter of 535 nm.

- Absorbance-meter was used to measure OD600 values.