Difference between revisions of "Team:Reading/Protocols"
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− | <p><title2>Taking optical density of culture to measure growth</title2> | + | <p><title2>Taking optical density of culture to measure growth</title2> </br> |
We measured the OD<sub>750</sub> to match that used in research papers on <i>Synechocystis</i><sup>1</sup>. | We measured the OD<sub>750</sub> to match that used in research papers on <i>Synechocystis</i><sup>1</sup>. | ||
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− | <p><title2>Solar water disinfection (SODIS)</title2> | + | <p><title2>Solar water disinfection (SODIS)</title2> </br> |
SODIS is an extremely cheap and simple method of sterilising water, requiring only sunlight, and Polyethylene terephthalate (PET) plastic bottles<sup>3</sup>. We used water from <a href="https://www.google.co.uk/maps/place/Whiteknights+Lake,+University+of+Reading,+Earley,+Reading,+Wokingham/@51.4416726,-0.9404284,16z/data=!3m1!4b1!4m2!3m1!1s0x487684b3ea7ada4f:0x487684b3f9714909">Whiteknights lake</a>on the University of Reading campus. | SODIS is an extremely cheap and simple method of sterilising water, requiring only sunlight, and Polyethylene terephthalate (PET) plastic bottles<sup>3</sup>. We used water from <a href="https://www.google.co.uk/maps/place/Whiteknights+Lake,+University+of+Reading,+Earley,+Reading,+Wokingham/@51.4416726,-0.9404284,16z/data=!3m1!4b1!4m2!3m1!1s0x487684b3ea7ada4f:0x487684b3f9714909">Whiteknights lake</a>on the University of Reading campus. | ||
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− | <p><title2>Miniprep: Isolation of plasmid DNA from bacteria</title2> | + | <p><title2>Miniprep: Isolation of plasmid DNA from bacteria</title2> </br> |
We used the Thermo Scientific GeneJET Plasmid Miniprep Kit<sup>4</sup> for our miniprep. This protocol closely follows protocol A, which is detailed in the booklet included in the kit. | We used the Thermo Scientific GeneJET Plasmid Miniprep Kit<sup>4</sup> for our miniprep. This protocol closely follows protocol A, which is detailed in the booklet included in the kit. | ||
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Revision as of 10:45, 1 September 2015
Note: This section is an account of all laboratory protocols used by the team this year. The references at the bottom of the page provide the sources for the protocols, however we have modified several of them to our needs.
- Thaw stock of 6803 on ice
- 100ml of BG-11 medium added to sterile conical flask aseptically
- Add 10µl or 5 loopfuls of 6803 to flask
- Incubate at ~30°C and on shaker at ~58rpm, under constant illumination
- Check growth each day by measuring OD750
- Set spectrophotometer to measure at OD750
- Blank with 1ml of BG-11
- Take OD750 of 1ml of culture
- If OD750 over 1 a.u, dilute 250µl of culture in 750µl of BG-11 (1/4 dilution)
- Pass water through a filter into a PET bottle to remove particulates
- Seal bottle and place in sunlight. Leave bottle exposed to intense sunlight for a minimum of 6 hours
- Pellet cells from 1.5ml of culture by centrifugation at 4000rpm for 2 minutes, and remove as much supernatant as possible and discard, leaving only the pellet.
- Resuspend pellet in 250µl of Resuspension Solution by vortexing breifly until pellet no longer visable.
- Lyse cells by adding 250µl of Lysis Solution and mixing thoroughly by inverting the tube 4-6 times until solution becomes viscous and clear
- Add 350µl of Neutralisation Solution and mix immediately and gently until solution becomes cloudy.
- Centrifuge for 5 minutes at 12,000rpm
- Transfer supernatant to a GeneJET spin column. Avoid disturbing white precipitate.
- Centrifuge for 1 minute at 12,000rpm and discard the flow-through.
- Add 500µl of Wash Solution to GeneJET spin column, centrifuge for 1 minute at 12,000rpm, and discard flow-through.
- Repeat step 8.
- Discard flow-through and centrifuge for 1 minute at 12,000rpm to remove residual Wash Solution.
- Transfer GeneJET spin column to a fresh 1.5ml microcentrifuge tube. Add 50µl of Elution Buffer, being careful not to touch the membrane with the pipette.
- Incubate at room temperature for 2 minutes and then centrifuge for 2 minutes at 12,000rpm
- Discard GeneJET spin column and store purified plasmid DNA at -20°C.
BG-11 plates are used to grow Synechocystis sp. PCC 6803 strains. Antibiotics are added as needed for selection. 1.5% agar is used.
- Add 7.55 g of agar to 500 ml BG-11 and autoclave to sterilise
- If making kanamycin plates cool to ~55℃ and add 50 ug/ml
- Agar melted in steamer and kept at 55℃ until needed for pouring
If making a kanamycin cap:
- 0.6% agar w/v
- Cool BG-11 to ~55ºC and add 0.5mg/ml kan
- Add ~3ml to a plain BG-11 plate with transformed colonies on it
- Leave for >1 week for Kan selection to occur
- Bradley, R. W., Bombelli, P., Lea-Smith, D. J. & Howe, C. J. Terminal oxidase mutants of the cyanobacterium Synechocystis sp. PCC 6803 show increased electrogenic activity in biological photo-voltaic systems. Phys. Chem. Chem. Phys. PCCP 15, 13611–13618 (2013).
- Pojidaeva E, Zichenko V, Shestakov SV, Sokolenko A (2004) Involvement of the SppA1 peptidase in acclimation to saturating light intensities in Synechocystis sp. strain PCC 6803. J Bacteriol 186: 3991–3999.
- SODIS. 2015. SODIS Method, Available at: href="http://www.sodis.ch/methode/index_EN
- ThermoScientific. 2013. Thermo Scientific GeneJET PCR Purification Kit #K0701, #K0702. [Online] Available at: https://www.lifetechnologies.com/order/catalog/product/K0502?ICID=search-k0502