Team:EPF-Lausanne/Protocols/Miniprep

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(Miniprep)
 
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{{:Team:EPF-Lausanne/Templates/Header|title=Miniprep}}
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{{:Team:EPF-Lausanne/Templates/ProtocolHeader|title=Plasmid preparation - Miniprep}}
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The miniprep is used to extract plasmids from a bacterial colony. The bacteria cells are lysed to release the plasmids, then the plasmids are filtered out, and finally their concentration is measured.
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Plasmid preparation procedure known as "miniprep" is used to extract plasmids from small bacterial cultures. Bacteria undergo alkaline lysis to release the plasmids, while genomic DNA stays bound to cell structures. Cell debris are eliminated by centrifugation and the supernatant containing plasmids is loaded to a DNA binding column, it is first washed, than DNA is eluted. DNA conentration can be measured with a spectrophotometer.
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'''TODO''': could somebody please provide some details on how the colonies are made?
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For miniprep procedure bacterial cultures are grown overnight in 5ml LB with with antibiotic. These cultures are started from a single colony grown on a LB-agar plate, usually the selection plate after transformation or it can be a streak of glycerin stock. 
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* '''Invitrogen PureLink Quick miniprep kit''': white and red box, kept in the storage room.
* '''Invitrogen PureLink Quick miniprep kit''': white and red box, kept in the storage room.
* '''Resuspension Buffer''': kept in the fridge. It's part of the miniprep kit, but kept cool since it contains RNAase.
* '''Resuspension Buffer''': kept in the fridge. It's part of the miniprep kit, but kept cool since it contains RNAase.
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* '''Centrifuge'''
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* '''Centrifuge''' with a rotor for Eppendorf tubes
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* '''Nanodrop 1000 Spectrophotometer''': on the left on the computer at the entrance of Sebastian's lab.
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* '''Nanodrop 1000 Spectrophotometer''': on the left of the computer at the entrance of Sebastian's lab.
=== Notes ===
=== Notes ===
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=== Miniprep ===
=== Miniprep ===
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All the steps of the miniprep are described in the instruction leaflet that is included in the miniprep kit. The plasmids are filtered by centrifuge, rather than by vacuum. Just heed these extra warnings:
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All the steps of the miniprep are described in the instruction leaflet that is included in the miniprep kit. For steps with DNA binding column centrifuge is used, rather than vacuum. Just heed these extra warnings:
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* To "resuspend", wash the solution up and down in a micropipette. Be careful to '''not create any foam'''.
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* To "resuspend", wash the solution up and down in a micropipette. Be careful to '''not create foam'''.
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* Return the resuspension buffer to the refrigerator once it is no longer used.
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* Return the resuspension buffer to the refrigerator when it is not longer needed.
=== Concentration measurement ===
=== Concentration measurement ===
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Plasmid concentration is finally measured using the Nanodrop 1000 photospectrometer. It is controlled by the "ND-1000" software (icon on the desktop).
Plasmid concentration is finally measured using the Nanodrop 1000 photospectrometer. It is controlled by the "ND-1000" software (icon on the desktop).
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* '''Load nucleic acid program''': if necessary, click "exit" to return to the main menu, then "Nucleic Acid". Initialise as instructed, by depositing a ul drop of water on the sensor.
* '''Calibrate the spectrometer''': deposit a 1 ul drop of buffer solution onto the sensor, and click the "blank" button.
* '''Calibrate the spectrometer''': deposit a 1 ul drop of buffer solution onto the sensor, and click the "blank" button.
* '''Measure plamsid concentration''': deposit 1 ul of plasmid solution onto the sensor, and measure with the "measure" button. The reported plasmid concentration is considered valid if the "260/280" ratio is larger than 1.80.  
* '''Measure plamsid concentration''': deposit 1 ul of plasmid solution onto the sensor, and measure with the "measure" button. The reported plasmid concentration is considered valid if the "260/280" ratio is larger than 1.80.  
{{:Team:EPF-Lausanne/Templates/Footer}}
{{:Team:EPF-Lausanne/Templates/Footer}}

Latest revision as of 08:49, 15 July 2011