Team:EPF-Lausanne/Protocols/Gel purification

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{{:Team:EPF-Lausanne/Templates/Header|title=Gel purification}}
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{{:Team:EPF-Lausanne/Templates/ProtocolHeader|title=Gel purification}}
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Purpose: to purify a band on a gel
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'''Purpose''': separate and extract products of a PCR.
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After having verified that the electrophoresis gives you the expected fragments, re-do an electrophoresis while using the thicker combs. You can put up to 25-30 ul in the wells.
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First, cut out the band from the gel
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'''General idea''': The PCR products are separated by gel electrophoresis, then mechanically cut out with the gel. The DNA is then extracted from each gel fragment.
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* Take the black box off the UV plate
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* Hold the anti-UV shield with one hand and switch on the UV light
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* Cut around the band, switch off the UV light and put the removed band in an eppendorf tube
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Then, to extract the DNA from the gel, use the Qiagen gel purification kit.
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Run a first electrophoresis with a low volume of PCR product, to verify the expected fragments were produced. If that is the case, run a new electrophoresis with all the PCR product, using a thicker combs to make larger wells. The well from our thick comb contain up to 25 or 30 ul.
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* To weight your samples, tare the scales with an empty tube
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* In the elution step, when you have to centrifuge the column in a new Eppendorf tupe, make sure the lid of the tube flies behind in the centrifugator. It turns counterclockwise.
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'''Warning''': the PCR products destined to extraction must be exposed to minimal amounts of UV radiation, to avoid any damage to DNA.
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== Equipement ==
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* '''Gel electrophoresis setup'''
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* '''Scalpel'''
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* '''Eppendorf tubes''': As many as there are gel samples. The 2 ml ones are necessary if more than 0.3 mg of gel is to be treated.
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* '''Qiagen QIAquick gel extraction kit (250)''': make sure the protocol is inside.
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* '''UV plate reader''' and UV-shield.
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== Cutting the gel ==
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From the first (low-volume) gel, determine which bands contain the PCR products. If necessary, adjust the duration of the second electrophoresis to increase spacing between bands.
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* Prepare as many Eppendorf tubes as PCR products to extract. Weigh them.
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To cut out a desired band from the gel:
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* Lift the black camera box off the UV plate.
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* Fix the anti-UV shield on the front of the device; switch on the UV light.
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* Quickly identify the desired band, cut around it, and switch off the UV light.
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* Remove the cut-out gel and store in an Eppendorf tube.
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* ''Clean the scalpel with DI water before cutting each band'' to avoid cross-contamination.
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'''Notes''':
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* Cut out as little gel as possible, i.e. cut out as close to the band as possible. This will ease the gel extraction.
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== DNA Extraction ==
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Then, to extract the DNA from the gel, use the Qiagen gel purification kit. Follow the included protocol.
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=== Supplementary notes ===
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* Weigh each sample on the microbalance, after taring with an empty tube.
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* In the elution step, when you have to centrifuge the column in a new Eppendorf tube, the tube's lid cannot be closed. Leave it open in the centrifuge, oriented towards the bottom right (i.e. behind the tube, as the platter rotates counter-clockwise).
{{:Team:EPF-Lausanne/Templates/Footer}}
{{:Team:EPF-Lausanne/Templates/Footer}}

Latest revision as of 08:49, 15 July 2011