Team:Cambridge/Protocols/Gel Extraction of DNA

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==Gel Extraction of DNA==
==Gel Extraction of DNA==
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protocol description
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A technique used to isolate a desired fragment of intact DNA from an agarose gel following agarose gel electrophoresis
===Theory===
===Theory===

Revision as of 09:58, 14 July 2011

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Gel Extraction of DNA

A technique used to isolate a desired fragment of intact DNA from an agarose gel following agarose gel electrophoresis

Theory

Gel extraction or gel isolation is a technique used to isolate a desired fragment of intact DNA from an agarose gel following agarose gel electrophoresis. After extraction, fragments of interest can be mixed, precipitated, and enzymatically ligated together in several simple steps. This process is the basis for rudimentary genetic engineering.

After DNA samples are run on an agarose gel, extraction involves four basic steps: identifying the fragments of interest, isolating the corresponding bands, isolating the DNA from those bands, and removing the accompanying salts and stain.

To begin, blue-light illumination is shone on the gel in order to illuminate all the DNA fragments(stained by SYBR safe dye). The desired band is identified and physically removed with pipette with a special rectangular pipette tip. The removed slice of gel should contain the desired DNA inside.

Practice

Used QIAgen quick gel extraction kit, the protocol is adapted from the QIAgen gel extraction protocol [http://openwetware.org/images/5/5e/QIAquick_Gel_Extraction_Kit_Protocol.pdf QIAquick Gel Extraction Kit Protocol].

Safety

The safety implication of the procedure.