Team:Todai-Tokyo/Protocols/Gel Extraction

Gel Purification Protocol

 * 1) Cut out volume of agarose gel containing the desired DNA and put in an eppendorf tube
 * 2) Use the Promega Gel Purification kit according to instructions
 * 3) Elute DNA with 50µl of MilliQ (or 30µl if yield is low)
 * 4) Measure concentration using a spectrophotometer and write on tube