I understand that PFU taq have proofreading activity, therefore can reduce error during amplification, therefore it is recommended to use polymerase with pfu ability for fragments that will be used for cloning. 

I need to amplify inserts of 1kb and 2kb for cloning purposes, either using Gibson, Slice or Aqua method. But our lab do not have pfu polymerase but we have long range taq polymerase which contain a mixture of normal taq and also pfu. I used it to amplify my fragments but unfortunately, the pcr products obtained are low in concentration no matter how i optimize it. Is the long range taq polymerase not suitable to amplify small fragments? 

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