01 January 1970 5 8K Report

This is my methods: Firstly, I amplify two fragment respectively, after gel purification of two fragments, a fusion step is carried out which only add two fragments, pfu polymerase, buffer and dNTP for about 5 cycles.

95℃  20s

55℃  20s

72℃  3min

then 3 micro liter fusion product will be taken as template for whole PCR amplification.

However, the final gel result is terrible, the gel is almost completely white. I have tried several times, I am sure the quality and quantity of two fragments are fine and overlap has 40bp more or less. The length of two fragments are 1480 and 4000bp.

Anyone can help me about this problem?

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