Abstract: Purpose: To construct the expression vector with the mutant apolipoprotein CⅡ(apoCⅡ) promoter for studying the transcript activity of the mutant apoCⅡ promoter on - 190 base pair. Methods: The plasmid pGL 3 with normal apoCⅡ promoter was used as the template, and a pair of completely complementary primers with the desired mutation was designed, which make the plasmid amplified and mutated on - 190 base pair of the apoCⅡ promoter using Stratagene's site- directed mutagenesis kit. After being transformed into XL- Blue supercompetent cells, the nicked mutant plasmid was repaired in these cells. Results: The normal apoCⅡ promoter was successfully changed from T to A on the - 190 base pair, the expression vector with the mutant apoCⅡ promoter was constructed. Conclusion: The whole circled plasmid with the desired mutation was obtained by a rapid and efficient method for site- directed mutagenesis, which has an implication for detecting the activity of the mutant apoCⅡ promoter.

Key words: Apolipoprotein CⅡ, Site- directed mutation, Promoter