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作 者:季朝能[1] 杜汉森[1] 郑佐华[1] 黄啸宇 毛裕民[1]
出 处:《中国生物化学与分子生物学报》1999年第3期432-435,共4页Chinese Journal of Biochemistry and Molecular Biology
基 金:国家自然科学基金
摘 要:通过参U法定点突变产生了TaqDNA聚合酶N端分别缺失3个,235个,287个和443个氨基酸的4个缺失体,利用Bal-31连续缺失法产生了TaqDNA聚合酶的C端分别缺失了2个、16个、29个、32个、34个氨基酸的5个缺失体.经DNA聚合酶活性测定表明N端缺失3个,235个,287个氨基酸后活力和完整的Taq相近,而缺失443个氨基酸后则失去了DNA聚合酶活力;C端的5个缺失体都失去了DNA聚合酶活性.据此TaqDNA聚合酶的功能区域被定位在287~832氨基酸之间.Four truncators with deletion of 3,235,287 and 443 amino acids at N terminus of Taq DNA polymerase were obtained through ural mediated site direct mutagenesis.Five truncators with deletion of 2,16,29,32 and 34 amino acids at C terminus were obtained through continuous deletion with Bal 31 nuclease.Their DNA polymerase activity was measured.It was found that truncators with deletion of 3,235 and 287 amino acids at N terminus maintained the DNA polymerase activity and their specific activity was identical to that of native Taq DNA polymerase while other truncators with deletion at N terminus or C terminus lost their DNA polymerase activity.Based on these,the domain responsible for the DNA polymerase activity of Taq DNA polymerase was located between 287 amino acid and 832 amino acid.
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