Yeast Apn2 is an AP endonuclease and DNA 3'-diesterase that belongs to the Exo III family with homology to the E. coli exonuclease III, Schizosaccharomyces pombe eth1, and human AP endonucleases APEX1 and APEX2. In the absence of Apn1, the major AP endonuclease in yeast, Apn2 can cleave the DNA backbone at an AP lesion initiating the base excision repair pathway. To study the role and relative contribution of Apn2, we took advantage of a reporter system that was previously used to delineate how uracil-derived AP sites are repaired. At this reporter, disruption of the Apn1-initiated base excision repair pathway led to a significant elevation of A:T to C:G transversions. Here we show that such highly elevated A:T to C:G transversion mutations associated with uracil residues in DNA are abolished when apn1â yeast cells are grown in glucose as the primary carbon source. We also show that the disruption of Apn2, either by the complete gene deletion or by the mutation of a catalytic residue, results in a similarly reduced rate of the uracil-associated mutations. Overall, our results indicate that Apn2 activity is regulated by the glucose repression pathway in yeast.
The activity of yeast Apn2 AP endonuclease at uracil-derived AP sites is dependent on the major carbon source.
酵母 Apn2 AP 核酸内切酶在尿嘧啶衍生的 AP 位点的活性取决于主要碳源
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作者:Stokdyk Kasey, Berroyer Alexandra, Grami Zacharia A, Kim Nayun
| 期刊: | Current Genetics | 影响因子: | 1.600 |
| 时间: | 2021 | 起止号: | 2021 Apr;67(2):283-294 |
| doi: | 10.1007/s00294-020-01141-4 | 种属: | Yeast |
| 研究方向: | 其它 | ||
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