Department of Chemistry, Wayne State University, Detroit, MI 48202, United States.
DNA Repair (Amst). 2010 Feb 4;9(2):153-60. doi: 10.1016/j.dnarep.2009.11.006. Epub 2009 Dec 11.
Most bacteria, including Escherichia coli, lack an enzyme that can phosphorylate deoxycytidine and its analogs. Consequently, most studies of toxicity and mutagenicity of cytosine analogs use ribonucleosides such as 5-azacytidine (AzaC) and zebularine (Zeb) instead of their deoxynucleoside forms, 5-aza-2'-deoxycytidine (AzadC) and 2'-deoxy-zebularine (dZeb). The former analogs are incorporated into both RNA and DNA creating complex physiological responses in cells. To circumvent this problem, we introduced into E. coli the Drosophila deoxynucleoside kinase (Dm-dNK), which has a relaxed substrate specificity, and tested these cells for sensitivity to AzadC and dZeb. We find that Dm-dNK expression increases substantially sensitivity of cells to these analogs and dZeb is very mutagenic in cells expressing the kinase. Furthermore, toxicity of dZeb in these cells requires DNA mismatch correction system suggesting a mechanism for its toxicity and mutagenicity. The fluorescence properties of dZeb were used to quantify the amount of this analog incorporated into cellular DNA of mismatch repair-deficient cells expressing Dm-dNK and the results showed that in a mismatch correction-defective strain a high percentage of DNA bases may be replaced with the analog without long term toxic effects. This study demonstrates that the mechanism by which Zeb and dZeb cause cell death is fundamentally different than the mechanism of toxicity of AzaC and AzadC. It also opens up a new way to study the mechanism of action of deoxycytidine analogs that are used in anticancer chemotherapy.
大多数细菌,包括大肠杆菌,缺乏能够磷酸化脱氧胞苷及其类似物的酶。因此,大多数关于胞嘧啶类似物的毒性和致突变性的研究使用核糖核苷,如 5-氮杂胞苷(AzaC)和 zebularine(Zeb),而不是它们的脱氧核苷形式,5-氮杂-2'-脱氧胞苷(AzadC)和 2'-脱氧 zebularine(dZeb)。前体类似物被掺入 RNA 和 DNA 中,在细胞中产生复杂的生理反应。为了避免这个问题,我们将果蝇脱氧核苷激酶(Dm-dNK)引入大肠杆菌,该激酶具有较宽松的底物特异性,并测试这些细胞对 AzadC 和 dZeb 的敏感性。我们发现,Dm-dNK 的表达大大增加了细胞对这些类似物的敏感性,并且激酶表达的细胞中 dZeb 非常具有致突变性。此外,这些细胞中 dZeb 的毒性需要 DNA 错配修复系统,这表明了其毒性和致突变性的一种机制。dZeb 的荧光特性用于定量表达 Dm-dNK 的 mismatch repair-deficient 细胞中这种类似物掺入细胞 DNA 的量,结果表明在 mismatch correction-defective 菌株中,可能有很高比例的 DNA 碱基被类似物取代,而没有长期的毒性影响。这项研究表明,Zeb 和 dZeb 导致细胞死亡的机制与 AzaC 和 AzadC 的毒性机制从根本上不同。它还为研究用于癌症化疗的脱氧胞苷类似物的作用机制开辟了新的途径。