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Strand specificity of mutagenic bypass replication of DNA containing psoralen monoadducts in a human cell extract.

机译:人细胞提取物中含有补骨脂素单加合物的DNA的诱变旁路复制的链特异性。

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摘要

Psoralens are mutagenic compounds of vegetable origin that are used as photosensitizing agents in the treatment of various skin diseases, blood cell cancer, and autoimmune disorders. To study the mechanism of mutagenicity of psoralens in humans, we examined the efficiency and fidelity of simian virus 40 origin-dependent replication in a human cell extract of M13mp2 DNA randomly treated with the psoralen derivative 4'-hydroxymethyl-4,5',8-trimethyl psoralen plus UVA irradiation. Replication of DNA treated with variable amounts of 4'-hydroxymethyl-4,5',8-trimethyl psoralen and a fixed UVA fluence was inhibited in a concentration-dependent manner. However, covalently closed monomer-length circular replication products were observed. Product analysis by renaturing agarose gel electrophoresis after cross-linking with 250- to 280-nm UV light indicated that approximately 1 of 9 psoralen monoadducts was bypassed during in vitro replication. Introduction of product DNA into Escherichia coli to score replication errors in the lacZalpha reporter gene demonstrated that replication of the damaged DNA was more mutagenic than was replication of undamaged DNA. Sequence analysis of lacZ mutants revealed that damage-dependent replication errors were predominantly T.A-->C.G transitions, transversions at C.G base pairs, and deletions of single A.T base pairs, the last occurring most frequently in homopolymeric runs. A comparison of error specificities with two substrates having the replication origin asymmetrically placed on opposite sides of the mutational target suggests that the lagging-strand replication apparatus is less accurate than the leading-strand replication apparatus for psoralen monoadduct-dependent deletion errors. A model is proposed based on the preferential loopout of the monoadducted base from the strand that templates retrograde discontinuous synthesis.
机译:补骨脂素是植物来源的诱变化合物,在各种皮肤疾病,血细胞癌和自身免疫性疾病的治疗中用作光敏剂。为了研究补骨脂素在人类中的致突变性机制,我们研究了用补骨脂素衍生物4'-羟甲基-4,5',8随机处理的M13mp2 DNA人类细胞提取物中猿猴病毒40起源依赖性复制的效率和保真度。 -三甲基补骨脂素加UVA照射。用浓度依赖的方式抑制了用可变量的4'-羟甲基-4,5',8-三甲基补骨脂素和固定的UVA通量处理的DNA的复制。但是,观察到共价封闭的单体长度的环状复制产物。在250-280 nm紫外光交联后,通过重振琼脂糖凝胶电泳进行的产品分析表明,在体外复制过程中绕过了9个补骨脂素单加合物中的大约1个。将产物DNA引入大肠杆菌以评估lacZalpha报告基因中的复制错误,这表明受损DNA的复制比未受损DNA的复制更具致突变性。 lacZ突变体的序列分析表明,损伤相关的复制错误主要是T.A-> C.G过渡,C.G碱基对的颠换以及单个A.T碱基对的缺失,最后一次发生在均聚物运行中。将错误特异性与复制起点不对称地置于突变靶标的相对侧的两个底物进行比较,结果表明,对于补骨脂素单加合物依赖性缺失错误,滞后链复制设备的准确性不如前导链复制设备。基于模板逆行不连续合成的链中单加成碱基的优先环出,提出了一个模型。

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