首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >The thymine-thymine pyrimidine-pyrimidone(6-4) ultraviolet light photoproduct is highly mutagenic and specifically induces 3 thymine-to-cytosine transitions in Escherichia coli.
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The thymine-thymine pyrimidine-pyrimidone(6-4) ultraviolet light photoproduct is highly mutagenic and specifically induces 3 thymine-to-cytosine transitions in Escherichia coli.

机译:胸腺嘧啶-胸腺嘧啶-嘧啶酮(6-4)紫外光照相产品是高度诱变的并且在大肠杆菌中特异性诱导3胸腺嘧啶向胞嘧啶的转变。

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摘要

We have constructed single-stranded, M13-based vectors that contain a specifically located thymine-thymine pyrimidine-pyrimidone(6-4) UV photoproduct and have used these to estimate the frequency and accuracy of DNA replication past this adduct in uvrA6 cells of Escherichia coli. Both the normal and the Dewar valence photoisomer of the (6-4) adduct were studied. In the absence of SOS induction, vectors carrying the photoproducts were rarely replicated; relative to the lesion-free control, 1.9% of vectors carrying the normal (6-4) isomer produced plaques, and with the Dewar valence isomer the proportion was 0.4%. In SOS-induced cells, these frequencies rose to 22.1% and 12.3%, respectively. The error frequency of replication past the normal isomer in SOS-induced cells was high; in a random sample of 185 progeny phage analyzed, 169 (91%) contained mutations, all of which were targeted. Equally striking, a high proportion of the mutations (158/169; 93%) were of only one type, namely 3' T----C transitions. Both the error frequency and the specificity were much reduced with the Dewar valence isomer; overall, 74/140 (53%) of the phage analyzed were mutant, and of these only 34 (46%) entailed the 3' T----C transition. We speculate that the high error frequency and specificity arise from the formation of a stable T-G base pair, involving hydrogen bonds at O-2 and N-3 in the pyrimidone ring. Potential hydrogen bonds at these sites are coplanar in the normal but not in the Dewar isomer, perhaps explaining the reduced specificity of mutagenesis with the latter adduct.
机译:我们构建了基于M13的单链载体,其中包含一个专门定位的胸腺嘧啶-胸腺嘧啶-嘧啶酮(6-4)紫外线光敏产物,并已用于估计通过该加合物在大肠杆菌uvrA6细胞中复制的频率和准确性。大肠杆菌。研究了(6-4)加合物的正态和杜瓦价光异构体。在没有SOS诱导的情况下,携带光产物的载体很少被复制。相对于无损伤的对照,携带正常(6-4)异构体的载体中有1.9%会产生噬菌斑,而使用杜瓦价异构体的比例为0.4%。在SOS诱导的细胞中,这些频率分别上升到22.1%和12.3%。在SOS诱导的细胞中,通过正常异构体复制的错误频率很高。在随机分析的185个子代噬菌体样本中,有169个突变(占91%)包含突变,所有这些突变都是靶向的。同样惊人的是,很大比例的突变(158/169; 93%)只有一种类型,即3'T–C转换。杜瓦价异构体降低了错误频率和特异性。总体而言,分析的噬菌体中有74/140(53%)是突变体,其中只有34(46%)涉及3'T ---- C过渡。我们推测,高错误频率和特异性来自稳定的T-G碱基对的形成,该碱基对涉及嘧啶酮环中O-2和N-3处的氢键。这些位点上的潜在氢键在正常情况下是共面的,但在杜瓦异构体中则不是共面的,这可能解释了后者加合物诱变的特异性降低。

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