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首页> 外文期刊>Chemical research in toxicology >Synthesis and characterization of DNA fluorescent probes containing a single site-specific stereoisomer of anti-benzo(a)pyrene diol epoxide-N2-dG.
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Synthesis and characterization of DNA fluorescent probes containing a single site-specific stereoisomer of anti-benzo(a)pyrene diol epoxide-N2-dG.

机译:含有抗苯并(a)py二醇环氧-N2-dG的单一位点特异性立体异构体的DNA荧光探针的合成与表征。

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We present a comprehensive study of synthesis and characterization of DNA probes containing covalently bound benzo[a]pyrene diol epoxide (BPDE) isomers at a defined site. Short oligonucleotides of 16mers containing a single trans-(+)- or trans-(-)-anti-BPDE-N(2)-guanine adducts (BPDE-16mer) were first synthesized and then ligated with a fluorescently labeled single-stranded oligonucleotide. The ligation products (double-stranded or single-stranded 90mers) contained a single BPDE adduct of defined stereochemistry and a fluorescent label. The BPDE adduct could be recognized by a specific antibody, and the fluorescent label was useful for highly sensitive laser-induced fluorescence detection. The incorporation of single BPDE in the 16mers was validated by liquid chromatography, UV spectroscopy, and tandem mass spectrometry analysis. The stereochemistry of the single BPDE adducts in the 16mers was further identified by enzyme digestion-coupled stereoselective chromatography analysis. The ligation of BPDE-16mer with normal oligonucleotides for the synthesis of tetramethylrhodamine (TMR)-BPDE-90mers was evaluated. It was found that the modification of the 16mer by anti-BPDE could significantly reduce the ligation yield of ds90mer and lead to the formation of gapped DNA. The incorporation of a single anti-BPDE adduct in ligated ds90mers was confirmed using an antibody specific to the anti-BPDE-dG and affinity capillary electrophoresis. The detection limits of the TMR-BPDE-90mers by capillary electrophoresis coupled with laser-induced fluorescence are below 4 x 10(-19) mol.
机译:我们提出了对DNA探针的合成和表征的全面研究,该DNA探针在定义的位点包含共价结合的苯并[a] py二醇环氧化合物(BPDE)异构体。首先合成包含单个反式(+)-或反式(-)-反BPDE-N(2)-鸟嘌呤加合物(BPDE-16mer)的16mer的短寡核苷酸,然后将其与荧光标记的单链寡核苷酸连接。连接产物(双链或单链90mers)包含定义的立体化学的单个BPDE加合物和荧光标记。 BPDE加合物可以被特异性抗体识别,并且荧光标记可用于高度敏感的激光诱导的荧光检测。通过液相色谱,紫外光谱和串联质谱分析验证了单一BPDE在16mers中的掺入。通过酶消化偶联的立体选择性色谱分析进一步鉴定了16聚体中单个BPDE加合物的立体化学。评估了BPDE-16mer与正常寡核苷酸的连接,以合成四甲基罗丹明(TMR)-BPDE-90mers。发现抗BPDE对16mer的修饰可显着降低ds90mer的连接产量并导致空缺DNA的形成。使用对抗BPDE-dG和亲和毛细管电泳具有特异性的抗体,证实了单个抗BPDE加合物在连接的ds90mers中的掺入。通过毛细管电泳结合激光诱导的荧光,TMR-BPDE-90mers的检测限低于4 x 10(-19)mol。

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