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环丙烯作为化学报告基团用于 DNA 的双生物正交和正交代谢标记。

Cyclopropenes as Chemical Reporters for Dual Bioorthogonal and Orthogonal Metabolic Labeling of DNA.

机构信息

Institute of Organic Chemistry, Karlsruhe Institute of Technology (KIT), Fritz-Haber-Weg 6, 76131, Karlsruhe, Germany.

出版信息

Angew Chem Int Ed Engl. 2024 May 27;63(22):e202403044. doi: 10.1002/anie.202403044. Epub 2024 Apr 19.

Abstract

Dual bioorthogonal labeling enables the investigation and understanding of interactions in the biological environment that are not accessible by a single label. However, applying two bioorthogonal reactions in the same environment remains challenging due to cross-reactivity. We developed a pair of differently modified 2'-deoxynucleosides that solved this issue for dual and orthogonal labeling of DNA. Inverse-electron demand Diels-Alder and photoclick reactions were combined to attach two different fluorogenic labels to genomic DNA in cells. Using a small synthetic library of 1- and 3-methylcyclopropenyl-modified 2'-deoxynucleosides, two 2'-deoxyuridines were identified to be the fastest-reacting ones for each of the two bioorthogonal reactions. Their orthogonal reactivity could be evidenced in vitro. Primer extension experiments were performed with both 2'-deoxyuridines investigating their replication properties as substitutes for thymidine and evaluating subsequent labeling reactions on the DNA level. Finally, dual, orthogonal and metabolic fluorescent labeling of genomic DNA was demonstrated in HeLa cells. An experimental procedure was developed combining intracellular transport and metabolic DNA incorporation of the two 2'-deoxyuridines with the subsequent dual bioorthogonal labeling using a fluorogenic cyanine-styryl tetrazine and a fluorogenic pyrene-tetrazole. These results are fundamental for advanced metabolic labeling strategies for nucleic acids in the future, especially for live cell experiments.

摘要

双生物正交标记能够研究和理解在单一标记无法达到的生物环境中的相互作用。然而,由于交叉反应,在同一环境中应用两种生物正交反应仍然具有挑战性。我们开发了一对不同修饰的 2'-脱氧核苷,解决了双正交 DNA 标记的问题。逆电子需求 Diels-Alder 和光点击反应结合起来,将两种不同的荧光标记物附着到细胞中的基因组 DNA 上。使用 1-和 3-甲基环丙烯基修饰的 2'-脱氧核苷的小合成文库,鉴定出两种 2'-脱氧尿嘧啶核苷,它们是两种生物正交反应中反应最快的两种。它们的正交反应性可以在体外得到证明。用两种 2'-脱氧尿嘧啶核苷进行引物延伸实验,研究它们作为胸苷替代品的复制特性,并评估随后在 DNA 水平上的标记反应。最后,在 HeLa 细胞中实现了基因组 DNA 的双正交和代谢荧光标记。开发了一种实验程序,将两种 2'-脱氧尿嘧啶核苷的细胞内转运和代谢 DNA 掺入与随后使用荧光氰基-styryl 四嗪和荧光芘-四唑的双生物正交标记相结合。这些结果对于未来核酸的先进代谢标记策略具有重要意义,特别是对于活细胞实验。

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