Cancer Sciences, Faculty of Medicine, University of Southampton, Southampton, SO16 6YD (UK).
Angew Chem Int Ed Engl. 2014 Feb 24;53(9):2362-5. doi: 10.1002/anie.201308691. Epub 2014 Jan 22.
Click DNA ligation promises an alternative to the current enzymatic approaches for DNA assembly, with the ultimate goal of using efficient chemical reactions for the total chemical synthesis and assembly of genes and genomes. Such an approach would enable the incorporation of various chemically modified bases throughout long stretches of DNA, a feat not possible with current polymerase-based methods. An unequivocal requirement for this approach is the biocompatibility of the resulting triazole-linked DNA. The correct function of this unnatural DNA linker in human cells is demonstrated here by using a click-linked gene encoding the fluorescent protein mCherry. Reverse transcription of mRNA isolated from these cells and subsequent sequencing of the mCherry cDNA shows error-free transcription. Nucleotide excision repair (NER) is shown to not play a role in the observed biocompatibility by using a NER-deficient human cell line. This is the first example of a non-natural DNA linker being functional in a eukaryotic cell.
点击 DNA 连接有望成为当前 DNA 组装酶法的替代方法,其最终目标是使用高效的化学反应来进行基因和基因组的全化学合成和组装。这种方法将能够在长片段的 DNA 中掺入各种化学修饰的碱基,这是当前基于聚合酶的方法所不可能实现的。这种方法的一个明确要求是得到的三唑键合 DNA 的生物相容性。通过使用点击连接的基因来编码荧光蛋白 mCherry,本文证明了这种非天然 DNA 接头在人类细胞中的正确功能。从这些细胞中分离出的 mRNA 的逆转录,以及随后对 mCherry cDNA 的测序表明,转录是无错误的。通过使用缺乏核苷酸切除修复 (NER) 的人类细胞系,证明 NER 并不在观察到的生物相容性中发挥作用。这是第一个非天然 DNA 接头在真核细胞中具有功能的例子。
