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在 DNA 支架上同时且无痕地连接肽片段。

Simultaneous and Traceless Ligation of Peptide Fragments on DNA Scaffold.

机构信息

Department of Chemistry and Biotechnology , The University of Tokyo , 7-3-1 Hongo, Bunkyo-ku , Tokyo 113-8656 , Japan.

Research Center for Advanced Science and Technology , The University of Tokyo , 4-6-1 Komaba, Meguro-ku , Tokyo 153-8904 , Japan.

出版信息

Biomacromolecules. 2019 Mar 11;20(3):1246-1253. doi: 10.1021/acs.biomac.8b01655. Epub 2019 Feb 7.

DOI:10.1021/acs.biomac.8b01655
PMID:30677290
Abstract

Peptide ligation is an indispensable step in the chemical synthesis of target peptides and proteins that are difficult to synthesize at once by a solid-phase synthesis. The ligation reaction is generally conducted with two peptide fragments at a high aqueous concentration to increase the reaction rate; however, this often causes unpredictable aggregation and precipitation of starting or resulting peptides due to their hydrophobicities. Here, we have developed a novel peptide ligation strategy harnessing the two intrinsic characteristics of oligodeoxynucleotides (ODNs), i.e., their hydrophilicity and hybridization ability, which allowed increases in the water solubility of peptides and the reaction kinetics due to the proximity effect, respectively. Peptide-ODN conjugates that can be cleaved to regenerate native peptide sequences were synthesized using novel lysine derivatives containing conjugation handles and photolabile linkers, via solid-phase peptide synthesis and subsequent conjugation to 15-mer ODNs. Two complementary conjugates were applied to carbodiimide-mediated peptide ligation on a DNA scaffold, and the subsequent DNA removal was conducted by photoirradiation in a traceless fashion. This DNA scaffold-assisted ligation resulted in a significant acceleration of the reaction kinetics and enabled ligation of a hydrophobic peptide at a micromolar concentration. On the basis of this chemistry, a simultaneous ligation of three different peptide fragments on two different DNA scaffolds has been conducted for the first time.

摘要

肽键连接是化学合成目标肽和蛋白质的不可或缺的步骤,这些肽和蛋白质难以通过固相合成一次合成。通常,为了提高反应速率,将两个肽片段在高水浓度下进行连接反应; 然而,由于其疏水性,这常常导致起始或生成的肽不可预测地聚集和沉淀。在这里,我们利用寡脱氧核苷酸 (ODN) 的两个固有特性,即其亲水性和杂交能力,开发了一种新型肽键连接策略,分别由于接近效应而增加了肽的水溶性和反应动力学。通过固相肽合成和随后与 15 聚体 ODN 的偶联,使用含有偶联基团和光不稳定连接体的新型赖氨酸衍生物合成了可以通过切割来再生天然肽序列的肽-ODN 缀合物。两个互补的缀合物被应用于在 DNA 支架上进行碳二亚胺介导的肽键连接,随后通过无痕迹光照射进行 DNA 的去除。这种 DNA 支架辅助的连接显著加速了反应动力学,并能够在微摩尔浓度下连接疏水性肽。在此基础上,首次在两个不同的 DNA 支架上同时连接三个不同的肽片段。

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