A capillary electrophoresis method to explore the self‐assembly of a novel polypeptide ligand with quantum dots

化学 量子点 配体(生物化学) 毛细管电泳 荧光 费斯特共振能量转移 组氨酸 咪唑 组合化学 纳米技术 立体化学 色谱法 材料科学 生物化学 受体 物理 氨基酸 量子力学
作者
Jianhao Wang,Chencheng Zhang,Li Liu,Karunakaran Kalesh,Lin Qiu,Shumin Ding,Minli Fu,Liqian Gao,Pengju Jiang
出处
期刊:Electrophoresis [Wiley]
卷期号:37 (15-16): 2156-2162 被引量:20
标识
DOI:10.1002/elps.201600164
摘要

Polyhistidine peptides are effective ligands to coat quantum dots (QDs). It is known that both the number of histidine (His) residues repeats and their structural arrangements in a peptide ligand play important roles in the assembly of the peptide onto CdSe/ZnS QDs. However, due to steric hindrance, a peptide sequence with more than six His residue tandem repeats would hardly coordinate well with Zn(2+) in the QD shell to further enhance the binding affinity. To solve this problem, a His-containing peptide ligand, ATTO 590-E2 G (NH)6 (ATTO-NH), was specifically designed and synthesized for assembly with QDs. With sequential injection of QDs and ATTO-NH into the capillary electrophoresis with fluorescence detection, strong Förster resonance energy transfer phenomenon between the QDs and the ATTO 590 dye was observed, indicating efficient self-assembly of the novel peptide onto the QDs to form ATTO-NH capped QDs inside the capillary. The binding stability of the ligand onto the QD was then systematically investigated by titrating with imidazole, His, and a his-tag containing competitive peptide. It is believed that this new in-capillary assay significantly reduced the sample consumption and the analysis time. By functionalizing QDs with certain metal cation-specific group fused peptide ligand, the QD-based probes could be even extended to the online detection of metal cations for monitoring environment in the future.
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