Differentiation of selectively labeled peptides using solid-state nanopores

被引:24
作者
Yu, Jae-Seok [1 ]
Hong, Seong Cheol [2 ]
Wu, Sangwook [3 ]
Kim, Hyun-Mi [1 ]
Lee, Cheolju [4 ,5 ,6 ]
Lee, Jun-Seok [2 ]
Lee, Ji Eun [4 ]
Kim, Ki-Bum [1 ,7 ]
机构
[1] Seoul Natl Univ, Dept Mat Sci & Engn, Seoul 08826, South Korea
[2] KIST, Mol Recognit Res Ctr, Seoul 02792, South Korea
[3] Pukyong Natl Univ, Dept Phys, Pusan 48513, South Korea
[4] KIST, Biomed Res Inst, Ctr Theragnosis, Seoul 02792, South Korea
[5] Kyung Hee Univ, KHU KIST Dept Converging Sci & Technol, Seoul 02447, South Korea
[6] Korea Univ Sci & Technol UST, KIST Sch, Div Biomed Sci & Technol, Seoul 02792, South Korea
[7] Seoul Natl Univ, Res Inst Adv Mat, Seoul 08826, South Korea
基金
新加坡国家研究基金会;
关键词
PROTEIN TRANSLOCATION; SINGLE PROTEIN; DNA TRANSPORT; RESOLUTION; DYNAMICS; SIZE;
D O I
10.1039/c8nr09315f
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Determination of the amino acid sequence of a protein is critical for understanding various biological processes. Mass spectrometry has mainly been used for protein identification; however, there are limitations to its sensitivity when detecting low abundance proteins. In this study, we attempted to distinguish between three similar peptide sequences (approximate to 40 amino acids, approximate to 5 kDa) that differed only by the location or number of cysteine residues with solid-state nanopores. The cysteine residues are located at one end, one at the center, and at both ends for each of the three peptides. We found that differentiation of the three types of peptides by nanopore signals was difficult. However, when the cysteine residue was labeled with a negatively charged molecule, Flamma (R) 496, the labeled peptides showed distinct signals for each peptide. Comparing the relative current blockades of labeled peptides with applied voltages, we found that the label was able to change peptide conformations and the resulting ionic current signals from the three labeled peptides were distinguished based on the relative current blockade, full width at half-maximum of the current blockade distribution, and single-molecule level peak shape analysis. Our results suggest that solid-state nanopores combined with a targeted labeling strategy could be used to obtain characteristic peptide signatures that could ultimately be used for protein identification.
引用
收藏
页码:2510 / 2520
页数:11
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