Sensing PEGylated Peptide Conformations Using a Protein Nanopore

被引:3
|
作者
Satheesan, Remya [1 ,2 ]
Vikraman, Devika [1 ,2 ]
Jayan, Parvathy [3 ]
Vijayan, Vinesh [3 ]
Chimerel, Catalin [4 ]
Mahendran, Kozhinjampara R. [1 ]
机构
[1] Rajiv Gandhi Ctr Biotechnol, Transdisciplinary Biol Program, Membrane Biol Lab, Thiruvananthapuram 695014, India
[2] Manipal Acad Higher Educ, Manipal 576104, Karnataka, India
[3] Indian Inst Sci Educ & Res Thiruvananthapuram, Sch Chem, Vithura 695551, Kerala, India
[4] Transilvania Univ Brasov, Fac Elect Engn & Comp Sci, Automat Dept, Brasov 500036, Romania
关键词
nanopore; peptides; conformation; single-channel; current blockages; OUTER-MEMBRANE; ALPHA-HEMOLYSIN; DISCRIMINATION; TRANSLOCATION; CYCLODEXTRIN; PORE; MOLECULES; POLYMERS; CYMA;
D O I
10.1021/acs.nanolett.3c03247
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Membrane pores are exploited for the stochastic sensing of various analytes, and here, we use electrical recordings to explore the interaction of PEGylated peptides of different sizes with a protein pore, CymA. This wide-diameter natural pore comprises densely filled charged residues, facilitating electrophoretic binding of polyethylene glycol (PEG) tagged with a nonaarginine peptide. The small PEG 200 peptide conjugates produced monodisperse blockages and exhibited voltage-dependent translocation across the pores. Notably, the larger PEG 1000 and 2000 peptide conjugates yielded heterogeneous blockages, indicating a multitude of PEG conformations hindering their translocation through the pore. Furthermore, a much larger PEG 5000 peptide occludes the pore entrance, resulting in complete closure. The competitive binding of different PEGylated peptides with the same pore produced specific blockage signals reflecting their identity, size, and conformation. Our proposed model of sensing distinct polypeptide conformations corresponds to disordered protein unfolding, suggesting that this pore can find applications in proteomics.
引用
收藏
页码:3566 / 3574
页数:9
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