4.5 Article

Partitioning of individual flexible polymers into a nanoscopic protein pore

Journal

BIOPHYSICAL JOURNAL
Volume 85, Issue 2, Pages 897-910

Publisher

BIOPHYSICAL SOCIETY
DOI: 10.1016/S0006-3495(03)74529-9

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Polymer dynamics are of fundamental importance in materials science, biotechnology, and medicine. However, very little is known about the kinetics of partitioning of flexible polymer molecules into pores of nanometer dimensions. We employed electrical recording to probe the partitioning of single poly(ethylene glycol) (PEG) molecules, at concentrations near the dilute regime, into the transmembrane beta-barrel of individual protein pores formed from staphylococcal alpha-hemolysin (alphaHL). The interactions of the alpha-hemolysin pore with the PEGs (M-w 940-6000 Da) fell into two classes: short-duration events (tausimilar to20 mus), similar to85% of the total, and long-duration events (tausimilar to100 ms),; 15% of the total. The association rate constants (k(on)) for both classes of events were strongly dependent on polymer mass, and values of k(on) ranged over two orders of magnitude. By contrast, the dissociation rate constants (k(off)) exhibited a weak dependence on mass, suggesting that the polymer chains are largely compacted before they enter the pore, and do not decompact to a significant extent before they exit. The values of k(on) and k(off) were used to determine partition coeffients (Pi) for the PEGs between the bulk aqueous phase and the pore lumen. The low values of Pi are in keeping with a negligible interaction between the PEG chains and the interior surface of the pore, which is independent of ionic strength. For the long events, values of Pi decrease exponentially with polymer mass, according to the scaling law of Daoud and de Gennes. For PEG molecules larger than similar tokDa, Pi reached a limiting value suggesting that these PEG chains cannot fit entirely into the beta-barrel.

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