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Large-peptide permeation through a membrane channel: understanding protamine translocation through cyma from klebsiella oxytoca

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dc.contributor.author Prajapati, Jigneshkumar Dahyabhai
dc.date.accessioned 2025-12-16T09:17:54Z
dc.date.available 2025-12-16T09:17:54Z
dc.date.issued 2021-02
dc.identifier.uri https://onlinelibrary.wiley.com/doi/full/10.1002/anie.202016943
dc.identifier.uri http://dspace.bits-pilani.ac.in:8080/jspui/handle/123456789/20412
dc.description.abstract Quantifying the passage of the large peptide protamine (Ptm) across CymA, a passive channel for cyclodextrin uptake, is in the focus of this study. Using a reporter-pair-based fluorescence membrane assay we detected the entry of Ptm into liposomes containing CymA. The kinetics of the Ptm entry was independent of its concentration suggesting that the permeation through CymA is the rate-limiting factor. Furthermore, we reconstituted single CymA channels into planar lipid bilayers and recorded the ion current fluctuations in the presence of Ptm. To this end, we were able to resolve the voltage-dependent entry of single Ptm peptide molecules into the channel. Extrapolation to zero voltage revealed about 1–2 events per second and long dwell times, in agreement with the liposome study. Applied-field and steered molecular dynamics simulations added an atomistic view of the permeation events. It can be concluded that a concentration gradient of 1 μm Ptm leads to a translocation rate of about one molecule per second and per channel. en_US
dc.language.iso en en_US
dc.publisher Wiley en_US
dc.subject Biology en_US
dc.subject Protamine translocation via CymA en_US
dc.subject Passive channel permeation kinetics en_US
dc.subject Single-molecule voltage-dependent entry en_US
dc.subject Atomistic simulation of peptide permeation en_US
dc.title Large-peptide permeation through a membrane channel: understanding protamine translocation through cyma from klebsiella oxytoca en_US
dc.type Article en_US


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