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Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation

[Image: see text] Cellular functions of membrane proteins are strongly coupled to their structures and aggregation states in the cellular membrane. Molecular agents that can induce the fragmentation of lipid membranes are highly sought after as they are potentially useful for extracting membrane pro...

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Autores principales: Yu, Tianyi, Omarova, Marzhana, Zhang, Meng, Hossain, Istiak, Chen, Jianqiang, Darvish, Omead, John, Vijay T., Zhang, Donghui
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Chemical Society 2023
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10015453/
https://www.ncbi.nlm.nih.gov/pubmed/36802533
http://dx.doi.org/10.1021/acs.biomac.3c00028
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author Yu, Tianyi
Omarova, Marzhana
Zhang, Meng
Hossain, Istiak
Chen, Jianqiang
Darvish, Omead
John, Vijay T.
Zhang, Donghui
author_facet Yu, Tianyi
Omarova, Marzhana
Zhang, Meng
Hossain, Istiak
Chen, Jianqiang
Darvish, Omead
John, Vijay T.
Zhang, Donghui
author_sort Yu, Tianyi
collection PubMed
description [Image: see text] Cellular functions of membrane proteins are strongly coupled to their structures and aggregation states in the cellular membrane. Molecular agents that can induce the fragmentation of lipid membranes are highly sought after as they are potentially useful for extracting membrane proteins in their native lipid environment. Toward this goal, we investigated the fragmentation of synthetic liposome using hydrophobe-containing polypeptoids (HCPs), a class of facially amphiphilic pseudo-peptidic polymers. A series of HCPs with varying chain lengths and hydrophobicities have been designed and synthesized. The effects of polymer molecular characteristics on liposome fragmentation are systemically investigated by a combination of light scattering (SLS/DLS) and transmission electron microscopy (cryo-TEM and negative stained TEM) methods. We demonstrate that HCPs with a sufficient chain length (DP(n) ≈ 100) and intermediate hydrophobicity (PNDG mol % = 27%) can most effectively induce the fragmentation of liposomes into colloidally stable nanoscale HCP–lipid complexes owing to the high density of local hydrophobic contact between the HCP polymers and lipid membranes. The HCPs can also effectively induce the fragmentation of bacterial lipid-derived liposomes and erythrocyte ghost cells (i.e., empty erythrocytes) to form nanostructures, highlighting the potential of HCPs as novel macromolecular surfactants toward the application of membrane protein extraction.
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spelling pubmed-100154532023-03-16 Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation Yu, Tianyi Omarova, Marzhana Zhang, Meng Hossain, Istiak Chen, Jianqiang Darvish, Omead John, Vijay T. Zhang, Donghui Biomacromolecules [Image: see text] Cellular functions of membrane proteins are strongly coupled to their structures and aggregation states in the cellular membrane. Molecular agents that can induce the fragmentation of lipid membranes are highly sought after as they are potentially useful for extracting membrane proteins in their native lipid environment. Toward this goal, we investigated the fragmentation of synthetic liposome using hydrophobe-containing polypeptoids (HCPs), a class of facially amphiphilic pseudo-peptidic polymers. A series of HCPs with varying chain lengths and hydrophobicities have been designed and synthesized. The effects of polymer molecular characteristics on liposome fragmentation are systemically investigated by a combination of light scattering (SLS/DLS) and transmission electron microscopy (cryo-TEM and negative stained TEM) methods. We demonstrate that HCPs with a sufficient chain length (DP(n) ≈ 100) and intermediate hydrophobicity (PNDG mol % = 27%) can most effectively induce the fragmentation of liposomes into colloidally stable nanoscale HCP–lipid complexes owing to the high density of local hydrophobic contact between the HCP polymers and lipid membranes. The HCPs can also effectively induce the fragmentation of bacterial lipid-derived liposomes and erythrocyte ghost cells (i.e., empty erythrocytes) to form nanostructures, highlighting the potential of HCPs as novel macromolecular surfactants toward the application of membrane protein extraction. American Chemical Society 2023-02-21 /pmc/articles/PMC10015453/ /pubmed/36802533 http://dx.doi.org/10.1021/acs.biomac.3c00028 Text en © 2023 The Authors. Published by American Chemical Society https://creativecommons.org/licenses/by/4.0/Permits the broadest form of re-use including for commercial purposes, provided that author attribution and integrity are maintained (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Yu, Tianyi
Omarova, Marzhana
Zhang, Meng
Hossain, Istiak
Chen, Jianqiang
Darvish, Omead
John, Vijay T.
Zhang, Donghui
Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation
title Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation
title_full Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation
title_fullStr Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation
title_full_unstemmed Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation
title_short Uncovering the Optimal Molecular Characteristics of Hydrophobe-Containing Polypeptoids to Induce Liposome or Cell Membrane Fragmentation
title_sort uncovering the optimal molecular characteristics of hydrophobe-containing polypeptoids to induce liposome or cell membrane fragmentation
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10015453/
https://www.ncbi.nlm.nih.gov/pubmed/36802533
http://dx.doi.org/10.1021/acs.biomac.3c00028
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