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1. Cytochrome c Facilitates Binding between Lipid Bilayers and Citrate-Coated Gold Nanoparticles in Coarse-Grained Simulations

   https://doi.org/10.1021/acs.jctc.5c00454  

   Wang, Yinhan; Hernandez, Rigoberto (July 2025, Journal of Chemical Theory and Computation)

   Characterization and prediction of the interactions between engineered nanoparticles (ENPs), proteins, and biological membranes is critical for advancing applications to nanomedicine and nanomanufacturing while mitigating nanotoxicological risks. In this work, we employ a coarse-grained dissipative particle dynamics (DPD) simulation to investigate the interactions among cytochrome c (CytC), lipid bilayers, and citrate-coated gold nanoparticles (AuNPs). We updated the DPD potential to accurately represent binding potentials between molecules, and validated the model relative to an all-atom representation. The DPD simulations successfully replicate experimental observations: CytC facilitates the binding of citrate-coated AuNPs to lipid bilayers composed of 90% dioleoylphosphatidylcholine (DOPC) mixed with 10% stearoylphosphatidylinositol (SAPI) or 10% tetraoleoyl cardiolipin (TOCL) but not to pure 100% DOPC bilayers. In addition, the simulations reveal nuanced differences in binding preferences between CytC, the lipid bilayers, and the ENP, at a scale that is not presently directly observable in experiments. Specifically, we found that the surface coating of the nanoparticles─viz variations in the CytC surface density─affects the protein-mediated binding with the bilayers. Such a molecular-sensitive result underscores the utility of DPD simulations in simulating complex biological systems. 

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2. Surface Coating Structure and its Interaction with Cytochrome c in EG6 Coated Nanoparticles Varies with Surface Curvature

   https://doi.org/10.1021/acs.langmuir.0c00681  

   Daly, Clyde A.; Allen, Caley R; Rozanov, Nikita D.; Chong, Gene; Melby, Eric S; Kuech, Thomas R.; Lohse, Samuel E.; Murphy, Catherine J.; Pedersen, Joel A.; Hernandez, Rigoberto (January 2020, Langmuir)

   The composition, orientation, and conformation of proteins in biomolecular coronas acquired by nanoparticles in biological media contribute to how they are identified by a cell. While numerous studies have investigated protein composition in biomolecular coronas, relatively little detail is known about how the nanoparticle surface influences the orientation and conformation of the proteins associated with them. We previously showed that the peripheral membrane protein cytochrome c adopts preferred poses relative to negatively charged MPA-AuNPs. Here, we employ molecular dynamics simulations and complementary experiments to establish that cytochrome c also assumes preferred poses upon association with nanoparticles functionalized with an uncharged ligand, and specifically ω-(1-mercaptounde-11-cyl)hexa(ethylene glycol) (EG6). We find that the display of the EG6 ligands is sensitive to the curvature of the surface—and consequently, the effective diameter of the nearly spherical nanoparticle core—which in turn affects the preferred poses of cytochrome c. 

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3. Melanin Zinc Complex as a Biocompatible Agent for Clearing Bacteremia

   https://doi.org/10.1002/admi.202300369  

   Eliato, Tahmineh Rahmani; Edwards, Seth; Tian, Zhen; Andam, Cheryl P.; Jeong, Kyung Jae; Kim, Young Jo (December 2023, Advanced Materials Interfaces)

   Abstract Sepsis, whole‐body inflammation caused by the contamination of blood by bacteria and endotoxins, affects millions of patients annually with high mortality rates. A recent promising approach to treat sepsis involves the removal of bacteria and endotoxins using extracorporeal blood‐cleansing devices. However, poor specificity, slow recognition of pathogens, and high costs remain the main limitations. Here, the melanin, a biologically derived pigment, is reported for the rapid binding of bacteria and endotoxins from the contaminated blood . This novel approach utilizes the specific binding between Zn²⁺‐loaded melanin and bacteria/endotoxins with minimal nonspecific interactions with human blood components. Melanin contains various chemical functional groups that allow reversible chelation of metallic ions such as Zn²⁺via redox reactions. Zn²⁺enables rapid and specific binding with bacteria/endotoxins due to the strong electrostatic interactions between Zn²⁺and phosphate ions. The presence of various zinc‐binding proteins on the bacterial cell membrane further enhances the binding. The well‐known biocompatibility and low cost make melanin an ideal material to interface with human blood. Zn²⁺‐charged melanin can remove 90% ofE. coliand 100% of endotoxin in PBS and human blood. Zn²⁺‐melanin also demonstrated excellent hemocompatibility shown by protein adsorption, blood coagulation, and hemolysis tests. 

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4. Chapter Six - Heterologous expression, purification, and characterization of proteins in the lanthanome

   https://doi.org/10.1016/bs.mie.2021.02.004  

   Featherston, Emily R; Mattocks, Joseph A; Trisch, Jonathan L; Cotruvo Jr, Joseph A (April 2021, Methods in enzymology)

   Cotruvo Jr, Joseph A (Ed.)

   Recent work has revealed that certain lanthanides—in particular, the more earth-abundant, lighter lanthanides—play essential roles in pyrroloquinoline quinone (PQQ) dependent alcohol dehydrogenases from methylotrophic and non-methylotrophic bacteria. More recently, efforts of several laboratories have begun to identify the molecular players (the lanthanome) involved in selective uptake, recognition, and utilization of lanthanides within the cell. In this chapter, we present protocols for the heterologous expression in Escherichia coli, purification, and characterization of many of the currently known proteins that comprise the lanthanome of the model facultative methylotroph, Methylorubrum extorquens AM1. In addition to the methanol dehydrogenase XoxF, these proteins include the associated c-type cytochrome, XoxG, and solute binding protein, XoxJ. We also present new, streamlined protocols for purification of the highly selective lanthanide-binding protein, lanmodulin, and a solute binding protein for PQQ, PqqT. Finally, we discuss simple, spectroscopic methods for determining lanthanide- and PQQ-binding stoichiometry of proteins. We envision that these protocols will be useful to investigators identifying and characterizing novel members of the lanthanome in many organisms. 

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5. Quantitative comparison of protein-protein interaction interface using physicochemical feature-based descriptors of surface patches

   https://doi.org/10.3389/fmolb.2023.1110567  

   Shin, Woong-Hee; Kumazawa, Keiko; Imai, Kenichiro; Hirokawa, Takatsugu; Kihara, Daisuke (February 2023, Frontiers in Molecular Biosciences)

   Driving mechanisms of many biological functions in a cell include physical interactions of proteins. As protein-protein interactions (PPIs) are also important in disease development, protein-protein interactions are highlighted in the pharmaceutical industry as possible therapeutic targets in recent years. To understand the variety of protein-protein interactions in a proteome, it is essential to establish a method that can identify similarity and dissimilarity between protein-protein interactions for inferring the binding of similar molecules, including drugs and other proteins. In this study, we developed a novel method, protein-protein interaction-Surfer, which compares and quantifies similarity of local surface regions of protein-protein interactions. protein-protein interaction-Surfer represents a protein-protein interaction surface with overlapping surface patches, each of which is described with a three-dimensional Zernike descriptor (3DZD), a compact mathematical representation of 3D function. 3DZD captures both the 3D shape and physicochemical properties of the protein surface. The performance of protein-protein interaction-Surfer was benchmarked on datasets of protein-protein interactions, where we were able to show that protein-protein interaction-Surfer finds similar potential drug binding regions that do not share sequence and structure similarity. protein-protein interaction-Surfer is available at https://kiharalab.org/ppi-surfer . 

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