Interfacial constraints on water and proton transport across nafion membranes

Water and proton transport across a Nafion membrane are measured as functions of water activity and applied electric potential with a polymer electrolyte hydrogen pump. Water and proton transport across the membrane must match water and proton transport entering and leaving the electrode/membrane/vapor three phase interfaces at the anode and cathode. At low applied electric potential proton and water fluxes are correlated. At moderate to high applied electric potential the proton current is constant, independent of applied electric potential, while the water transport increases with increasing electric potential. At high applied electric potential water and proton transport become uncoupled at the membrane interfaces; water is transported across the membrane/vapor interface and protons are transported across the membrane/electrode interface. The applied electric potential drives electro‐osmosis to redistribute the water in the membrane. Water redistribution is limited by the interfacial transport of water across the membrane/vapor interface. © 2015 Wiley Periodicals, Inc. J. Polym. Sci. Part B: Polym. Phys. 2015 , 53, 1580–1589     

Molecule‐Membrane Interactions in Biological Cells Studied with Second Harmonic Light Scattering

The nonlinear optical phenomenon second harmonic light scattering (SHS) can be used for detecting molecules at the membrane surfaces of living biological cells. Over the last decade, SHS has been developed for quantitatively monitoring the adsorption and transport of small and medium size molecules (both neutral and ionic) across membranes in living cells. SHS can be operated with both time and spatial resolution and is even capable of isolating molecule‐membrane interactions at specific membrane surfaces in multi‐membrane cells, such as bacteria. In this review, we discuss select examples from our lab employing time‐resolved SHS to study real‐time molecular interactions at the plasma membranes of biological cells. We first demonstrate the utility of this method for determining the transport rates at each membrane/interface in a Gram‐negative bacterial cell. Next, we show how SHS can be used to characterize the molecular mechanism of the century old Gram stain protocol for classifying bacteria. Additionally, we examine how membrane structures and molecular charge and polarity affect adsorption and transport, as well as how antimicrobial compounds alter bacteria membrane permeability. Finally, we discuss adaptation of SHS as an imaging modality to quantify molecular adsorption and transport in sub‐cellular regions of individual living cells.     

The Remarkable Effect of Halogen Substitution on the Membrane Transport of Fluorescent Molecules in Living Cells

Small‐molecule‐based fluorescent probes have become important tools in biology for sensing and imaging applications. However, the biological applications of many of the fluorescent molecules are hampered by low cellular uptake and high toxicity. In this paper, we show for the first time that the introduction of halogen atoms enhances the cellular uptake of fluorescent molecules and the nature of halogen atoms plays a crucial role in the plasma membrane transport in mammalian cells. The remarkably higher uptake of iodinated compounds compared to that of their chloro or bromo analogues suggests that the strong halogen bonding ability of iodine atoms may play an important role in the membrane transport. This study provides a novel strategy for the transport of fluorescent molecules across the plasma membrane in living cells.     

The Effect of Bacterial Signal Indole on the Electrical Properties of Lipid Membranes

Indole is an important biological signalling molecule produced by many Gram positive and Gram negative bacterial species, including Escherichia coli. Here we study the effect of indole on the electrical properties of lipid membranes. Using electrophysiology, we show that two indole molecules act cooperatively to transport charge across the hydrophobic core of the lipid membrane. To enhance charge transport, induced by indole across the lipid membrane, we use an indole derivative, 4 fluoro‐indole. We demonstrate parallels between charge transport through artificial lipid membranes and the function of complex eukaryotic membrane systems by showing that physiological indole concentrations increase the rate of mitochondrial oxygen consumption. Our data provide a biophysical explanation for how indole may link the metabolism of bacterial and eukaryotic cells.     

Driving force for hydraulic and pervaporative transport in homogeneous membranes

Experiments were designed to demonstrate that the chemical potential gradient required for liquid transport through swollen network polymer membranes manifests itself as a concentration gradient and that the rate of transport is independent of how this gradient is established. The fluxes of various liquids through a crosslinked rubber membrane were measured in hydraulic and pervaporation modes of permeation. The pressure applied downstream in the latter act simply to fix the activity of the liquid in the downstream membrane surface. The experiments show the flux is a unique function of this activity, and it does not matter how it is established. Sorption data were used to convert these results into a plot of flux versus concentration differential across the membrane which was analyzed by Fick's law using a model for the concentration dependence of the diffusion coefficient. Measured ceiling fluxes for pervaporation for a number of liquids were found to be the same as those estimated from hydraulic permeation data. A simple mathematical representation for an ideal system is used as a pedagogical device to demonstrate the conclusions.     

Permeability of the Perindopril Arginine under In Vitro Conditions across Caco-2 Monolayer and Biomimetic Phospholipid Membrane

Perindopril arginine (PA) as an angiotensin-converting enzyme (ACE) inhibitor is widely used in cardiovascular diseases, especially in systemic hypertension and heart failure. Although the pharmacokinetics of PA are well documented, there is no available detailed data on its permeation in in vitro conditions. The present study aimed to assess the transport of PA across both biological membranes and artificial biomimetic ones. For the determination of PA transport, the Caco-2 cell line was selected as a reliable in vitro model of gastrointestinal biological barriers. Additionally, a novel 96-well plate with phospholipid membrane PermeaPad was used to evaluate the transport of PA by passive diffusion. We confirmed that PA is relatively poorly permeable across the Caco-2 monolayer. The permeability results obtained from the non-cell-based model demonstrated higher transport of PA as compared to that of Caco-2. Thus, PA transport across the biological membranes might be suggested to be regulated by the membrane transporters.     

Utilization of photoinduced charge-separated state of donor-acceptor-linked molecules for regulation of cell membrane potential and ion transport

The control of ion transport across cell membranes by light is an attractive strategy that allows targeted, fast control of precisely defined events in the biological membrane. Here we report a novel general strategy for the control of membrane potential and ion transport by using charge-separation molecules and light. Delivery of charge-separation molecules to the plasma membrane of PC12 cells by a membranous nanocarrier and subsequent light irradiation led to depolarization of the membrane potential as well as inhibition of the potassium ion flow across the membrane. Photoregulation of the cell membrane potential and ion transport by using charge-separation molecules is highly promising for control of cell functions.     

Dipolar Relaxation Dynamics at the Active Site of an ATPase Regulated by Membrane Lateral Pressure

The active transport of ions across biological membranes requires their hydration shell to interact with the interior of membrane proteins. However, the influence of the external lipid phase on internal dielectric dynamics is hard to access by experiment. Using the octahelical transmembrane architecture of the copper‐transporting P_1B‐type ATPase from Legionella pneumophila as a model structure, we have established the site‐specific labeling of internal cysteines with a polarity‐sensitive fluorophore. This enabled dipolar relaxation studies in a solubilized form of the protein and in its lipid‐embedded state in nanodiscs. Time‐dependent fluorescence shifts revealed the site‐specific hydration and dipole mobility around the conserved ion‐binding motif. The spatial distribution of both features is shaped significantly and independently of each other by membrane lateral pressure.     

Ion transport across biomembranes and model membranes

The milestones formerly achieved in the comprehension of ion transport across biological membranes on the basis of electrochemical concepts and/or instrumentation are briefly summarized. The various types of model membranes presently employed for the investigation of ion transport across biomembranes are reviewed and their requirements for the incorporation and functional investigation of membrane proteins are examined. The potential of model membranes for the elucidation of many problems in molecular membrane biology and for the realization of microarray sensors individually addressable to membrane proteins by electrochemical means is assessed.     

Metal–Organic Framework Membrane Nanopores as Biomimetic Photoresponsive Ion Channels and Photodriven Ion Pumps

Biological ion channels and ion pumps with sub‐nanometer sizes modulate ion transport in response to external stimuli. Realizing such functions with sub‐nanometer solid‐state nanopores has been an important topic with wide practical applications. Herein, we demonstrate a biomimetic photoresponsive ion channel and photodriven ion pump using a porphyrin‐based metal–organic framework membrane with pore sizes comparable to hydrated ions. We show that the molecular‐size pores enable precise and robust optoelectronic ion transport modulation in a broad range of concentrations, unparalleled with conventional solid‐state nanopores. Upon decoration with platinum nanoparticles to form a Schottky barrier photodiode, photovoltage across the membrane is generated with “uphill” ion transport from low concentration to high concentration. These results may spark applications in energy conversion, ion sieving, and artificial photosynthesis.     

BROMOC suite: Monte Carlo/Brownian dynamics suite for studies of ion permeation and DNA transport in biological and artificial pores with effective potentials

The transport of ions and solutes by biological pores is central for cellular processes and has a variety of applications in modern biotechnology. The time scale involved in the polymer transport across a nanopore is beyond the accessibility of conventional MD simulations. Moreover, experimental studies lack sufficient resolution to provide details on the molecular underpinning of the transport mechanisms. BROMOC, the code presented herein, performs Brownian dynamics simulations, both serial and parallel, up to several milliseconds long. BROMOC can be used to model large biological systems. IMC‐MACRO software allows for the development of effective potentials for solute–ion interactions based on radial distribution function from all‐atom MD. BROMOC Suite also provides a versatile set of tools to do a wide variety of preprocessing and postsimulation analysis. We illustrate a potential application with ion and ssDNA transport in MspA nanopore. © 2014 Wiley Periodicals, Inc.     

Enzymatically Active Ultrathin Pepsin Membranes

Enzymatically active proteins enable efficient and specific cleavage reactions of peptide bonds. Covalent coupling of the enzymes permits immobilization, which in turn reduces autolysis‐induced deactivation. Ultrathin pepsin membranes were prepared by facile interfacial polycondensation of pepsin and trimesoyl chloride. The pepsin membrane allows for simultaneous enzymatic conversion and selective removal of digestion products. The large water fluxes through the membrane expedite the transport of large molecules through the pepsin layers. The presented method enables the large‐scale production of ultrathin, cross‐linked, enzymatically active membranes.     

Isothermal and non-isothermal water transport in porous membranes. II. The steady state

Thermoosmotic behaviour was studied in simple systems constituted of grossly porous hydrophobic membranes permeated by distilled water. Attention was focused on steady-state conditions, characterized by absence of net transmembrane volume flow, obtained equilibrating thermoosmotic pressure with an external counterpressure. Comparison of hydraulic and thermoosmotic fluxes with steady-state pressure gives insight in the peculiar thermofluidodynamics of volume flow in non-isothermal membrane channels. This investigation was extended to volume transport caused by combination of the two thermodynamic forces constituted of the temperature and pressure gradients, synergic or antagonistic across the membrane. The experimental findings can be fruitfully compared with theoretical predictions of the system's behaviour derived from different approaches. Results obtained with six different membrane types, under a wide range of experimental conditions, lend support to the “thermal radiation pressure theory” which attributes the various effects of matter transport produced by a temperature gradient to the transfer of momentum from drifting thermal excitations to atoms and molecules in the material crossed by heat flow.     

Positively charged liposomes consisting of the KTTKS pentapeptide conjugated with rhodamine increase rhodamine toxicity in E. coli and zebrafish embryo

Liposomes composed of cell‐penetrating peptide derivatives increased transport across the cell membrane. Conjugating rhodamine to a cell‐penetrating peptide increased the toxicity of rhodamine in E. coli and zebrafish embryos. A similar total protein inhibition pattern with different intensities, indicating that the interaction pathways of the rho‐KTTKS‐CONH₂ monomer and liposomes were the same. It suggests that the rho‐KTTKS‐CONH₂ liposomes showed higher toxicity because better transport across the cell membrane increased the effective concentration inside cells. The staining of zebrafish embryos using rho‐KTTKS‐CONH₂ liposomes showed a longer retention time, suggesting that it can penetrate deeper tissues or organs in zebrafish.     

Diffusive flows in ultrafiltration and their effect on membrane retention properties

In modelling the retention of ultrafiltration membranes, diffusive fluxes across the membrane have usually been neglected, mainly due to evidence derived from using symmetric track-etched membranes. The present paper reexamines this matter specifically for the case of “real” asymmetric membranes. A critical literature review on the use of irreversible thermodynamic (IT), hydrodynamic and Stefan-Maxwell (S-M) models is presented. It is shown that all three approaches yield the same basic retention equation for the case of non-negligible diffusive solute-flux. It is also shown that, for membranes with a coefficient close to one, a much simpler equation gives results almost identical to the more rigorous basic equation just mentioned. Furthermore an overview of available literature data indicates that diffusive fluxes do play a non-negligible role in the functioning of asymmetric ultrafiltration membranes. Further work is needed in order to predict solute transport properties in hydrodynamic terms. A simplified Stefan-Maxwell approach seems the appropriate tool for future work in studying multicomponent solutions.     

Inter-Vesicle Signal Transduction Using a Photo-Responsive Zinc Ionophore

Transmission of chemical information between cells and across lipid bilayer membranes is of profound significance in many biological processes. The design of synthetic signalling systems is a critical step towards preparing artificial cells with collective behaviour. Here, we report the first example of a synthetic inter-vesicle signalling system, in which diffusible chemical signals trigger transmembrane ion transport in a manner reminiscent of signalling pathways in biology. The system is derived from novel ortho-nitrobenzyl and BODIPY photo-caged Zn^II transporters, in which cation transport is triggered by photo-decaging with UV or red light, respectively. This decaging reaction can be used to trigger the release of the cationophores from a small population of sender vesicles. This in turn triggers the transport of ions across the membrane of a larger population of receiver vesicles, but not across the sender vesicle membrane, leading to overall inter-vesicle signal transduction and amplification.     

Mass transport of O2 and N2 in nanoporous carbon (C168 schwarzite) using a quantum mechanical force field and molecular dynamics simulations

A hierarchical approach is used to calculate the single-component fluxes of N2 and O2 in nanoporous carbon molecular sieves (represented by C168 schwarzite) over a wide range of pressures and pressure drops. The self- and corrected diffusivities are calculated using equilibrium molecular dynamics simulations with force fields for the gas-carbon interactions obtained from quantum mechanical calculations. These results are combined with previously reported adsorption isotherms of N2 and O2 in C168 to obtain transport diffusivities and, by use of the Fick's equation of mass transport, to obtain single-component fluxes across the membrane. The diffusion coefficients and fluxes are also calculated using an empirical potential, which has been obtained by fitting low coverage adsorption data of N2 and O2 on a planar graphite sheet. By analyzing the diffusivities calculated with the ab initio potential in the limit of infinite dilution over the temperature range from 80 to 450 K, it is observed that the N2/O2 separation is energetically driven and a high selectivity of O2 over N2 can be obtained at low temperatures. However, with the empirical potential both the energetic and entropic contributions to selectivity were found to be close to unity. Similarly, by calculating single-component fluxes and ideal selectivities at 300 K and finite pressures it is found that the ab initio potential better explains the large O2/N2 selectivities of similarly sized molecules that have been observed experimentally. An interesting reversal in ideal selectivity is observed by adjusting the pressure at the two ends of the membrane. As a consequence, we predict that a highly selective kinetic separation in favor of either nitrogen or oxygen could be obtained with the same membrane depending on the operating conditions.     

Phosphorylation‐Responsive Membrane Transport of Peptides

Phosphorylation and dephosphorylation of peptides by kinases and phosphatases is essential for signal transduction in biological systems, and many diseases involve abnormal activities of these enzymes. Herein, we introduce amphiphilic calixarenes as key components for supramolecular, phosphorylation‐responsive membrane transport systems. Dye‐efflux experiments with liposomes demonstrated that calixarenes are highly active counterion activators for established cell‐penetrating peptides, with EC₅₀ values in the low nanomolar range. We have now found that they can even activate membrane transport of short peptide substrates for kinases involved in signal transduction, whereas the respective phosphorylated products are much less efficiently transported. This allows regulation of membrane transport activity by protein kinase A (PKA) and protein kinase C (PKC), as well as monitoring of their activity in a label‐free kinase assay.     

How do P-type ATPases transport ions?

P-type ATPases are a large family of membrane proteins that perform active ion transport across biological membranes. In these proteins, the energy-providing ATP hydrolysis is coupled to ion transport of one or two ion species across the respective membrane. The pump function of the investigated pumps is described by a so-called Post-Albers cycle. Main features of the pumping process are (1) a Ping-Pong mechanism, i.e. both transported ion species are transferred successively and in opposite direction across the membrane, (2) the transport process for each ion species consists of a sequence of reaction steps, which are ion binding, ion occlusion, conformational transition of the protein, successive deocclusion of the ions and release to the other side of the membrane. (3) Recent experimental evidence shows that the ion-binding sites are placed in the transmembrane section of the proteins and that ion movements occur preferentially during the ion binding and release processes. The main features of the mechanism include narrow access channels from both sides, one gate per access channel, and an ion-binding moiety that is adapted specifically to the ions that are transported, and differently in both principal conformations.