Joanna Zemła

Selective protein adsorption on polymer patterns formed by self-organization and soft lithography.

Thin films, with both isotropic and ordered patterns of polymer domains, are used as substrates to study selective adsorption of two proteins (concanavalin A and lentil lectin) and to test reconstruction of polymer patterns by these proteins. Integral geometry approach is used to compare quantitatively fluorescence micrographs of protein patches with AFM images of original isotropic patterns, formed during blend casting of polystyrene/poly(methyl methacrylate) and PS/poly(ethylene oxide). Preferential adsorption of both lectins to PMMA phase domains, enhanced for PS/PMMA interfaces is concluded. In turn, protein binding to PS phase regions of PS/PEO blends is highly selective. Ordered protein grouping is obtained as a result of selective adsorption to alternating stripes of polystyrene (partly brominated to enable identification) and cross-linked PEO, prepared with solvent-assisted micromolding applied to PBrS/PEO bilayers. Biological activity test, performed with concanavalin A, confirms preserved functionality of a complementary protein, carboxypeptidase Y, adsorbed to polymer patterns.

Temperature and pH dual-responsive coatings of oligoperoxide-graft-poly(N-isopropylacrylamide): wettability, morphology, and protein adsorption.

Poly(N-isopropylacrylamide) (PNIPAM) coatings attached to glass with novel approach involving polymerization from oligoperoxide grafted to surface with (3-aminopropyl)triethoxysilane exhibit not only temperature- but also pH-dependence of wettability and protein adsorption. Wettability and composition of coatings, fabricated with different polymerization times, were determined using contact angle measurements and Time Of Flight-Secondary Ion Mass Spectrometry (TOF-SIMS), respectively. Thermal response of wettability, measured between 20 and 40°C, was prominent at pH 9 and 7 and diminished or absent at pH 5 and 3. This indicates a transition between hydrated loose coils and hydrophobic collapsed chains that is blocked at low pH. Higher surface roughness and dramatically increased adsorption of model protein (lentil lectin labeled with fluorescein isothiocyanate) were observed with AFM and fluorescence microscopy to occur in hydrophobic phases (at pH 3, for pH varied at constant temperature of 22°C and at ∼33°C, for temperature varied at constant pH 9). Protein adsorption response to pH was confirmed by TOF-SIMS and Principal Component Analysis.

Temperature and pH dual-responsive POEGMA-based coatings for protein adsorption

Poly(oligo(ethylene glycol)ethyl ether methacrylate (POEGMA246) coatings were successfully fabricated using novel approach via polymerization from oligoperoxide grafted to premodified glass substrate. Wettability, content and composition of coatings fabricated with different polymerization times were determined using contact angle measurements, ellipsometry and Time of Flight-Secondary Ion Mass Spectrometry (TOF-SIMS). Thermo- and pH-responsive properties of POEGMA246 coatings were found to depend significantly on concentration of the grafted POEGMA246. Coatings fabricated with polymerization time 30 h exhibit not only temperature- but also pH-dependence of wettability. Thermal response of wettability, measured between 20 and 32°C, was prominent at pH 9 and 7 and diminished or was absent at pH 5 and 3, indicating a transition between hydrated loose coils and hydrophobic collapsed chains, blocked at low pH. Protein adsorption, observed by fluorescence microscopy and analyzed semi-quantitatively using integral geometry approach, decreased dramatically for model protein (lentil lectin labeled with fluorescein isothiocyanate) at transition from pH 5 to pH 9, showing only very weak thermal-dependence. Strong protein adsorption response to pH and very weak one to temperature was confirmed by TOF-SIMS and Principal Component Analysis.

Integral Geometry Analysis of Fluorescence Micrographs for Quantitative Relative Comparison of Protein Adsorption onto Polymer Surfaces

Most methods developed to study protein binding to distinct surfaces can only determine the average amount of adsorbed protein or merely provide (qualitative) information on its spatial distribution. Both these features can be characterized rigorously by integral geometry analysis of fluorescence micrographs. This approach is introduced here to compare the relative protein adsorption onto various polymer surfaces: polystyrene (PS), poly(methyl methacrylate) (PMMA), poly( n-butyl methacrylate) (PnBMA), poly( tert-butyl methacrylate) (PtBMA), and PS(PETA) and cross-linked poly(ethylene oxide) (PEO*(PETA)), admixed with pentaerythritol triacrylate (PETA). The polymeric surfaces were incubated for 15 min in phosphate-buffered saline (pH 7.4) containing 125 mug/mL fluorescently labeled lectins, either lentil lectin (LcH) or concanavalin A (ConA). Fluorescence images were recorded at identical conditions (physiological buffer, same exposure time, magnification, gain). For each image, taken a few times for each polymer, the distribution and average value of the normalized intensity were determined. The results show that the binding of LcH to PS(PETA), PtBMA, PS, PnBMA, PMMA, and PEO*(PETA) can be expressed by the ratio of the following values (mean +/- 95% confidence interval): 0.356 +/- 0.022, 0.298 +/- 0.030, 0.241 +/- 0.014, 0.083 +/- 0.008, 0.039 +/- 0.008, and 0.010 +/- 0.006, respectively. In turn, the relative adsorption of ConA is described by the values 0.252 +/- 0.016, 0.217 +/- 0.014, 0.222 +/- 0.016, 0.046 +/- 0.006, 0.116 +/- 0.008, and 0.006 +/- 0.002, respectively. Low dispersions of fluorescence intensity around average values indicate homogeneous distribution of adsorbed proteins. The introduced approach enables a fast and easy way not only to quantify the relative amount of bound proteins but also to characterize quantitatively the organization of their surface distribution, as demonstrated for patchlike protein adsorption onto the polymer blend surface.

Synthesis and Postpolymerization Modification of Thermoresponsive Coatings Based on Pentaerythritol Monomethacrylate: Surface Analysis, Wettability, and Protein Adsorption

Properties of novel temperature-responsive hydroxyl-containing poly(pentaerythritol monomethacrylate) (PPM) coatings, polymerized from oligoperoxide grafted to glass surface premodified with (3-aminopropyl)triethoxysilane, are presented. Molecular composition, chemical state, thickness, and wettability are examined with time of flight-secondary ion mass spectrometry (ToF-SIMS), X-ray photoelectron spectroscopy (XPS), ellipsometry, and contact angle measurements, respectively. Temperature-induced changes in hydrophobicity of grafted PPM brushes are revealed by water contact angle and ellipsometric measurements. Partial postpolymerization modification of hydroxyl groups (maximum a few percent), performed with acetyl chloride or pyromellitic acid chloride, is demonstrated to preserve thermal response of coatings. Adsorption of bovine serum albumin to PPM brushes, observed with fluorescence microscopy, is higher than on glass in contrast to similar hydroxyl-containing layers reported as nonfouling. Enhanced and temperature-controlled protein adsorption is obtained after postpolymerization modification with pyromellitic acid chloride.

Temperature-responsive properties of poly(4-vinylpyridine) coatings: influence of temperature on the wettability, morphology, and protein adsorption

Although the pH-response of poly(vinylpyridine)-based systems is well-known and indeed used in several biomedical applications, the impact of temperature on the properties of this polymer has not been investigated in detail so far. Herein, we demonstrate the temperature-responsiveness and switchable wettability of two poly(4-vinylpyridine) coatings, mimicking the behavior of materials with lower critical solution temperature. The thermal response of P4VP spin-coated films, solvent cast on a glass, is weaker than that observed for P4VP-grafted brushes, fabricated via polymerization from an oligoperoxide grafted on an amino-silanized glass. Both the P4VP coatings exhibit a temperature dependence of the water contact angle with a well-defined transition at 13–14 °C. This transition is absent at acid pH levels wherein almost all pyridyl groups are protonated. The P4VP-grafted brushes were used to examine the impact of temperature on the surface morphology and protein adsorption. The coating surface, recorded with atomic force microscopy, evolved noticeably at alkaline pH, from being relatively smooth at 10 °C to structured and rough at 20 °C. In turn, at acid pH levels, flat surfaces with rare elevations were observed at both temperatures. The adsorption of bovine serum albumin and human fibrinogen was observed with fluorescence microscopy to be significantly more efficient for temperatures above the transition, indicating that P4VP coatings can act as a noteworthy switching material.

Proteins grouped into a variety of regular micro-patterns by substrate-guided domains of self-assembling poly(ethylene oxide)/polystyrene blends

Spin-casting of polymer blends provides one-step deposition and self-assembly of domains with contrasting surface properties. Resulting irregular structures are commonly used to guide protein adsorption and cell seeding. However, a more regular arrangement of biological material is required for more advanced biomedical applications. In this report, blends of poly(ethylene oxide) (PEO) and polystyrene (PS) (1 : 1 and 1 : 2 w/w) admixed with pentaerythritol triacrylate spin-cast (with inherent domain scale 1.6 ≤ 2R ≤ 4.0 μm) onto gold, micro-contact printed with hexadecanethiol (SAM) stripes (with periodicity λ = 4 and 8 μm), and cross-linked with ultraviolet are used as adsorption templates to group fluorescently labelled concanavalin A (ConA) into periodic protein micro-patterns with different morphologies depending on the 2R/λ ratio: strings of islands (2R/λ ≈ 0.2), branched stripes (∼0.33), stripe pairs (∼0.5) and stripes (∼1). Hierarchical (for 2R/λ < 1) protein micro-patterns reflect the phase rich in PS, assembled during spin-casting into domains elevated above the neighbouring PEO-rich phase on Au regions, and covered by the PEO-rich lamella with intermediate height on periodically repeated SAM areas. The relation between long-ranged regular ordering of blend films (adsorption templates), visualized with atomic force microscopy, and micro-patterns (grouped proteins), revealed with fluorescence microscopy, is examined with Fourier analysis.

Reverse contrast and substructures in protein micro-patterns on 3D polymer surfaces.

We characterize an approach enabling protein patterning over broad polymer areas based on selective protein adsorption on surfaces of spin-cast amino-terminated polystyrene structured topographically with elastomer molds (capillary force lithography) and passivated locally against adsorption with poly(ethylene oxide)-silanes printed with flat elastomer stamps (inverted micro-contact printing). Atomic force microscopy reveals uniformity of PS-NH(2) films with stripes of grooves and elevations alternating with periodicity 4<λ<200 μm. Film morphologies, prior and after selective adsorption of model protein, are mapped with optical and fluorescence microscopes, respectively. The examination with the Fourier analysis shows that elevated regions of polymer relief are replicated as dark or bright stripes on fluorescent micrographs for elevations forming plateaus (>3 μm) or narrow ridges, respectively. Reverse contrast in protein micro-patterns is induced by modified relief geometry, which affects surface flux of silanes from stamp to polymer surface both within and away from contact zones of micro-contact printing. In addition, protein substructures with a fraction λ/n of relief periodicity are observed on surfaces with elevated ridges (n=2) and plateaus (n=2 and 4). This is due to the locally modified protein adsorption with silane concentration and surface topography, respectively.

Self-organisation of di(perfluorohexyl)hexane in Langmuir and LB films

ABSTRACT Symmetrical triblock semifluorinated n-alkane, di(perfluorohexyl)hexane of the formula F(CF2)6(CH2)6(CF2)6F (abbreviated F6H6F6), has been synthesised and investigated at the air/water interface. Our results show for the first time that this unusual film-forming material, completely hydrophobic in nature and possessing no polar group, is capable of stable film formation at the free water surface. The surface pressure–area isotherm of the studied compound exhibited two regions: corresponding to monotonous pressure rise, followed by a pseudo-plateau region. Visualisation of film structure with Brewster angle microscope (BAM) proved the formation of domains within the pseudo-plateau region. A closer insight into the structure of these domains with atomic force microscope (AFM) proved their ordered, circular shape. The average area of F6H6F6 domain was found to depend on surface pressure value, as it is 4.98 ± 1.75 μm2 at π = 1.2 mN/m to 16.54 ± 0.31 μm2 at π = 1.7 mN/m. Following performed quantum-chemical calculations, it can be concluded that the observed surface aggregates from F6H6F6 are formed by linear conformers with shifted CF and CH parts. The calculated domain thickness is between 20 and 21 Å, which perfectly agrees with the experimental value estimated from AFM measurements (20.3 ± 1.4 Å).

The influence of an antitumor lipid - erucylphosphocholine - on artificial lipid raft system modeled as Langmuir monolayer.

Abstract Outer layer of cellular membrane contains ordered domains enriched in cholesterol and sphingolipids, called ‘lipid rafts’, which play various biological roles, i.e., are involved in the induction of cell death by apoptosis. Recent studies have shown that these domains may constitute binding sites for selected drugs. For example alkylphosphocholines (APCs), which are new-generation antitumor agents characterized by high selectivity and broad spectrum of activity, are known to have their molecular targets located at cellular membrane and their selective accumulation in tumor cells has been hypothesized to be linked with the alternation of biophysical properties of lipid rafts. To get a deeper insight into this issue, interactions between representative APC: erucylphosphocholine, and artificial lipid raft system, modeled as Langmuir monolayer (composed of cholesterol and sphingomyelin mixed in 1:2 proportion) were investigated. The Langmuir monolayer experiments, based on recording surface pressure-area isotherms, were complemented with Brewster angle microscopy results, which enabled direct visualization of the monolayers structure. In addition, the investigated monolayers were transferred onto solid supports and studied with AFM. The interactions between model raft system and erucylphosphocholine were analyzed qualitatively (with mean molecular area values) as well as quantitatively (with ΔGexc function). The obtained results indicate that erucylphosphocholine introduced to raft-mimicking model membrane causes fluidizing effect and weakens the interactions between cholesterol and sphingomyelin, which results in phase separation at high surface pressures. This leads to the redistribution of cholesterol molecules in model raft, which confirms the results observed in biological studies.