Coatings of polyethylene glycol for suppressing adhesion between solid microspheres and flat surfaces

This article describes the development and the examination of surface coatings that suppress the adhesion between glass surfaces and polymer microspheres. Superparamagnetic doping allowed for exerting magnetic forces on the microbeads. The carboxyl functionalization of the polymer provided the means for coating the beads with polyethylene glycol (PEG) with different molecular weight. Under gravitational force, the microbeads settled on glass surfaces with similar polymer coatings. We examined the efficacy of removing the beads from the glass surfaces by applying a pulling force of ~1.2 pN. The percent beads remaining on the surface after applying the pulling force for approximately 5 s served as an indication of the adhesion propensity. Coating of PEG with molecular weight ranging between 3 and 10 kDa was essential for suppressing the adhesion. For the particular substrates, surface chemistry and aqueous media we used, coatings of 5 kDa manifested optimal suppression of adhesion: that is, only 3% of the microbeads remained on the surface after applying the pulling magnetic force. When either the glass or the beads were not PEGylated, the adhesion between them was substantial. Addition of a noncharged surfactant, TWEEN, above its critical micelle concentrations (CMCs) suppressed the adhesion between noncoated substrates. The extent of this surfactant-induced improvement of the adhesion suppression, however, did not exceed the quality of preventing the adhesion that we attained by PEGylating both substrates. In addition, the use of surfactants did not significantly improve the suppression of bead-surface adhesion when both substrates were PEGylated. These findings suggest that such surfactant additives tend to be redundant and that covalently grafted coatings of PEGs with selected chain lengths provide sufficient suppression of nonspecific interfacial interactions.     

Polyglycerol based coatings to reduce non-specific protein adsorption in sample vials and on SPR sensors

Coatings based on dendritic polyglycerol (dPG) were investigated for their use to control nonspecific protein adsorption in an assay targeted to analyze concentrations of a specific protein. We demonstrate that coating of the sample vial with dPG can significantly increase the recovery of an antibody after incubation. First, we determine the concentration dependent loss of an antibody due to nonspecific adsorption to glass via quartz crystal microbalance (QCM). Complementary to the QCM measurements, we applied the same antibody as analyte in an surface plasmon resonance (SPR) assay to determine the loss of analyte due to nonspecific adsorption to the sample vial. For this purpose, we used two different coatings based on dPG. For the first coating, which served as a matrix for the SPR sensor, carboxyl groups were incorporated into dPG as well as a dithiolane moiety enabling covalent immobilization to the gold sensor surface. This SPR-matrix exhibited excellent protein resistant properties and allowed the immobilization of amyloid peptides via amide bond formation. The second coating which was intended to prevent nonspecific adsorption to glass vials comprised a silyl moiety that allowed covalent grafting to glass. For demonstrating the impact of the vial coating on the accuracy of an SPR assay, we immobilized amyloid beta (Aβ) 1-40 and used an anti-Aβ 1-40 antibody as analyte. Alternate injection of analyte into the flow cell of the SPR device from uncoated and coated vials, respectively gave us the relative signal loss (1 − RU_uncoated/RU_coated) caused by the nonspecific adsorption. We found that the relative signal loss increases with decreasing analyte concentration. The SPR data correlate well with concentration dependent non-specific adsorption experiments of the analyte to glass surfaces performed with QCM. Our measurements show that rendering both the sample vial and the sensor surface is crucial for accurate results in protein assays.     

Permeability of anti-fouling PEGylated surfaces probed by fluorescence correlation spectroscopy

The present work reports on in situ observations of the interaction of organic dye probe molecules and dye-labeled protein with different poly(ethylene glycol) (PEG) architectures (linear, dendron, and bottle brush). Fluorescence correlation spectroscopy (FCS) and single molecule event analysis were used to examine the nature and extent of probe-PEG interactions. The data support a sieve-like model in which size-exclusion principles determine the extent of probe-PEG interactions. Small probes are trapped by more dense PEG architectures and large probes interact more with less dense PEG surfaces. These results, and the tunable pore structure of the PEG dendrons employed in this work, suggest the viability of electrochemically-active materials for tunable surfaces.     

Simple test system for single molecule recognition force microscopy

We have established an easy-to-use test system for detecting receptor-ligand interactions on the single molecule level using atomic force microscopy (AFM). For this, avidin-biotin, probably the best characterized receptor-ligand pair, was chosen. AFM sensors were prepared containing tethered biotin molecules at sufficiently low surface concentrations appropriate for single molecule studies. A biotin tether, consisting of a 6 nm poly(ethylene glycol) (PEG) chain and a functional succinimide group at the other end, was newly synthesized and covalently coupled to amine-functionalized AFM tips. In particular, PEG₈₀₀ diamine was glutarylated, the mono-adduct NH₂-PEG-COOH was isolated by ion exchange chromatography and reacted with biotin succinimidylester to give biotin-PEG-COOH which was then activated as N-hydroxysuccinimide (NHS) ester to give the biotin-PEG-NHS conjugate which was coupled to the aminofunctionalized AFM tip. The motional freedom provided by PEG allows for free rotation of the biotin molecule on the AFM sensor and for specific binding to avidin which had been adsorbed to mica surfaces via electrostatic interactions. Specific avidin-biotin recognition events were discriminated from nonspecific tip-mica adhesion by their typical unbinding force (∼40 pN at 1.4 nN/s loading rate), unbinding length (<13 nm), the characteristic nonlinear force-distance relation of the PEG linker, and by specific block with excess of free d-biotin. The convenience of the test system allowed to evaluate, and compare, different methods and conditions of tip aminofunctionalization with respect to specific binding and nonspecific adhesion. It is concluded that this system is well suited as calibration or start-up kit for single molecule recognition force microscopy.     

Sol–gel coatings with covalently attached methyl,octyl, and octadecyl ligands for capillary microextraction. Effects of alkyl chain length and sol–gel precursor concentration on extraction behavior

Fused silica capillaries with surface-bonded sol–gel coatings containing covalently attached octadecyl, octyl, and methyl groups were prepared for capillary microextraction (CME) hyphenated on-line with high-performance liquid chromatography (HPLC). For this, octadecyltrimethoxysilane (C₁₈TMS), octyltrimethoxysilane (C₈TMS), or methyltrimethoxysilane (MTMS) was used as the respective sol–gel precursor. Hydrolytic polycondensation of these precursors led to the formation of surface-bonded sol–gel sorbents with pendant alkyl groups ready to serve as the extraction medium; no additional surface derivatization reactions were needed to anchor these ligands to the surface. Extraction behaviors of two sets of microextraction capillaries with alkyl-bonded sol–gel coatings were investigated: (a) capillaries prepared with a constant molar concentration of these precursors in the sol solution, and (b) capillaries prepared with varied molar concentrations of C₈TMS in the sol solution. Among the capillaries prepared using sol solutions with the same molar concentration of sol–gel precursor, the detection limits for nonpolar and polar analytes ranged from 0.3 ng/L to 213.9 ng/L. The sol–gel octadecyl-coated capillaries were found to be the most efficient at extracting these analytes, followed by the sol–gel octyl-coated capillaries, followed by the sol–gel methyl-coated capillaries. The results of this study point to the possibility that polar analytes are extracted through synergistic molecular level interactions of the polar and nonpolar parts of the analyte molecules with the alkyl chains and silanol groups within the sol–gel coatings. These coatings also demonstrated run-to-run and capillary-to-capillary reproducibility, with HPLC peak area RSD values ranging from 1.1% to 9.6% and 1.3% to 10.0%, respectively. In the set of sol–gel octyl capillaries with varied molar concentrations, the capillaries prepared with 0.514 M concentration of C₈TMS in the sol solution were most efficient in extracting nonpolar and polar analytes. When higher or lower concentrations of C₈TMS were used in the sol solution, the resulting sol–gel coated capillaries were less efficient in extracting nonpolar and polar analytes.     

Characterization of 40 kDa poly(ethylene glycol) polymers by proton transfer reaction QTOF mass spectrometry and 1H-NMR spectroscopy

Several electrospray mass spectrometry (ESI-MS) techniques have been described during the past years to enable the characterization work of large poly(ethylene glycol)s (PEGs) and PEGylated proteins. The proton transfer reaction ESI-MS method utilizes amines to charge reduce the electrospray envelope of PEGs, hence PEG molecules are aminated instead of protonated. This method simplifies the mass spectrum of large PEGs, and enables the interpretation of the charge state of the observable envelopes (R ≥ 3,000 (FWHM) measured at the (M + 6H)⁶⁺ ion from 40 K PEG compound 7,324.19). Hence, deconvolution of the MS data can be performed and relative molecular masses of the individual chain lengths of the PEGs can be calculated. However, as the poly-dispersity of PEGs may vary from batch to batch and from sample to sample, it was of interest to examine if the method could distinguish between these kinds of different material. Therefore, sample materials of each intermediate obtained at five synthetic steps during synthesis of a 40 kDa PEG molecule were collected. These four intermediates, starting material and the target molecule were examined by ¹H-NMR spectroscopy and ESI-MS using a proton stripping base. The study revealed that the charge-stripping ESI-MS method is able to differentiate between even small changes in the structure of the polymeric molecules only when the analysis is assisted by ¹H-NMR spectroscopy. A proper characterization of polymer molecules requires besides relative molecular mass, also poly-dispersity and end-group characterization. No end-group information is obtained based on MS data. Examination of the PEG polymers by ¹H-NMR spectroscopy provides the needed information. In addition, the ¹H-NMR spectra clearly distinguishes the examined polymers.     

Preparation and structural evolution of SiO(2)-TiO(2) pillared layered manganese oxide nanocomposite upon intercalating reaction

Poly(ethylene glycol) possessing pentaethylenehexamine at one end (N6-PEG) was prepared via a reductive amination reaction of aldehyde-ended PEG with pentaethylenehexamine. Using N6-PEG, an antibody/PEG co-immobilized surface was constructed on magnetic particles via an active ester reaction method. After immobilization of the antibody on the active ester surface, N6-PEG was reacted on the magnetic beads. A sandwich enzyme-linked immunosorbent assay (ELISA) system was newly constructed using PEG/antibody co-immobilized magnetic beads combined with an alkaline phosphatase (ALP)-assisted fluorescent detection system using alpha-fetoprotein (AFP) as a model antigen. The co-immobilization of both antibody and PEG on the magnetic bead surfaces reduced the nonspecific adsorption of proteins from cell lysates. Especially, when the magnetic particle surface was modified by N6-PEG mixtures with different molecular weights of 6000 and 2500 (6 kDa:2.5 kDa=9:1 w/w), the nonspecific adsorption of proteins was strongly suppressed. It is rather surprising for us that the sensitivity of the antibody on the surface was enhanced significantly when the PEG tethered chain was constructed in between the surface antibodies. Consequently, the mixed N6-PEG treatment showed a much higher S/N ratio than for the corresponding beads treated with bovine serum albumin (BSA), a conventional blocking reagent. Actually, when alpha-fetoprotein was analyzed by the magnetic bead-assisted ELISA thus constructed, the S/N ratio was about 20-fold higher for the mixed coating with PEG (6 kDa):PEG (2.5 kDa)=9:1, compared to the conventional BSA.     

Versatile biosensor surface based on peptide nucleic acid with label free and total internal reflection fluorescence detection for quantification of endocrine disruptors

In recent years, the simultaneous detection of hundreds of substances has become increasingly important in medical diagnostics and environmental monitoring. This calls for methods that allow fast and simultaneous measurement of many analytes and require only a minimum of attendance. Biosensor-applications including easy implementation and long-term stability of the sensor element are more and more designed to meet these demands.In this paper, a surface based on covalently immobilised peptide nucleic acid (PNA) for the detection of different endocrine disruptors is used. The surface was characterised with a label free detection system, the reflectometric interference spectroscopy (RIfS). A hybridisation capacity with DNA oligonucleotides of 1.3 ng/mm² (180 fmol/mm²) on PNA-surfaces was achieved. The PNA transducer is stable for half a year and for more than 300 regeneration steps.With this modified surface various environmentally relevant endocrine disruptors could be detected by an immunoassay. The detection is done on an optical waveguide system, based on total internal reflection fluorescence (TIRF) by using an auxiliary-system consisting of a conjugate which is formed of DNA-oligomers and analyte-derivatives. The successive detection of different analytes on the same spot by using this auxiliary-system is demonstrated as one application of multianalyte detection. Quantification of different endocrine disruptors on the same PNA-surface is demonstrated by three calibration curves.     

Evaluation of doped and undoped poly (o‐anisidine) as sensing materials for a sensor array for volatile organic compounds

Poly (o‐anisidine) (PoANI) and PoANI doped with nickel oxide and zinc oxide were evaluated as sensing materials for four gas analytes (methanol, ethanol, acetone, and benzene). The sensing materials had high sensitivity (showing an affinity towards the target analytes even at low concentrations, in the range of 1‐5 ppm), but rather poor selectivity, especially when the gas analytes were in a mixture. To exploit the poor selectivity, the three sensing materials were combined into a sensor array using principal component analysis (PCA) as a sensing algorithm. It was found that using a sensor array, the four individual gases could be separated. However, when all four gases were present (in analyte mixtures), there was too much overlap in the responses to distinguish between individual gas analytes and their related mixtures.     

Effect of solution viscosity on dynamic surface tension detection

A dynamic surface tension detector (DSTD) was used to examine the molecular diffusion and surface adsorption characteristics of surface-active analytes as a function of solution viscosity. Dynamic surface tension is determined by measuring the differential pressure across the air/liquid interface of repeatedly growing and detaching drops. Continuous surface tension measurement throughout the entire drop growth is achieved for each eluting drop (at a rate of 30 drops/min for 2 μl drops), providing insight into the kinetic behavior of molecular diffusion and orientation processes at the air/liquid interface. Three-dimensional data are obtained through a calibration procedure previously developed, but extended herein for viscous solutions, with surface tension first converted to surface pressure, which is plotted as a function of elution time axis versus drop time axis. Thus, an analyte that lowers the surface tension results in an increase in surface pressure. The calibration procedure derived for the pressure-based DSTD was successfully extended and implemented in this report to experimentally determine standard surface pressures in solutions of varied viscosity. Analysis of analytes in viscous solution was performed at low analyte concentration, where the observed analyte surface activity indicates that the surface concentration is at or near equilibrium when in a water mobile phase (viscosity of 1.0 Cp). Two surface-active analytes, sodium dodecyl sulfate (SDS) and polyethylene glycol (MW 1470 g/mol, PEG 1470), were analyzed in solutions ranging from 0 to 60% (v/v) glycerol in water, corresponding to a viscosity range of 1.0-15.0 Cp. Finally, the diffusion-limited surface activity of SDS and PEG 1470 were observed in viscous solution, whereby an increase in viscosity resulted in a decreased surface pressure early in drop growth. The dynamic surface pressure results reported for SDS and PEG 1470 are found to correlate with solution viscosity and analyte diffusion coefficient via the Stokes-Einstein equation.     

Reflectometric interference spectroscopy (RIfS) as a new tool to measure in the complex matrix milk at low analyte concentration

Measurements in complex matrices like milk still present a challenge in biosensor development. This is especially important when using a label-free detection method or when measuring low analyte concentrations. The direct optical method reflectometric interference spectroscopy (RIfS) was used for investigating matrix effects in immunoassay development. Furthermore, approaches to reduce these effects have been established. As a model system, the hormone testosterone has been chosen because this immunoassay has been well characterized in buffer. In a first step, the immunoassay for the detection of testosterone in buffer was improved beyond former published results. Therefore, the sensor surface was optimized, resulting in a fivefold lower limit of detection (70.2 ng L⁻¹) and limit of quantification (130.0 ng L⁻¹). Additionally, the assay time could be reduced to 15 min. Consequently, we used this improved assay to investigate matrix effects of whole pasteurized bovine milk. To minimize these effects, the surface chemistry was adapted and a suitable evaluation method was established, reducing the effects of Tyndall scattering and nonspecific binding to the sensor surface. These improvements allow for very reliable quantitative measurements in milk. The assay developed required no sample pretreatment and allowed for the regeneration of the sensor surface so that calibration could be performed on one chip. The calibration in milk (3.5% fat) resulted in a limit of detection of 94.4 ng L⁻¹ and a limit of quantification of 229.3 ng L⁻¹. Furthermore, recovery rates between 70% and 120% could be obtained. Thus, for the first time, an analyte in the matrix milk was successfully quantified with RIfS at low concentrations.     

Signal enhancement in laser diode thermal desorption‐triple quadrupole mass spectrometry analysis using microwell surface coatings

Laser‐diode thermal desorption (LDTD) is an ionization source usually coupled to triple quadrupole mass spectrometry (QqQMS) and specifically designed for laboratories requiring high‐throughput analysis. It has been observed that surface coatings on LDTD microwell plates can improve the sensitivity of the analysis of small polar molecules. The objective of the present study is to understand and quantify the effect of microwell surface coatings on signal intensity of small organic molecules of clinical, environmental, and forensic interest. Experiments showed that the peak areas of diclofenac, chloramphenicol, salicylic acid, and 11‐nor‐9‐carboxy‐Δ⁹‐tetrahydrocannabinol obtained by LDTD‐QqQMS increased by up to 3 orders of magnitude when using microwells coated with ethylenediaminetetraacetic acid (EDTA). Tests with different chelating agents and polytetrafluoroethylene as microwell surface coatings showed that nitrilotriacetic acid gave significantly higher peak areas for five out of the nine compounds that showed signal enhancement using chelating agents as coatings. Scanning electron microscopy studies of EDTA‐coated and uncoated microwells showed that analytes deposited in the former formed more uniform and thinner films than in the latter. The enhancement effect of surface coatings in LDTD‐QqQMS was explained mainly by the formation of homogenous and thinner layers of nanocrystals of analytes that are easier to desorb thermally than the layers formed when the analytes dry in direct contact with the bare stainless‐steel surface. Chemisorption of some analytes to the stainless‐steel surface of the microwell plate appeared to be a minor factor. Surface coatings widen the number of compounds analyzable by LDTD‐QqQMS and can also improve sensitivity and limits of detection.     

The adsorption of salicylic acid onto γ-alumina and kaolinite from solution in hexane studied using diffuse reflectance infrared Fourier transform spectroscopy (DRIFT)

It was possible to determine the maximum loading of salicylic acid adsorbed onto γ-alumina and kaolinite clay after exposure to salicylic acid dissolved in hexane by examination using diffuse reflectance infrared Fourier transform infrared spectroscopy (DRIFTS). The maximum surface loading of salicylic acid (which resisted washing with fresh hexane) on γ-alumina was four times that observed using water as a solvent (approximately 3.0 compared with 0.7 molecules/nm²). Washing the sample with water removed the organic which was in excess to the maximum level observed for samples prepared with aqueous solution. The spectra of samples prepared with a loading up to the maximum observed with aqueous solution showed no significant differences to those of samples where the organic had been adsorbed from hexane (with the same surface loading). New peaks were observed for loadings greater than 1 molecules/nm², but the salicylic acid was still present as carboxylate (with no clear evidence for the carbonyl group). Salicylic acid adsorbed more readily to the surface of kaolinite from solution in hexane than from aqueous solution (up to maximum average loading of 2 molecules/nm²). Washing the samples with water removed the organic to a loading in the region of 0.2 molecules/nm², independent of the initial loading. Salicylic acid was adsorbed onto kaolinite as the carboxylate. The findings indicate that uptake is mediated by a surface water layer even in the absence of bulk water.     

High swelling gels for sensing applications

Crosslinked hydrophilic polymers of different chemical structures can be used as sensor coatings for the detection of gaseous analytes. If their crosslink density is low, these materials behave in aqueous media as soft hydrogels with high swelling capacity. From a physico-mechanical standpoint, they are amorphous rubber-like materials, with high flexibility of their macromolecular chains. This property is particularly significant in view of applications in the sensors field, because it favours diffusion of the analyte molecules through the coating layer. This paper deals with the application of poly(ethylene glycols) (PEG)- and poly(N-vinylpyrrolidinone) (PVP)-based crosslinked resins as relative humidity (RH) sorbing materials, and of a poly(amidoamine)(PAA)-based resin as SO₂-sorbing material. The electronic devices used for evaluating the sorption capability of these polymeric coatings were gravimetric resonant sensors. Resins of various crosslink density, and therefore of various swelling ratios in water, were purposely prepared and characterized. Thin coating, layers, prepared by casting from dilute aqueous suspensions of the resins, previously micronized in water, were used for sorption experiments. All experiments were performed in controlled RH and temperature environments.     

Linear Poly(methyl glycerol) and Linear Polyglycerol as Potent Protein and Cell Resistant Alternatives to Poly(ethylene glycol)

The nonspecific interaction of proteins with surfaces in contact with biofluids leads to adverse problems and is prevented by a biocompatible surface coating. The current benchmark material among such coatings is poly(ethylene glycol) (PEG). Herein, we report on the synthesis of linear polyglycerol derivatives as promising alternatives to PEG. Therefore, gold surfaces as a model system are functionalized with a self‐assembled monolayer (SAM) by a two‐step anhydride coupling and a direct thiol immobilization of linear poly(methyl glycerol) and polyglycerol. Surface plasmon resonance (SPR) spectroscopy reveals both types of functionalized surfaces to be as resistant as PEG towards the adsorption of the test proteins fibrinogen, pepsin, albumin, and lysozyme. Moreover, linear polyglycerols adsorb even less proteins from human plasma than a PEG‐modified surface. Additional cell adhesion experiments on linear poly(methyl glycerol) and polyglycerol‐modified surfaces show comparable cell resistance as for a PEG‐modified surface. Also, in the case of long‐term stability, high cell resistance is observed for all samples in medium. Additional in vitro cell‐toxicity tests add to the argument that linear poly(methyl glycerol) and polyglycerol are strong candidates for promising alternatives to PEG, which can easily be modified for biocompatible functionalization of other surfaces.     

Semiconductor sensor embedded microfluidic chip for protein biomarker detection using a bead-based immunoassay combined with deoxyribonucleic acid strand labeling

Two major issues need to be addressed in applying semiconductor biosensors to detecting proteins in immunoassays. First, the length of the antibody on the sensor surface surpasses the Debye lengths (approximately 1 nm, in normal ionic strength solution), preventing certain specifically bound proteins from being tightly attached to the sensor surface. Therefore, these proteins do not contribute to the sensor’s surface potential change. Second, these proteins carry a small charge and can be easily affected by the pH of the surrounding solution. This study proposes a magnetic bead-based immunoassay using a secondary antibody to label negatively charged DNA fragments for signal amplification. An externally imposed magnetic force attaches the analyte tightly to the sensor surface, thereby effectively solving the problem of the analyte protein’s distance to the sensor surface surpassing the Debye lengths. In addition, a normal ion intensity buffer can be used without dilution for the proposed method. Experiments revealed that the sensitivity can be improved by using a longer DNA fragment for labeling and smaller magnetic beads as solid support for the antibody. By using a 90 base pair DNA label, the signal was 15 times greater than that without labeling. In addition, by using a 120 nm magnetic bead, a minimum detection limit of 12.5 ng mL⁻¹ apolipoprotein A1 can be measured. Furthermore, this study integrates a semiconductor sensor with a microfluidic chip. With the help of microvalves and micromixers in the chip, the length of the mixing step for each immunoassay has been reduced from 1 h to 20 min, and the sample volume has been reduced from 80 μL to 10 μL. In practice, a protein biomarker in a urinary bladder cancer patient’s urine was successfully measured using this technique. This study provides a convenient and effective method to measure protein using a semiconductor sensor.     

Dense passivating poly(ethylene glycol) films on indium tin oxide substrates

We describe the formation and characterization of surface-passivating poly(ethylene glycol) (PEG) films on indium tin oxide (ITO) glass substrates. PEG chains with a molecular weight of 2000 and 5000 D were covalently attached to the substrates in a systematic approach using different coupling schemes. The coupling strategies included the direct grafting with PEG-silane, PEG-methacrylate, and PEG-bis(amine), as well as the two-step functionalization with aldehyde-bearing silane films and subsequent coupling with PEG-bis(amine). Elemental analysis by X-ray photoelectron spectroscopy (XPS) confirmed the successful surface modification, and XPS and ellipsometry provided values for film thicknesses. XPS and ellipsometry thickness values were almost identical for PEG-silane films but differed by up to 400% for the other PEG layers, suggesting a homogeneous layer for PEG-silane but an inhomogeneous distribution for other PEG coatings on the molecularly rough ITO substrates. Atomic force microscopy (AFM) and water contact angle goniometry confirmed the different degrees of surface homogeneity of the polymer films, with PEG-silane reducing the AFM rms surface roughness by 50% and the water contact angle hysteresis by 75% compared to uncoated ITO. The ability of the PEG layers to passivate the substrate against the nonspecific adsorption of biopolymers was tested using fluorescence-labeled immunoglobulin G and DNA oligonucleotides in combination with fluorescence microscopy. The results indicate a positive relationship between film density and homogeneity on one hand and the ability to passivate against biopolymer adhesion on the other hand. The most homogeneous layers prepared with PEG-silane reduced the nonspecific adsorption of fluorescence-labeled DNA by a factor of 300 compared to uncoated ITO. In addition, the study finds that the ratio of film thicknesses derived by ellipsometry and XPS is a useful parameter to quantify the structural integrity of PEG layers on molecularly rough ITO surfaces. The findings may be applied to characterize PEG or other polymeric films on similarly coarse substrates.     

Fast and sensitive trace analysis of malachite green using a surface-enhanced Raman microfluidic sensor

A rapid and highly sensitive trace analysis technique for determining malachite green (MG) in a polydimethylsiloxane (PDMS) microfluidic sensor was investigated using surface-enhanced Raman spectroscopy (SERS). A zigzag-shaped PDMS microfluidic channel was fabricated for efficient mixing between MG analytes and aggregated silver colloids. Under the optimal condition of flow velocity, MG molecules were effectively adsorbed onto silver nanoparticles while flowing along the upper and lower zigzag-shaped PDMS channel. A quantitative analysis of MG was performed based on the measured peak height at 1615 cm⁻¹ in its SERS spectrum. The limit of detection, using the SERS microfluidic sensor, was found to be below the 1–2 ppb level and this low detection limit is comparable to the result of the LC-Mass detection method. In the present study, we introduce a new conceptual detection technology, using a SERS microfluidic sensor, for the highly sensitive trace analysis of MG in water.     

Development of dextran-derivative arrays to identify physicochemical properties involved in biofouling from serum

To control protein adsorption on surfaces, low-fouling polymer coatings such as poly(ethylene oxide) (PEG or PEO) and polysaccharides are used. Their ability to resist protein adsorption is related to the layer structure, hence the immobilization mode. A polymer array technology was developed to study the structural diversity of carboxymethyl dextran (CMD) layers, whose immobilization conditions were varied. CMD arrays were analyzed by X-ray photoelectron spectroscopy (XPS) and by atomic force microscopy (AFM) colloidal probe force measurements. Serum protein adsorption was studied directly on the CMD arrays using surface plasmon resonance (SPR) microscopy. Physicochemical characterization revealed that pinning density regulates surface coverage and the amount of adsorbed molecules, and that salt concentration influences the surface structure of the charged polymer, forming extended or short layers. Protein adsorption experiments from serum showed that repulsive CMD layers are dense, with extended flexible chains. The present study underlines the usefulness of polymer arrays to study structural diversity of thin graft layers and to relate their physicochemical properties to their resistance to nonspecific protein adsorption.     

Surface characterization of poly(L-lactic acid)-methoxy poly(ethylene glycol) diblock copolymers by static and dynamic contact angle measurements, FTIR, and ATR-FTIR

The surface composition and surface free energy properties of two types of amphiphilic and semicrystalline diblock copolymers consisting of poly(L-lactic acid) coupled to (methoxy poly(ethylene glycol) (PLLA-MePEG) having differing block lengths of PEG were investigated by using static and dynamic contact angle measurements, transmission Fourier infrared spectroscopy (FTIR), and attenuated total reflection spectroscopy (ATR-FTIR) and compared with results obtained from PLLA and MePEG homopolymers. The contact angle results were evaluated by using the van Oss-Good method (acid-base method), and it was determined that the Lewis base surface tension coefficient (gamma-) of the copolymers increased with an increase of the PEG molar content at the copolymer surface. This result is in good agreement with the transmission FTIR and ATR-FTIR results but not proportional to them, indicating that the surfaces of the copolymers are highly mobile and that the molecular rearrangement takes place upon contact with a polar liquid drop. The dynamic contact angle measurements showed that the strong acid-base interaction between the oxygen atoms in the copolymer backbone of the relatively more hydrophilic PEG segments with the Lewis acidic groups of the polar and hydrogen-bonding water molecules enabled the surface molecules to restructure (conformational change) at the contact area, so that the PEG segments moved upward, whereas the apolar methyl pendant groups of PLLA segments buried downward.