ABSTRACT
Open-surface microfluidics is promising in terms of enabling economical and rapid biochemical analysis for addressing challenges associated with medical diagnosis and food safety. To this end, we present a simple and economical approach to develop an open-surface microfluidic platform suitable for facile liquid transport and mixing. Customizable patterns with tailored wettability are deposited using a plasma-assisted deposition technique under atmospheric pressure. The flow of the dispensed liquid is driven by gravity, and the tilting angle of the device determines the extent of mixing. First, a hexamethyldisiloxane film was deposited to create hydrophobic patterns on glass, and then, hydrophilic acrylic acid was deposited by a patterned cardboard mask to construct a channel suitable for forming channels to transport aqueous liquids without the need of an external energy input; the liquid can be confined to designated pathways. Several designs including Y-junctions, serpentine-shaped patterns, splitting channels, and concentration gradient generation patterns are presented. The proposed method can spatially pattern a surface with a hydrophobic/hydrophilic area, which can function as a microfluidic channel, and the surface can be applied in microfluidic devices with other types of substrates.
ABSTRACT
Glow discharge polymerization is not well understood due to the rapid/complex reaction at the plasma/gas precursor interface. Plasma reaction in a submerged condition allows post-plasma-polymerization, leading to further polymer growth and thus a stable structure. Electron collision with acetonitrile at the interface initiates the formation of radical monomers, which undergoes further rearrangement to form low-molecular (LM) nitrogen polymers (NPs). The radical-rich LM NPs go through further polymerization, forming stable high-molecular (HM) NPs (as determined using liquid chromatography/mass spectrometry). LM NPs absorb light at a wavelength of 270 nm (λ max) whereas HM NPs show absorption at 420 nm (λ max), as determined from ultraviolet-visible absorption spectra. The fluorescence spectra of HM NPs show characteristic emission at 430 nm, which indicates the presence of nitrogen functional groups with external conjugation. The proposed structure of HM NPs is verified with different analytical instruments.
Subject(s)
Nitrogen Compounds/chemical synthesis , Plasma Gases/chemistry , Polymers/chemical synthesis , Materials TestingABSTRACT
PURPOSE: A low-temperature low-energy capillary-tube-based argon micro-plasma system was applied to disinfect Streptococcus mutans-containing biofilm. MATERIALS AND METHODS: The micro-plasma system uses a hollow inner electrode that is ignited by a radio-frequency power supply with a matching network. The energy content was analyzed using optical emission spectroscopy. The micro-plasma-induced effect on a biofilm cultured for 24 or 48 h with a working distance of ≈3 mm at low temperature was evaluated. The morphologies of the treated live/dead bacteria and the produced polysaccharides after micro-plasma treatment were examined. RESULTS: Scanning electron microscopy images and staining results show that most of the S. mutans on the treated biofilm were acutely damaged within a micro-plasma treatment time of 300 s. CONCLUSIONS: The number of living bacteria underneath the treated biofilm greatly decreased with treatment time. The proposed micro-plasma system can thus disinfect S. mutans on/in biofilms.
Subject(s)
Biofilms/drug effects , Biofilms/radiation effects , Disinfection/instrumentation , Microtechnology/instrumentation , Plasma Gases/pharmacology , Tooth/microbiology , Cell Membrane/drug effects , Cell Membrane/radiation effects , Cell Survival/drug effects , Cell Survival/radiation effects , Streptococcus mutans/cytology , Streptococcus mutans/drug effects , Streptococcus mutans/radiation effects , Time FactorsABSTRACT
A custom-made atmospheric argon micro-plasma system was employed to dissociate dimethyl sulfide (DMS) into a non-foul-smelling species. The proposed system takes the advantages of low energy requirement and non-thermal process with a constant flow rate at ambient condition. In the experiments, the compositions of DMS/argon plasma, the residual gaseous phases, and solid precipitates were respectively characterized using an optical emission spectrometer, various gas-phase analyzers, and X-ray photoemission spectroscopy. For 400 ppm DMS introduced into argon plasma with two pairs of electrodes (90 W), a complete decomposition of DMS was achieved; the DMS became converted into excited species such as C, C(2), H, and CH. When gaseous products were taken away from the treatment area, the excited species tended to recombine and form stable compounds or species, which formed as solid particles and gaseous phases. The solid deposition was likely formed by the agglomeration of C-, H-, and S-containing species that became deposited on the quartz inner tube. For the residual gaseous phases, low-molecular-weight segments mostly recombined into relatively thermodynamic stable species, such as hydrogen, hydrogen sulfide, and carbon disulfide. The dissociation mechanism and treatment efficiency are discussed, and a treatment of converting DMS into H(2)-, CS(2)-, and H(2)S-dominant by-products is proposed.
Subject(s)
Air Pollutants/isolation & purification , Argon/chemistry , Electrochemical Techniques/methods , Plasma Gases/chemistry , Sulfides/isolation & purification , Air Pollutants/chemistry , Carbon/chemistry , Hydrogen/chemistry , Kinetics , Odorants/analysis , Sulfides/chemistry , VolatilizationABSTRACT
PURPOSE: An aqueous solution containing Escherichia coli can be completely inactivated within a short treatment time using a capillary-tube-based oxygen/argon micro-plasma source. MATERIALS AND METHODS: A capillary-tube-based oxygen/argon micro-plasma system with a hollow inner electrode was ignited by a 13.56 MHz radio frequency power supply with a matching network and characterised by optical emission spectroscopy. An aqueous solution containing E. coli was then treated at various the working distances, plasma exposure durations, and oxygen ratios in argon micro-plasma. The treated bacteria were then assessed and qualitatively investigated. The morphologies of treated bacteria were examined using a scanning electron microscope (SEM). RESULTS: In the proposed oxygen/argon micro-plasma system, the intensities of the main emission lines of the excited species, nitric oxide (NO), hydrated oxide (OH), argon (Ar), and atomic oxygen (O), fluctuated with the addition of oxygen to argon micro-plasma. Under a steady state of micro-plasma generation, the complete inactivation of E. coli in aqueous solution was achieved within 90 s of argon micro-plasma exposure time with a working distance of 3 mm. SEM micrographs reveal obvious morphological damage to the treated E. coli. The addition of oxygen to argon micro-plasma increased the variety of O-containing excited species. At a given supply power, the relative intensities of the excited species, NO and OH, correlated with the ultraviolet (UV) intensity, decreased. CONCLUSION: For the proposed capillary-tube-based micro-plasma system with a hollow inner electrode, the oxygen/argon micro-plasma source is efficient in inactivating E. coli in aqueous solution. The treatment time required for the inactivation process decreases with decreasing working distance or the increasing synthesised effect of reactive species and UV intensity.
Subject(s)
Argon/chemistry , Escherichia coli/physiology , Microbial Viability , Oxygen/chemistry , Plasma Gases/chemistry , Sterilization/instrumentation , Water/chemistry , Electrodes , Equipment Design , Escherichia coli/ultrastructure , Microscopy, Electron, Scanning , Solutions , Surface Properties , SuspensionsABSTRACT
Micro/nano-lithographic techniques are usually employed as a straightforward process for roughening a thin-film Au surface for surface-enhanced Raman scattering (SERS). However, a topographical pattern with deepened edges is difficult to control in a rapid and environmental-friendly way. In this study, a simple physical procedure is proposed for tailoring a thin-film Au surface with triangular nanostructures using nano-indentation technique. The as-fabricated nano-indented cavities on Au (nAu) were structured as a characterization substrate for SERS. By calculating the geometries of nAu and the increase of surface area as a function of the concentration of chemically adsorbed 2-nitro-5-thiobenzoic acid (NTB), a combined chemical and electromagnetic effect was estimated. Particularly-made nAu was adjusted for examining chemically adsorbed NTB molecules with differently intensified Raman-active groups by tuning the indentation depth and the tip-to-tip displacement. SERS enhancement factor on a specific NTB/nAu could be increased to 2.1×10(6).
Subject(s)
Dithionitrobenzoic Acid/chemistry , Gold , Molecular Probes/chemistry , Nanostructures , Spectrum Analysis, Raman/methods , Adsorption , Molecular Probe Techniques , Sulfhydryl Reagents , Surface PropertiesABSTRACT
PURPOSE: A radio-frequency dielectric barrier discharge (DBD) was applied as a micro-plasma device for the inactivation of bacteria, e.g., Escherichia coli. MATERIALS AND METHODS: The cultured bacteria were placed on a polydimethyl siloxane (PDMS) film and placed inside the DBD cavity. The bacteria were exposed to micro-plasmas of varying oxygen/argon ratios for different exposure times. The survival of the bacteria was measured by determining bacterial growth using optical methods. RESULTS: The excited oxygen species increased with the increase in the oxygen to argon ratio as measured by optical emission spectroscopy (OES), but the increase of excited oxygen species in argon micro-plasma did not enhance the inactivation of bacteria. In contrast, increases in the time the bacteria were exposed to the micro-plasma were of importance. The results show that a continuous plasma flow containing energetic and reactive species may result in electro-physical interactions with bacteria exposed to the plasma leading to their inactivation. CONCLUSION: For currently-employed DBD device, addition of 0.5% oxygen to the argon micro-plasma for an exposure time of 30 sec was optimum for the inactivation of E. coli.
Subject(s)
Argon/pharmacology , Escherichia coli/drug effects , Escherichia coli/physiology , Oxygen/pharmacology , Argon/chemistry , Atmosphere , Dimethylpolysiloxanes , Electric Impedance , Escherichia coli/growth & development , Free Radicals/pharmacology , Microbial Viability/drug effects , Oxygen/chemistry , Temperature , Time FactorsABSTRACT
The modification of octadecanethiolate self-assembled monolayers on Au and Ag by nitrogen-oxygen downstream microwave plasma with variable oxygen content (up to 1%) has been studied by synchrotron-based high-resolution X-ray photoelectron spectroscopy. The primary processes were dehydrogenation, desorption of hydrocarbon and sulfur-containing species, and the oxidation of the alkyl matrix and headgroup-substrate interface. The exact character and the rates of the plasma-induced changes were found to be dependent on the substrate and plasma composition, with the processes in the aliphatic matrix and headgroup-substrate interface being mostly decoupled. In particular, the rates of all major plasma-induced processes were found to be directly proportional to the oxygen content in the plasma, which can be, thus, considered as a measure of the plasma reactivity. Along with the character of the observed changes, exhibiting a clear dominance of the oxidative processes, this suggests that the major effect of the oxygen-nitrogen downstream microwave plasma is provided by reactive oxygen-derived species in the downstream region, viz. long-living oxygen radicals and metastable species.
ABSTRACT
Modification of octadecanethiolate self-assembled monolayers on Au by nitrogen-oxygen or argon-oxygen downstream microwave plasma with a low oxygen content (estimated below several percent) has been studied by synchrotron-based high-resolution X-ray photoelectron spectroscopy and water contact angle measurements. For both types of plasma, the primary processes were found to be the loss of conformational and orientational order and the oxidation of the alkyl matrix and headgroup-substrate interface. At the same time, the film modification occurred much faster and with different intermediates for the nitrogen plasma than for the argon plasma. The reasons for these differences are considered in terms of the different reactivities and different efficiencies of the energy transfer between the plasma constituents in these two types of plasma.
ABSTRACT
Exposure to ultra-violet (UV)-C radiation is a frequently used method to prevent bacteria from invasion of blood-contact biomedical products. Potential damage induced by UV radiation to collagen is of concern due to the decay of bioactivity, considerably correlated with structural alterations. Our current investigation studies the collagen-bonded non-woven polypropylene (PP) fabric surface. In this experiment, antenna-coupling microwave plasma is utilized to activate PP fabric and then the sample is grafted with acrylic acid (AAc). Type III collagen is immobilized by using water soluble 1-ethyl-3-(3-dimethylaminopropyl) carbodiimide as coupling agent. The collagen-bonded samples with sample temperature ca. 4 degrees C are then exposed to UV-254nm radiation for different time intervals. By using fourier-transformed infrared with attenuated total reflection (FTIR-ATR) and XPS (X-ray photoelectron spectroscopy), we examine the chemical structures of samples with different treatments. Coomassie brilliant blue G250 method is utilized to quantify the immobilized collagen on the PP fabric surfaces. Blood-clotting effects are evaluated by activated partial thromboplastin time, thrombin time, and fibrinogen concentration tests. By means of cell counter and scanning electron microscopy we count red blood cells and platelets adhesion in the modified porous matrix. Our experimental results have demonstrated that with pAAc-grafting of ca. 173 microg cm(-2) and immobilized collagen of 80.5+/-4.7 microg cm(-2), for human plasma incubated samples of various intervals of UV-254 nm radiation, fibrinogen concentration decreases in human plasma, while platelets and red blood cells adhesions increase before UV radiation. However, the required time for thrombination shows significant change for UV radiation exposure of less than 20 h (alpha = 0.05). The decay of bioactivity for the UV-irradiated, collagen-bonded surfaces is thus evaluated. Surface analyses indicate that the decrease of R-COOH (derivated from grafted-pAAc or de-carboxylation of collagen), amides degradation (broken-NH), and phenylalanine scission (terminated by -OH, tyrosine formation) may gradually damage collagen by increasing the intervals of UV radiation. These effects considerably influence the bioactivity of the collagen-bonded fabric. The XPS measurements of C 1s core levels at 288.4 eV (O = C-NH) and at 289.1 eV (O = C-O) illustrate significant decreases of intensity after radiation time ca. 44 h. It is clear that UV-254 nm radiation exposure for ca. 20 h has the potential impact to moderate the bioactivities of collagen and therefore act as a vital factor to accelerate biodegradation.
