The relationship between surface chemistry and morphology of flame treated low-density polyethylene (LDPE) was studied by various characterization techniques across different length scales. The chemical composition of the surface was determined on the micrometer scale by Xray photoelectron spectroscopy (XPS) as well as with time of flight secondary ion mass spectrometry (ToF-SIMS), while surface wettability was obtained through contact angle (CA) measurements on the millimeter scale. The surface concentration of hydroxyl, carbonyl and carboxyl groups, as a function of the ''number'' of the flame treatment passes (which is proportional to the treatment time) was obtained. Moreover, a correlation was found with chemical composition and polarity, emphasizing the role of oxygen-containing functional groups introduced during the treatment. Carboxyl functional groups were specifically identified by fluorescent labeling and the results were compared with the ToF-SIMS data. In addition, atomic force microscopy (AFM) was used to evaluate changes in surface topography and roughness on the nanometer to micrometer length scales. After flame treatment, water-soluble low molecular weight oxidized materials (LMWOM), which were generated as products of oxidation and chain scission of the LDPE surface, agglomerated into small topographical mounds that were visible in the AFM micrographs. After rinsing the flame treated samples with water and ethanol, bead-like nodular surface structures were observed. The ionization state of flame treated LDPE surfaces was monitored by chemical force microscopy (CFM). The effective surface pK a values of carboxylic acid (-COOH) obtained by AFM were revealed by chemical force titration curves and the effective surface pK a values were found to be around 6. #
The surface chemistry and ionization state of cross-linked poly(dimethylsiloxane) (PDMS) exposed to UV/ozone were studied as a function of treatment time. Various complementary and independent experimental techniques were utilized, which yielded information on the macroscopic as well as the nanometric scale. The average chemical composition of the PDMS surface was quantitatively investigated by time-of-flight secondary ion mass spectrometry (ToF-SIMS). It was found that the top 1-2 nm surface layer was dominated by silanol groups (-SiOH) for which the concentration increased with increasing treatment dose. The lateral distributions of the silanol groups were analyzed on the nanometer scale by means of atomic force microscopy (AFM) with chemically functionalized tip probes in aqueous buffer solutions at varying pHs. Spatially dependent pull-off force curves (also called "force volume" imaging) indicated the presence of strong chemical heterogeneity of the probed surface. This heterogeneity took the form of patches of silanol functionalities with high local concentration surrounded by a matrix of predominantly hydrophobic domains at low pH. The average pull-off forces for the entire surface scanned were significantly reduced for pH values larger than a characteristic pK(a) constant (in the range between 4.5 and 5.5). The extent of the decrease in the pull-off force and the particular value of pK(a) were found to be a function of treatment time and to differ from the commonly reported values for silanol functional groups on a homogeneous silica surface. These dependences were ascribed to the evoking of a protonation/deprotonation process of the surface silanol groups which was sensitive to the hydrophobic/hydrophilic balance of their close molecular environment. Intermolecular hydrogen bonding may also account for the shifts in the surface pK(a). Furthermore, depending on the nature of the electrolyte, a third effect related to double layer composition, as determined by specific ion adsorption, was quantitatively analyzed by streaming potential measurements in the presence of sodium chloride and phosphate electrolytes.
Nucleic acid chips are based on the method of sequencing by hybridization, where unknown DNA fragments are hybridized to complementary nucleic acid sequences that are immobilized on a solid surface in an array format. One novel approach is to use peptide nucleic acid (PNA) biosensor chips. These DNA analogue possess the ability to hybridize with complementary DNA sequences. Because the backbone of DNA contains phosphates as opposed to PNA that does not, a technique that identifies the presence of these phosphates in a molecular surface layer would allow unlabelled DNA fragments hybridized to complementary PNAs to be detected. We have successfully shown that time-of-flight secondary ion mass spectrometry (ToF-SIMS) is a very useful tool for identifying hybridized DNA on PNA biosensor chips by detecting the phosphorus present in the DNA. ToF-SIMS is also a very effective technique for studying the complexity of the immobilization and hybridization process.
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