Small angle X-ray scattering study of chiral side chain liquid crystalline polymers in 5CB and 8CB solvents

Small angle X-ray scattering was used to examine the new chiral side chain liquid crystalline polyacrylates (P_4M and P_11M) and their mixtures (2?wt?%) in the low molar mass nematogenics 4′-n-pentyl-4-cyanobiphenyl (5CB) and 4′-octyl-4-cyanobiphenyl (8CB). Complementary data were obtained by polarizing optical microscopy. In agreement with previous studies, the mesophases of the bulk polymers show a dependence on the aliphatic spacers linking the mesogenic units to the polymer backbone. Chiral nematic and smectic A₁ phases were observed for the polyacrylates with four (P_4M) and eleven (P_11M) methylene units as spacers, respectively. In solution with 5CB and 8CB, P_4M exhibits an injected smectic phase, whereas P_11M maintains the smectic arrangement already observed in the bulk, with swollen smectic layers. In all the mixtures, layer stability was found to depend on the liquid crystal used as solvent, as well as on the temperature. At temperatures corresponding to the nematic 5CB and 8CB, the coexistence of two mesophases was observed in the mixtures. Moreover, with the liquid crystal solvents in the isotropic phase, microstructures suspended in the solvent matrix containing the liquid crystalline polymer in the smectic arrangement were detected.     

Heterogenic catalytic hydrolysis and analysis of natural pyrethrins in subcritical water coupled with solid phase microextraction (SPME) and GC-MS

The methodology for the detection of picogram quantities of nucleotides directly from TLC plates without the use of radioactive labeling has been developed. The method couples thin-layer chromatography (TLC) separation with matrix-assisted laser desorption/ionization mass spectrometry (MALDI MS) detection. The TLC/MALDI coupling protocol was studied and optimized for the separation and detection of deoxyribonucleotides. Several ammonia based solvents were examined as potential extraction solvents for the TLC/MALDI coupling protocol. It was found that in order to obtain maximum MALDI signal intensity and minimal analyte spreading, the extraction solvent should produce R_f-values for the analytes in the range of 0.3–0.4. R_f-values above this range led to extensive analyte spreading and those below this range resulted in poor extraction. Various MALDI matrices and co-matrices were investigated, the best results were obtained using 2′,4′,6′-trihydroxyacetophenone (THA) as a matrix. The extraction solvent chosen was an ammonium hydroxide/methanol (100 mM/30%, R_f = 0.28–0.38) solvent system which was found to provide the best sensitivity, minimal lateral spreading and excellent matrix transfer. Using the optimized coupling protocol, the detection limits for the deoxyribonucleotide monophosphates were established at or better than 10 picograms. Received: 27 May 1998 / Revised: 18 June 1999 / Accepted: 22 June 1999     

Physicochemical constants as a factor determining the need for the derivatization of organic substances in analysis by gas chromatography

A criterion was proposed to estimate the necessity of the derivatization of organic substances for their determination on conventional nonpolar phases, based on such characteristic of analytes as molecular weight (M _r), normal boiling point (T _bp), and molar refraction (MR _D). All these constants can be presented as indices relative to nonpolar n-alkanes (similarly to chromatographic retention indices), I(M), I(T), and I(MR _D), which can be compared to each other as differences Δ_{T − M} = I(T) − I(M) and Δ_{T − M} R _D = I(T) − I(MR _D). Substances do not require derivatization if Δ_{T − M} < 400 and Δ_{T − M} R _D < 600, while at Δ_{T − M} > 600 and Δ_{T − MRD} > 800, derivatization is necessary.     

Automated coupling of capillary-HPLC to matrix-assisted laser desorption/ionization mass spectrometry for the analysis of small molecules utilizing a reactive matrix

This study describes the application of a novel, reactive matrix for the mass spectral analysis of steroids by capillary-high performance liquid chromatography (capillary-HPLC) coupled to matrix-assisted laser desorption/ionization (MALDI). The mass spectral analysis of steroids was accomplished after fully automated peak deposition of chromatographic peaks onto MALDI targets. The seven corticosteroids used as test compounds were: triamcinolone, prednisone, cortisone, fludrocortisone, dexamethasone, deoxycorticosterone, and budesonide. They were separated using a PepMap C₁₈ (3 m particle size, 100 Å pore width) column at five different concentration levels of 25, 15, 7.5, 2.5 and 1 ng/L, and the peaks were detected at a wavelength of 237 nm. The column effluent was mixed with 2,4-dinitrophenylhydrazine (DNPH) directly following the UV detector. The chromatographic peaks were then deposited onto the MALDI target with a robotic micro-fraction collector triggered by the UV detector signals. A special hydrophobic surface coating allowed the deposition of up to 4 L (up to 90 % of the chromatographic peak volume) onto one sample spot. The compounds were then identified by MALDI mass spectrometry. Depending on the nature of the analyte, radical cations ([M]^+.) and sodium adduct ions ([M+Na]⁺) of the steroids as well as protonated steroid-dinitrophenylhydrazone derivatives ([M_D+H]⁺) were detected in positive ion mode. The detection limits were between 0.5 and 15 ng injected with capillary-HPLC-MALDI-TOF-MS and between 0.3 and 3 ng on target with MALDI-TOF when deposited manually.     

Effect of solvent in radical polymerization of butadiene 1-carboxylic acid

The radical polymerization and copolymerization of butadiene 1-carboxylic acid (Bu-1-Acid) were studied in a variety of the electron-donor solvents such as dimethylformamide (DMF), tetrahydrofuran (THF), methyl ethyl ketone (MEK), acetonitrile (ACN), and benzene (BZ) using AIBN as an initiator at 50°C. Under these conditions, the polymerization rate of Bu-1-Acid increased in the order, DMF < THF < MEK < ACN < BZ in the various solvents. In copolymerization with styrene [M₂] and acrylonitrile [M₂], the monomer reactivity ratio r₁ increased and r₂ decreased in the same order. Moreover, it was found that Alfrey-Price Q-e value of Bu-1-Acid increased depending on solvent in the order DMF < THF < MEK < ACN < BZ. These variations were correlated to the electron-donating power (Δvcm^?) of the solvents used and are discussed on the basis of the solvation of Bu-1-Acid into the solvent. Also, it was found that the microstructures of these polymers were always trans-1,4 and did not change with the solvent used.     

On‐target separation of analyte with 3‐aminoquinoline/α‐cyano‐4‐hydroxycinnamic acid liquid matrix for matrix‐assisted laser desorption/ionization mass spectrometry

3‐Aminoquinoline/α‐cyano‐4‐hydroxycinnamic acid (3AQ/CHCA) is a liquid matrix (LM), which was reported by Kumar et al. in 1996 for matrix‐assisted laser desorption/ionization (MALDI) mass spectrometry. It is a viscous liquid and has some advantages of durability of ion generation by a self‐healing surface and quantitative performance. In this study, we found a novel aspect of 3AQ/CHCA as a MALDI matrix, which converges hydrophilic material into the center of the droplet of analyte‐3AQ/CHCA mixture on a MALDI sample target well during the process of evaporation of water derived from analyte solvent. This feature made it possible to separate not only the buffer components, but also the peptides and oligosaccharides from one another within 3AQ/CHCA. The MALDI imaging analyses of the analyte‐3AQ/CHCA droplet indicated that the oligosaccharides and the peptides were distributed in the center and in the whole area around the center of 3AQ/CHCA, respectively. This 'on‐target separation' effect was also applicable to glycoprotein digests such as ribonuclease B. These features of 3AQ/CHCA liquid matrix eliminate the requirement for pretreatment, and reduce sample handling losses thus resulting in the improvement of throughput and sensitivity. Copyright © 2012 John Wiley & Sons, Ltd.     

Evidence of Molecular Fragmentation inside the Charged Droplets Produced by Electrospray Process

The behavior of the analyte molecules inside the neutral core of the charged droplet produced by the electrospray (ES) process is not unambiguously known to date. We have identified interesting molecular transformations of two suitably chosen analytes inside the ES droplets. The highly stable Ni(II) complex of 1,8-dimethyl-1,3,6,8,10,13-hexaazacyclotetradecane (1) that consists of a positive charge at the metal center, and the allyl pendant armed tertiary amine containing macrocycle 3,4,5:12,13,14-dipyridine-2,6,11,15-tetramethyl-1,7,10,16-tetraallyl-1,4,7,10,13,16-hexaazacyclooctadeca-3,13-diene (M _4p ) have been studied by ESI mass spectrometry as the model analytes. We have shown that these two molecules are not representatively transferred from solution to gas phase by ESI; rather, they undergo fragmentation inside the charged droplets. The results indicated that a charged analyte such as 1 was possibly unstable inside the neutral core of the ES droplet and undergoes fragmentation due to the Coulombic repulsion imparted by the surface protons. Brownian motion of the neutral analyte such as M _4p inside the droplet, on the other hand, may lead to proton attachment on interaction with the charged surface causing destabilization that leads to fragmentation of M _4p and release of resonance stabilized allyl cations from the core of the droplet. Detailed solvent dependence and collision-induced dissociation (CID) studies provided compelling evidences that the fragmentation of the analytes indeed occurs inside the charged ES droplets. A viable model of molecular transformations inside the ES droplet was proposed based on these results to rationalize the behavior of the analyte molecules inside the charged ES droplets.     

Investigation of the profiling depth in matrix-assisted laser desorption/ionization imaging mass spectrometry

Matrix-assisted laser desorption/ionization (MALDI) imaging mass spectrometry is generally considered to be a surface analysis technique. In this report, the profiling depth of imaging mass spectrometry was examined. MALDI matrix solution was found to be able to gain access to the tissue interior and extract analyte molecules to the tissue surface. As a consequence, prazosin, a small molecule pharmaceutical compound, located as deep as 40 microm away from the surface was readily detected after matrix application. Likewise, cytochrome c, a 12 kDa protein, was also detectable from the tissue interior. Moreover, for prazosin, not only the extent of matrix effect, but also the extraction efficiency of the matrix solvent appeared to be dependent on the type of tissue. These results indicated that experimental conditions that decrease the matrix solvent evaporation during matrix application may increase analyte extraction efficiency and hence sensitivity of the analysis. Furthermore, thin sections should be used to avoid differential extraction efficiency of matrix solvent in different tissues for whole-body analysis.     

Sequence determination of αs1‐casein isoforms from donkey by mass spectrometric methods

Four co‐eluting components, with experimentally measured M_r of 23 658, 23 786, 24 278 and 24 406 Da, were detected by reversed‐phase high‐performance liquid chromatography (RP‐HPLC) and matrix‐assisted laser desorption/ionization time‐of‐flight mass spectrometry (MALDI‐TOF MS) analysis in the dephosphorylated casein fraction of a milk sample collected at middle lactation stage from an individual donkey belonging to the Ragusano breed. By coupling RP‐HPLC, two‐dimensional polyacrylamide gel electrophoresis (2D‐PAGE), enzymatic digestions, MALDI‐TOF MS and capillary RP‐HPLC/nano‐electrospray ionization tandem mass spectrometry (nESI‐MS/MS) analyses, the four components were identified as donkey's α_s1‐CNs and their sequences completely characterized, using the known mare's α_s1‐CN (GenBank Acc. No. AAK83668; M_r 23750.7 Da) as reference. The proteins with M_r of 23 786 and 23 658 Da differ in the presence of a glutamine residue at position 83 in the full‐length component and present the amino acid substitutions Q⁸→H and H¹¹⁵→Y with respect to the mare's α_s1‐CN. The other two components with M_r 24 406 and 24 278 Da, which also differ in the presence of a glutamine residue at position 88 in the full‐length component, show the insertion of the pentapeptide HTPRE between Leu³³ and the Glu³⁴. The two α_s1‐CNs bearing the pentapeptide insertion were named variants A (202 amino acids; M_r 24 406) and A₁ (201 amino acids; M_r 24 278), whereas the two α_s1‐CNs without the pentapeptide were named variants B (197 amino acids; M_r 23 786) and B₁ (196 amino acids; M_r 23 658). Copyright © 2009 John Wiley & Sons, Ltd.     

Ultrasonic energy as a tool in the sample treatment for polymer characterization through matrix-assisted laser desorption ionization time-of-flight mass spectrometry

Different ultrasonic devices including ultrasonic bath with dual frequency, sonoreactor and ultrasonic probe, were tested for their viability in the sample treatment for polymer characterization by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry analysis. The effect of sonication frequency (35 kHz, 40 kHz and 130 kHz), sonication amplitude, and sonication time on the polymer's number-average molecular weight (M_n) and weight-average molecular weight (M_w) were investigated. The effect of those variables in the molecular mass distribution of three polymer standards, poly(styrene) 2000 Da and 10,000 Da and poly(ethylene glycol) 1000 Da, was evaluated. In addition, the influence of ultrasonic energy on the sample treatment as a function of the matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI) matrix was also studied through two common standard matrices, dithranol and 2,5-dihydroxybenzoic acid. The results obtained show that the ultrasonic bath at 35 kHz is the best option for the purpose of fast sample treatment for polymer characterization. The M_n and M_w values obtained for this ultrasonic device and for the three polymers tested using dithranol as MALDI matrix, were not statistically different from the ones acquired with vortex mixing and also were in concordance with the values recommended by the polymer manufacturers.     

Rapid analysis of aflatoxin M1 in milk using dispersive liquid–liquid microextraction coupled with ultrahigh pressure liquid chromatography tandem mass spectrometry

A simple, rapid, and sensitive method based on simultaneous protein precipitation and extraction of aflatoxin M₁ (AFM₁) followed by dispersive liquid–liquid microextraction (DLLME) and ultrahigh pressure liquid chromatography tandem mass spectrometry (UHPLC-MS/MS) analysis was developed for the determination of AFM₁ in milk samples. In order to precipitate the proteins and extract AFM₁ from milk, a sample pretreatment using acetonitrile and NaCl as the extraction/denaturant solvent and salting-out agent, respectively, was optimised. Subsequently, the acetonitrile (upper) phase, containing AFM₁, was used as the disperser solvent in DLLME, and extractant (chloroform) and water were added in turn to the extract to perform the DLLME process. The main parameters affecting the extraction efficiency of the whole analytical procedure, such as acetonitrile volume, amount of salt, type and volume of extractant and water volume, were carefully optimised by experimental design. Under optimum conditions, the developed method provides an enrichment factor of 33 and detection and quantification limits (0.6 and 2.0 ng kg^?1, respectively) below the maximum levels imposed by current regulations for AFM₁ in milk and infant milk formulae. Recoveries (61.3–75.3 %) and repeatability (RSD?<?10, n?=?3), tested in different types of milk at four AFM₁ levels, met the performance criteria required by EC Regulation No. 401/2006. Moreover, the matrix effect on the signal intensity of the analyte was negligible. The proposed method provides a rapid extraction and an accurate determination of AFM₁ in milk and formula milk using a simple and inexpensive sample preparation procedure.

A simple microextraction and preconcentration approach based on a mixed matrix membrane

A simple adsorption/desorption procedure using a mixed matrix membrane (MMM) as extraction medium is demonstrated as a new miniaturized sample pretreatment and preconcentration technique. Reversed-phase particles namely polymeric bonded octadecyl (C₁₈) was incorporated through dispersion in a cellulose triacetate (CTA) polymer matrix to form a C₁₈-MMM. Non-steroidal anti-inflammatory drugs (NSAIDs) namely diclofenac, mefenamic acid and ibuprofen present in the environmental water samples were selected as targeted model analytes. The extraction setup is simple by dipping a small piece of C₁₈-MMM (7 mm × 7 mm) in a stirred 10 mL sample solution for analyte adsorption process. The entrapped analyte within the membrane was then desorbed into 100 μL of methanol by ultrasonication prior to high performance liquid chromatography (HPLC) analysis. Each membrane was discarded after single use to avoid any analyte carry-over effect. Several important parameters, such as effect of sample pH, salting-out effect, sample volume, extraction time, desorption solvent and desorption time were comprehensively optimized. The C₁₈-MMM demonstrated high affinity for NSAIDs spiked in tap and river water with relative recoveries ranging from 92 to 100% and good reproducibility with relative standard deviations between 1.1 and 5.5% (n = 9). The overall results obtained were found comparable against conventional solid phase extraction (SPE) using cartridge packed with identical C₁₈ adsorbent.     

In situ implantation of PolyPOSS blocks in Nafion matrix to promote its performance in direct methanol fuel cell

Fabrication of recast Nafion^®-117 membrane using the dipolar aprotonic solvent will normally lead to a random matrix. On the contrary, when a designed amount of vinyl-pendant octasiloxane (Q₈M₈^V) cubic molecules was included into the Nafion^® matrix during the recasting process and then subjected to polymerization, a nonrandom matrix was obtained. This paper provides an insight into the matrix-formatting role of rigid poly(Q₈M₈^V) blocks, generated in situ in Nafion^® matrix, according to thermal analyses (thermogravimetric analysis (TGA), dynamic mechanical analysis (DMA) and Differential Scanning Calorimetry (DSC)) and electron microscopic images of the resulting composite matrix. The P(Q₈M₈^V) played a role in restricting random extensions of proton-conducting channels (PCCs) and promoted ordered assembling of Nafion^® molecules. As a result, compared with the recast pristine Nafion^® membrane, the composite membranes containing P(Q₈M₈^V) of 5–15 wt.% manifested obvious improvement on both repression of methanol permeability and promotion of power density output of the single direct methanol fuel cell (DMFC).     

On the inner and outer radial density functions

Starting from the two-electron radial density D ₂(r ₁,r ₂), a generalized partitioning of the one-electron radial density function D(r) into two component densities D _a (r) and D _b (r) is discussed for many-electron systems. The literature partitioning (Koga and Matsuyama Theor Chem Acc 115:59, 2006) of D(r) into the inner D _<(r) and outer D _>(r) radial densities is shown to minimize the average variance of the two component density functions D _a (r) and D _b (r). It is also found that the average radial separation halved, , constitutes a lower bound to the standard deviation σ of D(r).     

Inner and outer radial density functions in many-electron atoms

When any two electrons are considered simultaneously, the radial density function D(r) in many-electron atoms is shown to be rigorously separated into inner D _<(r) and outer D _>(r) radial densities. Accordingly, radial properties such as the electron–nucleus attraction energy V _en and the diamagnetic susceptibility χ _d are the sum of the inner and outer contributions. The electron–electron repulsion energy V _ee has an approximate relation with the minus first moment of the outer density D _>(r). For the 102 atoms He through Lr in their ground states, different characteristics of local maxima in the radial densities D _<(r), D _>(r), and D(r) are reported based on the numerical Hartree-Fock wave functions. Relative contributions of the inner and outer components to V _en and are also discussed for these atoms.     

Solvent‐ and counterion‐specific swelling behavior of poly(acrylic acid) gels

The collapse of alkali metal poly(acrylate) (PAAM) gels was investigated for various water/organic solvent mixture systems: methanol (MeOH), ethanol (EtOH), 2‐propanol (2PrOH), t‐butanol (tBuOH), dimethyl sulfoxide (DMSO), acetonitrile (AcN), acetone, tetrahydrofuran (THF), and dioxane. In order to ascertain the counterion specificity in the swelling behavior, four kinds of alkali metal counterions were used: Li⁺, Na⁺, K⁺, and Cs⁺. Remarkable solvent and counterion specificities were observed for every counterion species and every solvent system, respectively. For example, in aqueous EtOH the dielectric constants (D_cr) at which collapse occurred were in the order PAACs < PAALi < PAAK < PAANa. On the other hand, the D_cr at which PAALi gel collapsed increased in the order tBuOH < dioxane < THF < MeOH < 2PrOH < EtOH < acetone < AcN < DMSO, where the D_cr ranged from about 39 to about 67. This was in contrast to our previous observation for a partially quaternized poly(4‐vinyl pyridine) (P4VP) gel, which collapsed in a much narrower D_cr region in similar mixed solvents. The present solvent‐ and counterion‐specific collapses are discussed on the basis of solvent properties such as the dielectric constant and Gutmann's donor number and acceptor number of a pure solvent. © 2000 John Wiley & Sons, Inc. J Polym Sci B: Polym Phys 38: 2791–2800, 2000     

Determination of block size in poly(ethylene oxide)‐b‐polystyrene block copolymers by matrix‐assisted laser desorption/ionization time‐of‐flight mass spectrometry

Characterization of block size in poly(ethylene oxide)‐b‐poly(styrene) (PEO‐b‐PS) block copolymers could be achieved by matrix‐assisted laser desorption/ionization time‐of‐flight mass spectrometry (MALDI‐TOF‐MS) after scission of the macromolecules into their constituent blocks. The performed hydrolytic cleavage was demonstrated to specifically occur on the targeted ester function in the junction group, yielding two homopolymers consisting of the constitutive initial blocks. This approach allows the use of well‐established MALDI protocols for a complete copolymer characterization while circumventing difficulties inherent to amphiphilic macromolecule ionization. Although the labile end‐group in PS homopolymer was modified by the MALDI process, PS block size could be determined from MS data since polymer chains were shown to remain intact during ionization. This methodology has been validated for a PEO‐b‐PS sample series, with two PEO of number average molecular weight (M_n) of 2000 and 5000 g mol^?1 and M_n(PS) ranging from 4000 to 21,000 g mol^?1. Weight average molecular weight (M_w), and thus polydispersity index, could also be reached for each segment and were consistent with values obtained by size exclusion chromatography. This approach is particularly valuable in the case of amphiphilic copolymers for which M_n values as determined by liquid state nuclear magnetic resonance might be affected by micelle formation. © 2009 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 47: 3380–3390, 2009     

Vibrational spectral studies of ion-ion and ion-solvent interactions. II. Zinc nitrate in water/dioxane mixtures

Raman and infrared spectral data have been collected forp-dioxane and solvated and bound nitrate ions for Zn(NO₃)₂/p-dioxane/water systems. It is concluded that Zn²⁺ is preferentially solvated by water and that this aquation is also responsible for a lower concentration of ion pairs than is found for methanol/Zn(NO₃)₂ solutions for which the dielectric constant of the bulk solvent is similar. Values of K₁ (M^–1), the association constant for Zn(NO₃)⁺, are 0.22±0.02 (2/1 solvent,D=12.6) and 0.071±0.01 (4/1 solvent,D=33.0). The log K₁ against 1/D plot is not linear.     

Solid-phase microextraction using octadecyl-bonded silica immobilized on the surface of a rotating disk: Determination of hexachlorobenzene in water

Solid-phase microextraction of hexachlorobenzene from water was implemented for the first time on a rotating disk coated with an octadecyl-bonded silica (C₁₈) sorptive phase. The results indicate that the sorption performance of this phase for the model analyte selected is similar to that observed using a rotating disk containing PDMS. In both cases, equilibrium is achieved within approximately 120 min for samples volumes of 50 mL and decreases to 20–30 min when the sample volume is decreased to 10 mL. The comparable behavior observed for the sorption of HCB in both phases is consistent with a similar rate-determining step for extraction, which suggests that the overall mass transfer of analyte is not limited by internal diffusion into the phase but by diffusion into the aqueous stagnant layer. The main advantage in the use of the C₁₈ phase is that the elution of the analyte was achieved in 15 min compared with 45 min for PDMS because, in the case of C₁₈, dichloromethane can be used as the eluting solvent.     

Clustering of pentacene and functionalized pentacene ions in a matrix-assisted laser desorption/ionization orthogonal TOF mass spectrometer

A high-performance orthogonal time-of flight (TOF) mass spectrometer, in combination with the matrix assisted laser desorption/ionization (MALDI) source operating at elevated pressure (∼1 torr in N₂), was used to perform MALDI-TOF analyses of pentacene and some of its derivatives with and without an added matrix. These molecules are among the most interesting semiconductor materials for organic thin film transistor applications (OTFT). The observation of ion-molecule reactions between “cold” analyte ions and neutral analyte molecules in the gas phase has provided some insight into the mechanism of pentacene cluster formation and its functionalized derivatives. Furthermore, some of the matrices employed to assist the desorption/ionization process of these compounds were observed to influence the outcome via ion-molecule reactions of analyte ions and matrix molecules in the gas phase. The stability and reactivity of the compounds and their clusters in the MALDI plume during gas-phase expansion were evaluated; possible structures of the resulting clusters are discussed. The MALDI-TOF technique was also helpful in distinguishing between two isomeric forms of bis-[(triisopropylsilyl)-ethynyl]-pentacene.