High‐performance liquid chromatographic analysis: applications to nutraceutical content and urinary disposition of oxyresveratrol in rats

A high‐performance liquid chromatographic (HPLC) method was developed for the analysis of the stilbene, oxyresveratrol. This method involves the use of a Luna® C₁₈ column with ultraviolet detection at 320 nm. The mobile phase consisted of acetonitrile, water and formic acid (30 : 70 : 0.04 v/v) with a flow rate of 0.6 mL/min. The calibration curves were linear over the range of 0.5–100.0 μg/mL. The mean extraction efficiency was between 98.9 and 109%. The precision of the assay was 0.069–18.4% (RSD%), and within 20% at the limit of quantitation (0.5 μg/mL). The bias of the assay was <15% and within 15% at the limit of quantitation. This assay was successfully applied to pre‐clinical pharmacokinetic samples from rat urine and to nutraceutical product analysis. Copyright © 2009 John Wiley & Sons, Ltd.     

(Salen)CrIIIX catalysts for the copolymerization of carbon dioxide and epoxides: role of the initiator and cocatalyst

The copolymerization of CO(2) and cyclohexene or propylene oxide has been examined employing (salen)Cr(III)Nu complexes (Nu = Cl or N(3)) as catalysts. The addition of various cocatalysts, including phosphines and PPN+ or Bu4N+ Cl- salts serves to greatly enhance the rate of copolymer production. In these instances, the mechanism of the initiation step appears to be unimolecular in catalyst concentration, unlike the bimolecular process cocatalyzed by N-methylimidazole. The copolymers were produced with >95% carbonate linkages with TOFs in the range 39-494 mol epoxide consumed/mol Cr.h. In the presence of phosphine cocatalysts, no cyclic carbonate was produced as a byproduct.     

Alkali metal ion binding to amino acids versus their methyl esters: affinity trends and structural changes in the gas phase

The relative alkali metal ion (M(+)) affinities (binding energies) between seventeen different amino acids (AA) and the corresponding methyl esters (AAOMe) were determined in the gas phase by the kinetic method based on the dissociation of AA-M(+)-AAOMe heterodimers (M=Li, Na, K, Cs). With the exception of proline, the Li(+), Na(+), and K(+) affinities of the other aliphatic amino acids increase in the order AAAAOMe is already observed for K(+). Proline binds more strongly than its methyl ester to all M(+) except Li(+). Ab initio calculations on the M(+) complexes of alanine, beta-aminoisobutyric acid, proline, glycine methyl ester, alanine methyl ester, and proline methyl ester show that their energetically most favorable complexes result from charge solvation, except for proline which forms salt bridges. The most stable mode of charge solvation depends on the ligand (AA or AAOMe) and, for AA, it gradually changes with metal ion size. Esters chelate all M(+) ions through the amine and carbonyl groups. Amino acids coordinate Li(+) and Na(+) ions through the amine and carbonyl groups as well, but K(+) and Cs(+) ions are coordinated by the O atoms of the carboxyl group. Upon consideration of these differences in favored binding geometries, the theoretically derived relative M(+) affinities between aliphatic AA and AAOMe are in good overall agreement with the above given experimental trends. The majority of side chain functionalized amino acids studied show experimentally the affinity order AAAAOMe. The latter ranking is attributed to salt bridge formation.     

Lysosomal cholesterol accumulation inhibits subsequent hydrolysis of lipoprotein cholesteryl ester.

Human macrophages incubated for prolonged periods with mildly oxidized LDL (oxLDL) or cholesteryl ester-rich lipid dispersions (DISP) accumulate free and esterified cholesterol within large, swollen lysosomes similar to those in foam cells of atherosclerosis. The cholesteryl ester (CE) accumulation is, in part, the result of inhibition of lysosomal hydrolysis due to increased lysosomal pH mediated by excessive lysosomal free cholesterol (FC). To determine if the inhibition of hydrolysis was long lived and further define the extent of the lysosomal defect, we incubated THP-1 macrophages with oxLDL or DISP to produce lysosome sterol engorgement and then chased with acetylated LDL (acLDL). Unlike oxLDL or DISP, CE from acLDL normally is hydrolyzed rapidly. Three days of incubation with oxLDL or DISP produced an excess of CE in lipid-engorged lysosomes, indicative of inhibition. After prolonged oxLDL or DISP pretreatment, subsequent hydrolysis of acLDL CE was inhibited. Coincident with the inhibition, the lipid-engorged lysosomes failed to maintain an acidic pH during both the initial pretreatment and subsequent acLDL incubation. This indicates that the alterations in lysosomes were general, long lived, and affected subsequent lipoprotein metabolism. This same phenomenon, occurring within atherosclerotic foam cells, could significantly affect lesion progression.     

Effect of high-temperature on high-performance liquid chromatography column stability and performance under temperature-programmed conditions

Six commercially available analytical (4.1 or 4.6 mm i.d.) columns were evaluated under temperature-programmed high-temperature liquid chromatography (HTLC) conditions to access their stability and performance at extreme temperatures. Seven components consisting of acidic, basic and neutral compounds were analyzed under temperature-programmed conditions and solvent gradient conditions using three different mobile phase compositions (acidic, basic and neutral). Each column was checked with a two-component test mix at various stages of the evaluation to look for signs of stationary phase collapse. Three zirconia based stationary phases studied exhibited column bleed under temperature-programmed conditions. The other three columns, a polydentate silica column, a polystyrene-divinylbenzene (PS-DVB) polymeric column, and a graphitic carbon column performed well with no evidence of stationary phase degradation. The R.S.D. for the retention times and efficiencies were less than 10% for most conditions, and not more than 15% during the course of the evaluation for each column. The polydentate silica stationary phase was temperature programmed to 100 degrees C, the PS-DVB stationary phase was temperature programmed up to 150 degrees C, and the graphitic carbon column was used with temperature programming up to 200 degrees C. Comparable peak capacities and similar retention behaviors were observed under solvent gradient and temperature-programmed conditions. Temperature programming with dynamic mobile phase preheating can replace solvent gradient analysis without a loss of peak capacity when used with 4.1 or 4.6 mm columns.     

Invariants of Composite Networks Arising as a Tensor Product

We generalize Brylawski’s formula of the Tutte polynomial of a tensor product of matroids to colored connected graphs, matroids, and disconnected graphs. Unlike the non-colored tensor product where all edges have to be replaced by the same graph, our colored generalization of the tensor product operation allows individual edge replacement. The colored Tutte polynomials we compute exists by the results of Bollobás and Riordan. The proof depends on finding the correct generalization of the two components of the pointed Tutte polynomial, first studied by Brylawski and Oxley, and on careful enumeration of the connected components in a tensor product. Our results make the calculation of certain invariants of many composite networks easier, provided that the invariants are obtained from the colored Tutte polynomials via substitution and the composite networks are represented as tensor products of colored graphs. In particular, our method can be used to calculate (with relative ease) the expected number of connected components after an accident hits a composite network in which some major links are identical subnetworks in themselves.      

Reversible electrochemical generation of a rhodium(II) porphyrin: thwarting disproportionation with weakly coordinating anions

We report electrochemical generation of a stable Rh(II) porphyrin (Rh(II)(F(28)TPP)) from a four-coordinate Rh(I) precursor [Rh(I)(F(28)TPP)](-) dissolved in weakly coordinating electrolyte solutions. This work provides the first example of an unambiguously reversible one-electron electrochemical oxidation of a Rh(I)(por), and demonstrates that electrochemical oxidation can be performed under conditions that are compatible with alkane activation. These studies begin to classify those media capable of supporting a stable Rh(II)(por), and those that induce disproportionation.     

Asymptotic Spectral Measures, Quantum Mechanics, and E-Theory

We study the relationship between POV-measures in quantum theory and asymptotic morphisms in the operator algebra E-theory of Connes–Higson. This is done by introducing the theory of “asymptotic” PV-measures and their integral correspondence with positive asymptotic morphisms on locally compact spaces. Examples and applications involving various aspects of quantum physics, including quantum noise models, semiclassical limits, strong deformation quantizations, and pure half-spin particles, are also discussed. Received: 27 December 2000 / Accepted: 8 October 2001     

Stereospecific high‐performance liquid chromatography of taxifolin,applications in pharmacokinetics,and determination in tu fu ling (Rhizoma smilacis glabrae) and apple (Malus × domestica)

A stereospecific method of analysis of racemic taxifolin (+/?3,5,7,3′,4′‐pentahydroxyflavanone) in biological fluids is necessary to study pharmacokinetics and disposition in fruit and herbs. A simple high‐performance liquid chromatographic method was developed for the determination of all four taxifolin enantiomers. Separation was achieved on a Chiralcel® OJ‐RH column with UV detection at 288 nm. The standard curves in serum were linear over a range of 0.5–100.0 µg/mL for each enantiomer. The mean extraction efficiency was >88.0%. Precision of the assay was <15% (CV), and was within 12% at the limit of quantitation (0.5 µg/mL). The bias of the assay was <15%, and was within 6% at the limit of quantitation. The assay was successfully applied to stereospecific disposition of taxifolin enantiomers in rats and to the quantification of taxifolin enantiomers in tu fu ling (Rhizoma smilacis glabrae) and apple (Malus × domestica). Copyright © 2009 John Wiley & Sons, Ltd.