Dereplication of oligostilbenes in dipterocarpaceous plants using LCMS-ESI-Ion trap-database

A method for compound identification based on mass fragmentation patterns was developed to distinguish known oligostilbenes directly in crude plant extracts. Eleven pure oligostilbenes were used as standard compounds, and a pilot database of MS data was established. Seven extracts from Dipterocarpaceous plants; three from Neobalanocarpus heimii, three from Dryobalanops spp. and one from Dipterocarpus semivestitus were used as test materials. Eleven compounds were positively identified in the heartwood extract, nine in the bark, and six in the leaves of Neobalanocarpus heimii, one compound each in Dryobalanops lanceolata, D. rappa and D. aromatica, as well as two in Dipterocarpus semivestitus extract. Identification of all compounds were performed within a short analysis time.     

Four New Stilbene Oligomers in the Root of Gnetum gnemon

Four new stilbene oligomers, gnemonols G, H, I, and J ( 1 – 4 ), were isolated from acetone extract of the root of Gnetum gnemon along with five known stilbenoids, ampelopsin E, cis‐ampelopsin E, gnetins C, D, and E. The structures were elucidated on the basis of spectroscopic evidence.     

High‐performance liquid chromatography separation of unsaturated organic compounds by a monolithic silica column embedded with silver nanoparticles

The optimization of a porous structure to ensure good separation performances is always a significant issue in high‐performance liquid chromatography column design. Recently we reported the homogeneous embedment of Ag nanoparticles in periodic mesoporous silica monolith and the application of such Ag nanoparticles embedded silica monolith for the high‐performance liquid chromatography separation of polyaromatic hydrocarbons. However, the separation performance remains to be improved and the retention mechanism as compared with the Ag ion high‐performance liquid chromatography technique still needs to be clarified. In this research, Ag nanoparticles were introduced into a macro/mesoporous silica monolith with optimized pore parameters for high‐performance liquid chromatography separations. Baseline separation of benzene, naphthalene, anthracene, and pyrene was achieved with the theoretical plate number for analyte naphthalene as 36 000 m^?1. Its separation function was further extended to cis/trans isomers of aromatic compounds where cis/trans stilbenes were chosen as a benchmark. Good separation of cis/trans‐stilbene with separation factor as 7 and theoretical plate number as 76 000 m^?1 for cis‐stilbene was obtained. The trans isomer, however, is retained more strongly, which contradicts the long‐ established retention rule of Ag ion chromatography. Such behavior of Ag nanoparticles embedded in a silica column can be attributed to the differences in the molecular geometric configuration of cis/trans stilbenes.     

Preparative separation of isoquinoline alkaloids from Corydalis impatiens using a middle‐pressure chromatogram isolated gel column coupled with two‐dimensional liquid chromatography

We established a two‐dimensional strong cation exchange/reversed‐phase liquid chromatography protocol to isolate and purify isoquinoline alkaloids from Corydalis impatiens. Isoquinoline alkaloids were first enriched from a C. impatiens extract in which liposoluble components were removed using a medium‐pressure chromatographic tower containing middle chromatogram isolated gel. A strong cation exchange column was employed to separate and obtain 30 fractions. We chose fractions 22–29 for reversed‐phase liquid chromatography purification using characteristic isoquinoline alkaloid ultraviolet absorption spectra. Several isoquinoline alkaloid fractions (22–29) were further separated, and those of low resolution were isolated via two‐dimensional liquid chromatography in the orthogonal plane. A total of eight novel isoquinoline alkaloids with characteristic ultraviolet spectra were obtained from C. impatiens. We thus demonstrate the benefits of off‐line two‐dimensional strong cation exchange/reversed‐phase liquid chromatography to isolate isoquinoline alkaloids from C. impatiens.     

Monitoring of the synthesis ofcis andtrans ruthenium macrocyclic complexes by reversed-phase high-performance liquid chromatography

Summary The synthesis of the complex [Ru(cyclam)Cl₂]Cl (cyclam=1,4,8,11-tetraazacyclotetradecane) has been monitored by reversed-phase high-performance liquid chromatography. The analytical results obtained during the reaction have shown that it is feasible to identify and isolate the two isomerscis- andtrans- [Ru(cyclam)-Cl₂]Cl. The use of an octadecylsiloxy preparative column enabled the separation and purification of these two isomers and the compounds have been obtained in high purity. The use of reversed-phase high-performance liquid chromatography has afforded complete analytical control of the syntheses of saturated nitrogendonor macrocyclic complexes of ruthenium, enabling identification of thecis andtrans isomers of the complex [Ru(cyclam)Cl₂]Cl.     

Monitoring of the synthesis ofcis andtrans ruthenium macrocyclic complexes by reversed-phase high-performance liquid chromatography

Summary The synthesis of the complex [Ru(cyclam)Cl₂]Cl (cyclam=1,4,8,11-tetraazacyclotetradecane) has been monitored by reversed-phase high-performance liquid chromatography. The analytical results obtained during the reaction have shown that it is feasible to identify and isolate the two isomerscis- andtrans- [Ru(cyclam)Cl₂]Cl. The use of an octadecylsiloxy preparative column enabled the separation and purification of these two isomers and the compounds have been obtained in high purity. The use of reversed-phase high-performance liquid chromatography has afforded complete analytical control of the syntheses of saturated nitrogendonor macrocyclic complexes of ruthenium, enabling identification of thecis andtrans isomers of the complex [Ru(cyclam)Cl₂]Cl.     

Coleone C,D, I,I′ aus einer madegassischen Plectranthus sp. nov. Interkonversion von cis- und trans-A/B-6,7-Diketoditerpenen

Coleons C, D, I, I′, obtained from a Madagascan Plectranthus sp. nov.. Interconversion of cis- and trans-A/B-6,7-Diketoditerpenes. Fairly large amounts of Coleons C and D, as well as Coleons I and I′ (3-O-formyl derivative of Coleon I) can bc isolated from the orange glands of an unclassified North Madagascan Plectranthus sp. A reversible transformation of cis- and trans-A/B-6,7-dioxo-abietane via its diosphenol has been achieved for the first time. CD.-Spectra of these compounds are presented. Hydrogenolysis of Coleon D leads to 6β,16-dihydroxy-royleanone.     

Preparative isolation of tetra-, penta- and hexapurine oligonucleotides from partial hydrolysates of depyrimidinated herring sperm DNA

Herring sperm DNA is chemically degraded to a complex mixture of purine nucleotides. The oligonucleotides are separated from the partial hydrolysates by column chromatography. The resulting mixture of trimer to hexamer purine oligonucleotides is subsequently fractionated on QAE-Sephadex into different mixtures of sequence-isomeric purine oligonucleotides. In a final separation, which uses reversed-phase (Nucleosil C18) high-performance liquid chromatography, these mixtures are separated under isocratic conditions into 35 pure defined purine oligonucleotides with four to six monomer units, 14 defined mixtures of sequence-isomeric purine oligonucleotides and several unidentified products. Purity and sequence of the isolated oligonucleotides are determined by the "fingerprint" method. The results of the high-performance liquid chromatographic and the "fingerprint" methods of the isolated oligonucleotides are discussed.     

Semiempirical studies of ring twisting in cis‐stilbene and related biomolecules

The geometric and energetic predictions of the MNDO, AM1, and SAM1 models as they describe rotation of the dihedral angle between the plane of one of the phenyl rings and the plane of the olefin core of cis‐stilbene (cis‐1,2‐diphenylethylene) were tested for a variety of constraints. All three models predict that distortions away from the stable structure fixed by a compromise between π‐electron and steric repulsions lead to small (at most 1–2 kcal/mol) strain energies and geometry relaxations. Extensive peripheral substitution on the phenyl rings present in a prototype natural product having the cis‐stilbene structure, Combretastatin A‐4 (3,4,5‐trimethoxy‐3′‐hydroxy‐4′‐methoxy‐(Z)‐stilbene), distorted the shapes of the cis‐stilbene barriers to conformation change only minimally. It is concluded that natural products having the cis‐stilbene structure should be expected to interact with other biomolecules as if the phenyl twists are barrier free. ©1999 John Wiley & Sons, Inc. Int J Quant Chem 71: 57–62, 1999     

Structure of Globularidin: An Unusual Iridoid Glucoside from Globularia alypumL.

A novel iridoid glucoside, named globularidin, lacking the typical double bond between C(3) and C(4), has been isolated from the whole plant of Globularia alypum by the combination of open column- and high-performance liquid chromatography. The structure of this compound was established by chemical transformation and spectral data.     

Determination of stilbene derivatives in Burgundy red wines by ultra-high-pressure liquid chromatography

The polyphenols, for example stilbenes and flavonoids, are an important family of compounds present in grapes and wines. Several studies have shown that stilbenes are antioxidants and cancer-preventing agents. For the first time, eight natural stilbenes (trans-resveratrol, trans-piceid, cis-piceid, trans-astringin, trans-piceatannol, (+)-trans-ε-viniferin, pallidol, and hopeaphenol), isolated and purified from Vitis vinifera, were simultaneously analysed by ultra-high-pressure liquid chromatography coupled with photodiode-array detection. Separation of the stilbenes by UHPLC was optimized with the assistance of “Quality-by-Design” commercial software. Four different reversed-phase columns packed with 1.5–1.7-μm particles were tested and compared for their retention behaviour and separation efficiency. On the basis of the performance characteristics determined, the VisionHT C18 HL column was selected for the stilbenes studied, because resolution of the critical pair was 1.5 with a peak width of 2–4 s. The optimized method resulted in highly repeatable retention times (RSD 0.03–0.07%), peak areas (RSD 3–6%), and linear ranges were between 0.005 and 50 mg L⁻¹ for most of the compounds. All stilbenes, except trans-astringin, trans-piceatannol, and pallidol were identified and quantified in Burgundy red wines at different concentrations after direct injection of the wines.     

Identification of flavonoids in Dendrobium huoshanense and comparison with those in allied species of Dendrobium by TLC,HPLC and HPLC coupled with electrospray ionization multi‐stage tandem MS analyses

Dendrobium huoshanense, a unique species in the genus Orchidaceae, is only found in China and is known as “mihu”. Due to the lack of quality control, the use of D. huoshanense in the herbal market has been limited. In this study, methods based on thin‐layer chromatography, high‐performance liquid chromatography and high‐performance liquid chromatography coupled with electrospray ionization multi‐stage tandem mass spectrometry were used to identify the flavonoids in D. huoshanense and distinguish this species from other Dendrobium species. Using thin‐layer chromatography, a characteristic band was observed for D. huoshanense, and this band was absent from the thin‐layer chromatography plates of other Dendrobium species. Then, using high‐performance liquid chromatography, nine peaks of flavonoids were observed in the chromatograms of ten batches of D. huoshanense. Ultimately, 22 flavonoids in D. huoshanense were identified by multi‐stage tandem mass spectrometry, and 11 of these compounds are being reported from D. huoshanense for the first time. In addition, two compounds both with molecular weights of 710, were identified as being unique to D. huoshanense; one of these compounds, apigenin‐6‐C‐α‐L‐rhamnosyl‐(1→2)‐β‐D‐glucoside‐8‐C‐α‐L‐arabinoside, was proven to be responsible for the characteristic thin‐layer chromatography band of D. huoshanense. These analysis methods can be applied for the identification and quality control of D. Huoshanense.     

Rapid separation of lactucin and lactucopicrin from Cichorium glandulosum by medium-pressure preparative liquid chromatography and quantitative analyses by high-performance thin-layer chromatography

Medium-pressure preparative liquid chromatography (MPPLC) was used to isolate and prepare lactucin and lactucopicrin from the whole herb of Cichorium glandulosum. After extracting the methanolic extract of the whole plant with petroleum ether and ethyl acetate several times to obtain ethyl acetate extract, the crude products, namely, lactucin and lactucopicrin were separated using MPPLC and thin-layer chromatography (TLC) tracking, and their purity rates reached more than 80%. The qualitative and quantitative analyses of lactucin and lactucopicrin were carried out by high-performance thin-layer chromatography (HPTLC) on the whole herb of C. glandulosum. The contents of lactucin and lactucopicrin were determined by scanning at 256 nm in the whole herb of C. glandulosum. The R_F values of lactucin and lactucopicrin were 0.42 ± 0.05 and 0.65 ± 0.05 with linear ranges of 0.498–2.988 and 0.499–2.994 μg/band, respectively. The correlation coefficients were 0.9938 and 0.9946, respectively, thereby showing a good linear relationship. The average recoveries were 99.96% and 99.52%, and the relative standard deviations (RSDs) were 2.49% and 2.45%, respectively. The crude products, namely, lactucin and lactucopicrin, can be isolated with high purity from the whole herbs of C. glandulosum by MPPLC. The lactucin and lactucopicrin contents of C. glandulosum can be determined rapidly and accurately by HPTLC.

     

Quantification of cis-Abienol in Oriental Tobacco Leaves by LC

A rapid and accurate method for the quantification of cis-abienol in oriental tobacco leaves by normal phase liquid chromatography was developed. Freeze-dried tobacco samples were sonicated in methylene chloride for 10 min. The supernatant was purified using a silica gel solid phase extraction cartridge. Ten milliliter of the resulting methylene chloride eluate was collected, then separated on a 250 × 4.6 mm, 5 μm particle-size CN column with n-hexane: ethyl acetate, 100:2 (v/v) at a flow rate of 1 mL min⁻¹. cis-Abienol was detected by UV absorption at 254 nm. The linear range was from 2.14 × 10⁻⁴ to 4.28 × 10⁻² mg mL⁻¹ and the correlation coefficient was 1.000. The average recovery was 98.7, 105.2 and 103.1% in five replicated sets of tobacco samples spiked with 0.2856, 0.7140 and 1.904 mg cis-abienol. The relative standard deviations (RSDs) were 1.04, 0.63 and 1.25%, respectively (n = 5). Limit of detection (S/N = 3) was 21.84 μg g⁻¹ and limit of quantification (S/N = 10) was 72.80 μg g⁻¹. The method was found to be suitable for determination of cis-abienol in oriental tobacco leaves. Furthermore, pure cis-abienol used for method validation was obtained by preparative reversed phase high-performance liquid chromatography. Identification was performed by UV detection, nuclear magnetic resonance and mass spectrometry.     

Purification of CIS-trimedlure isomers by high-performance liquid chromatography

Summary High-performance liquid chromatographic procedures were developed to make it possible to obtain the fourcis-trimedlure isomers (V, W, X, and Y) in pure form. Trimedlure-V and-Y were each readilt separated from the four-componentcis-trimedlure mixture through high-performance liquid chromatographic analysis on 5-μm and 3-μm silica, but trimedlure-W and-X were not adequately resolved. Chromatography of 5-μm silica of the mixtures obtained by epimerization of thetrans-trimedlure isomers, C and B₂, yielded the respective epimers, trimedlure-W and-X, in pure form.     

Cis/trans ISOMERIZATION OF CAROTENOIDS BY THE TRIPLET CARBONYL SOURCE 3-HYDROXYMETHYL-3,4,4-TRIMETHYL-1,2-DIOXETANE*

Abstract— The interaction of biological carotenoids with 3-hydroxymethyl-3,4,4-trimethyl-1,2-dioxetane (HTMD), a thermodissociable source of electronically excited ketones, was investigated using reversed-phase high-performance liquid chromatography. Incubation of the all-trans isomers of β-carotene, lycopene and canthaxanthin with HTMD led to significant trans-to-cis isomerization, with cis isomers accounting for 20–50% of products formed (the balance assigned as oxidation products). The isomers forming from all-trans-β-carotene were identified as 9-cis-, 13-cis- and 15-cis-β-carotene by cochromatography of cis isomer standards and by on-line diode array absorbance spectroscopy. An HTMD-dependent cis-to-trans isomerization was observed in incubations started with 15-cis-β-carotene, and it occurred more rapidly and to a greater extent than the isomerization of all-trans-β-carotene. The isomer patterns generated from lycopene and β-carotene are generally similar to those reported recently for various human tissues (Stahl et al, 1992, Arch. Biochem. Biophys. 294 , 173–177).     

Biotransformation of some monoterpenoid ketones by <Emphasis Type="Italic">Chlorella vulgaris</Emphasis> MCCS 012

Biotransformation of several monoterpene ketones, including carvone, pulegone, piperitone, menthone, and fenchone, was carried out by the locally isolated unicellular microalgae Chlorella vulgaris. The microalgal strain was isolated during a screening program from soil samples collected from paddy-fields of Fars Province, in the south of Iran. Chlorella vulgaris was cultured in 250 mL conical flasks, each containing 50 mL of BG-11 liquid medium and 20 μL levels of terpene substrates, incubated at a temperature of 28±2°C and illuminated continuously with fluorescent lamps with shaking at 80 rpm. The metabolites were identified by thin-layer chromatography and GC-MS. Chlorella vulgaris has the ability to reduce the C=C double bond of carvone to yield trans-dihydrocarvone and cis-dihydrocarvone. The cell line reduced menthone and pulegone to the same product and gave menthol. Study of Chlorella vulgaris with substrates of piperitone and fenchone showed no reaction in these substrates. Chlorella vulgaris MCCS 012 was assigned according to the 18S rRNA gene sequence. The DNA sequence of the 18S rRNA gene of Chlorella vulgaris MCCS 012 was recorded in the NCBI under the accession number EU374170.     

Preparative isolation and purification of 12 main antioxidants from the roots of Polygonum multiflorum Thunb. using high‐speed countercurrent chromatography and preparative HPLC guided by 1,1′‐diphenyl‐2‐picrylhydrazyl‐HPLC

A hyphenated strategy by off‐line coupling of 1,1′‐diphenyl‐2‐picrylhydrazyl‐high‐performance liquid chromatography, high‐speed countercurrent chromatography, and preparative high‐performance liquid chromatography was established to screen and separate antioxidants from ethyl acetate fraction of the roots of Polygonum multiflorum. Under the targeted guidance of 1,1′‐diphenyl‐2‐picrylhydrazyl‐high‐performance liquid chromatography experiment, 12 compounds were identified as potential antioxidants and readily isolated by high‐speed counter‐current chromatography and preparative high‐performance liquid chromatography. Ultraviolet spectroscopy, mass spectrometry, and ¹H NMR spectroscopy were employed to identify their structures, which were assigned as gallic acid ( 1 , 6.2 mg, 98.28%), catechin ( 2 , 8.8 mg, 90.69%), epicatechin ( 3 , 4.1 mg, 96.71%), polydatin ( 4 , 5.3 mg, 94.91%), 2,3,5,4′‐tetrahydroxy stilbene‐2‐Ο‐β‐D‐glucoside ( 5 , 20.2 mg, 95.23%), piceatannol ( 6 , 5.3 mg, 96.85%), rutin ( 7 , 5.4 mg, 97.92%), resveratrol ( 8 , 5.2 mg, 96.94%), isorhapontigenin ( 9 , 11.4 mg, 94.81%), hyperoside ( 10 , 9.7 mg, 98.52%), rhein ( 11 , 4.9 mg, 97.46%), and emodin ( 12 , 8.2 mg, 95.74%). Notably, compounds 6 and 9 were isolated from Polygonum multiflorum for the first time. In addition, antioxidant activity of compounds 1–12 were evaluated, and compounds 1–8 and 10 exhibited stronger antioxidant activity than ascorbic acid (positive control). These results indicated that the proposed method is a highly efficient strategy to screen and isolate antioxidants from complex natural products.     

Catalysis in competing isocyanate reactions. II. Competing phenyl isocyanate reactions catalyzed with N,N′,N″-pentamethyldipropylenetriamine

The kinetics of the N,N′,N″-pentamethyl dipropylene triamine (PMPT)-catalyzed reaction of phenyl isocyanate with n-butanol was studied in acetonitrile between 26.5 and 50°C by measuring the NCO disappearance as well as the formation of the various reaction products by means of the standard dibutylamine back-titration method and the high-performance liquid chromatography (HPLC) method. The resulting products from the phenyl isocyanate and n-butanol reaction were found to be N-butyl phenylcarbamate, N-butyl-α,γ-diphenylallophanate, and triphenylisocyanurate. Trimer formed at the expense of carbamate formation even at a high OH/NCO ratio. Allophanate appeared to be an intermediate in the formation of trimer. PMPT was found to be a urethane and trimerization catalyst for the model reaction of phenyl isocyanate with n-butanol in acetonitrile. The PMPT-catalyzed reaction of phenyl isocyanate with n-butanol in the presence of water in acetonitrile at 50°C was also investigated. The resulting reaction products consisted of n-butyl phenylcarbamate, n-butyl-β,γ-diphenylallophanate, triphenylisocyanurate, sym-triphenylbiuret, and N,N′-diphenylurea. The presence of water retarded the disappearance of NCO groups as well as the trimer formation. Aniline (the product of phenyl isocyanate and water) was detected in the reaction of equivalent amounts of phenyl isocyanate and water in acetonitrile.     

Synthesis,characterization, and ring opening polymerization of poly(1,4‐cyclohexylenedimethylene terephthalate) cyclic oligomers

Cyclic oligomers of poly(1,4‐cyclohexylenedimethylene terephthalate) (PCT) were prepared by reaction of 1,4‐cyclohexanedimethanol (CHDM) with terephthaloyl chloride under diluted conditions and separated from the linear products by silica gel column at a yield of 23.7 wt %. Cyclic dimer, trimer, tetramer, pentamer, and hexamer were further separated by high performance liquid chromatography, and found to constitute 98% of the cyclics mixtures. The structures of PCT cyclics were confirmed by means of mass spectrometry, Fourier transform infrared, and ¹H NMR analysis. A series of experiments were carried out to study the effects of catalysts and cis/trans configuration of isomers of CHDM on the yield of cyclic oligomers. Ring opening polymerization of the cyclic oligomers was carried out by heating the sample mixtures at 310 °C for 30 min in the presence of antimony oxide. Polymerization was confirmed by inherent viscosity changes and infrared spectra of the resulting polyesters. © 2000 John Wiley & Sons, Inc. J Polym Sci A: Polym Chem 38: 1828–1833, 2000