Separation and Determination of Low Abundant Flavonoids in Scutellaria Baicalensis Georgi by Micellar Electrokinetic Capillary Electrophoresis

Abstract

Flavonoids are secondary metabolites in many plants with diverse biological activities. A simple and rapid micellar electrokinetic capillary electrophoresis method was developed for simultaneous determination of three low abundant flavonoids (chrysin, 5,7,4′-trihydroxy-8-methoxyflavone, and skullcapflavone II) in Scutellaria baicalensis Georgi within 12 min. The calibration curves revealed a good linear relationship between the peak areas of analytes and their concentrations (11.38 to 436.67 mg/L). The standard deviations of the migration time of the three flavonoids were determined to be 0.64%, 0.83%, and 1.17%, and peak areas were 6.14%, 7.57%, and 8.33%. Recoveries ranged between 90.37 and 109.4%.     

Chromatographic Tandem Mass Spectrometric Detection of Physostigmine and its Major Metabolites in Rat Urine

Abstract

A rapid, sensitive, and specific liquid chromatographic‐electrospray ionization (ESI) tandem ion trap mass spectrometric method has been developed for identification of physostigmine and its metabolites in rat urine. 300 µg kg^–1 of physostigmine were used as a safe oral gavage dose for studies on its metabolites. 0–24 h urine was purified using a C18 solid‐phase extraction cartridge, and then detected by an on‐line MS detector. Identification and structural elucidation of the metabolites were performed by comparing their MSⁿ spectra with physostigmine. Six metabolites and unchanged physostigmine existed in rat urine. All of the metabolites were reported for the first time.     

Comparison of Solid-Phase Extraction and Liquid-Liquid Extraction Methods for Liquid Chromatographic Determination of Diltiazem and its Metabolites in Plasma

Abstract

A rapid solid-phase extraction method for the determination of diltiazem and its metabolites from plasma was compared to a conventional liquid-liquid extraction procedure we have described previously. Analytical recovery for all compounds was greater than 90 % for solid-phase extraction whereas for liquid-liquid extraction, mean recovery ranged from 67 to 82 %. The increase of extraction efficiency was closely related to an improvement of the detection limit for the metabolites. Solid phase extraction procedure was found to be more convenient, rapid and sensitive than liquid-liquid extraction and represents a useful analytical tool for the monitoring of diltiazem and its metabolites in clinical investigations.     

Analysis of Fenitrothion and Metabolites in Stored Wheat

Abstract

A simple and rapid method for the analysis of fenitrothion and its metabolites, fenitrooxon, S-methyl fenitrothion, demethyl fenitrothion, demethyl S-methyl fenitrothion, 3-methyl-4-nitrophenol, and dimethyl phosphorothioic acid in stored wheat has been developed. Simultaneous analysis of the extract was conducted using FPD-GLC after derivatization with diazoethane except for 3-methyl-4-nitrophenol which was analyzed directly by EC-GLC. Recoveries of all compounds from wheat fortified at the levels from 0.1 to 5.0 ppm were greater than 90%.

The developed method was used to quantitatively determine major metabolites found in grain treated with fenitrothion and stored at 20°C for 12 months. Demethyl fenitrothion, 3-methyl-4-nitrophenol, and dimethyl phosphorothioic acid were the major breakdown products of fenitrothion found in stored wheat. Confirmation of these metabolites was carried out by chemical derivatization plus FPD-GLC and by TLC.     

High-Performance Liquid Chromatographic Assay for Chlorquine and its Two Major Metabolites,Desethylchloroquine and Bidesethylchloroquine in Biological Fluids

Abstract

A high-performance liquid chromatography (HPLC) method for the determination of chloroquine and its two major metabolites in biological fluids is described. Hydroxychloroquine is used as an internal standard (I.S.). Drug, metabolites and I.S. were extracted as bases with diethyl ether by a single step procedure. After drying and evaporation of the organic phase, the residue was dissolved into the mobile phase and injected into the chromatographic system. Separation was performed using a normal phase column (Inertsil sill with mixture of acetonitrile, methanol and ammonia as mobile phase. The detection was carried out by fluorescence measurement : excitation wavelength was set at 325 nm and emission at 380 nm. The limit of detection was near 3.7 ng ml^?1 for chloroquine and metabolites. No chromatographic interference could be detected by endogenous compounds or other antimalarial drugs. Because of the good accuracy of the method, concentrations were determinated with a relative standard deviation lower than 7% at the 25 ng ml^?l level for all substances.

An excellent precision was obtained over the range of concentrations tested, 25–1000ng ml^?l. This method can be applied to therapeutic, pharmacokinetic and epidemial studies.     

Determination of Diethylstilbestrol by Time-resolve Fluoroimmunoassay

Abstract

A time-resolved fluoroimmunoassay (TRFIA) was developed for the determination of diethylstilbestrol (DES). The method was based on a competitive immunoassay using europium-labeled anti-DES antibody and DES-bovine serum albumin (DES-BSA) as coated antigen. The TRFIA exhibited a typical response for DES at concentrations of 0.001–100 ng · mL^?1, the linear correlation coefficient is 0.9933, and the detection limit (LOD) is 0.595 pg · mL^?1. Some serum and water samples have been analyzed by using this method with satisfactory results. Compared with the routine fluorescence immunoassay (FIA), this method was more sensitive. The TRFIA may offer a valuable alternative method for the DES detection and could be applied to routine analysis.     

Metabolite profiling of Huaiyang Medicago polymorpha with different mowing crops

Abstract

The main purpose of our study was to identify and compare secondary metabolites due to different mowing in order to make better use of Huaiyang Medicago polymorpha. The metabolite profiling of Huaiyang Medicago polymorpha with two mowing crops was performed using a rapid resolution liquid chromatography system with quadrupole time-of-flight mass spectrometer (RRLC-QTOFMS) followed by multivariate statistical analyses. Principal Component Analysis (PCA) results showed a clear distinction between two mowing crops. The major metabolites that contributed to mowing discrimination were identified. The results also showed that the content of major active compounds in Medicago polymorpha from the second crop are higher significantly than the first crop. This study suggests that the strategy is a reliable and simple method for the rapid discrimination of subtle variations due to different mowing crops.     

HPLC Separation of Theophylline,Paraxanthine, Theobromine,Caffeine and Other Caffeine Metabolites in Biological Fluids

Abstract

An HPLC method is described for rapid analysis of caffeine and seven of its metabolites in plasma, urine, milk and saliva in a single operation using a 5 μ C₁₈ reverse phase column. The metabolites are extracted with chloroform - iso-propanol (85:15) from 100 μL samples added to NH₄HCO₃. No interference from normal blood, urine, milk or saliva constituents was observed. The method is accurate and precise and separates 1,7-dimethylxanthine (paraxanthine) from 1,3-dimethylxanthine (theophylline). Sensitivity for most metabolites is in the range of 0.1 to 0.3 μg/mL and the detectability is at the nanogram level.     

A Low-Resolution Separation of C14 -Glyburide and Its Metabolites from Plasma Extracts Using a High-Performance Liquid Chromatograph Guard Column

Abstract

A low-resolution method for simultaneous, rapid determination of radiolabeled glyburide and its metabolites in human plasma is described. Plasma samples were extracted with ethyl acetate. Extracts were redissolved in 300 μl of mobile phase, and injected into a 3 cm guard column, which was incorporated as a loop in a six-port switching valve. C¹⁴-glyburide was collected as a single 4-min fraction at a flow rate of 4 ml per min.

Following collection of a 1-ml fraction, the column was backflushed with methanol to allow collection of the metabolites of glyburide. The mean value of recovered radioactivity was 95.5 ± 5.7%. The validity of the separation was verified in a high-resolution HPLC system and no cross contamination of the fractions was observed.     

Simultaneous Determination of Diazepam,Oxazepam and Temazepam in Spiked Urine By Hplc

ABSTRACT|Oxazepam and temazepam are two minor metabolites of diazepam. These three benzodiazepines may be found in presence of each other in biological fluids.

Therefore, in this study an HPLC method was developed to separate and analyze them. Benzodiazepines have ability to form inclusion complexes with p-cyclodextrin (β-CyD). According to the degree of binding constant with β-CyD, these compounds can be separated by β-CyD bound to silica (cyclobond column) as the stationary phase using HPLC.

The development and validation of the HPLC procedure for the separation and determination of these compounds in mixtures were studied. The mobile-phase system consisted of phosphate buffer (pH 7): methanol [75:25], with flow rate 0.8 ml min^?1 and UV detection at 240 nm was used.

The calibration graphs were rectilinear from 0.1-2.5 μg/ml and coefficients of variation were <2% for the three compounds in bulk forms.

The method was used to analyse these bezodiazepines in spiked urine containing all three compounds in combination. Recoveries were 97-99.8%

The limit of detection and limit of quantitation were 0.05 μg/ml and 0.1 μg/ml, respectively.

The described method is selective, rapid, simple, reproducible and accurate.     

Desferrioxamine dehydrogenates bilirubin in two stages,leading to a 1:1 red‐coloured adduct. Characterization of the products by high‐performance liquid chromatography/electrospray ionization mass spectrometry

We have used open‐chain tetrapyrroles, such as bilirubin, as molecular probes to investigate the pro‐oxidant activity of desferrioxamine (DES) and its modulation by Trolox. On exposure to Fe‐EDTA/H₂O₂, bilirubin and mesobilirubin underwent bleaching. When DES was present, bleaching was prevented and both rubins were converted into green‐coloured derivatives and then into red pigments. Trolox added with DES inhibited the colour changes induced by DES. The oxidative products were resolved from their parent compounds by high‐performance liquid chromatography (HPLC) and studied by electrospray ionization mass spectrometry and by UV/visible spectroscopy. The green products were identified as biliverdin or mesobiliverdin; the red pigments as the 1:1 molar adduct of DES with biliverdin or mesobiliverdin, less two hydrogens in both cases. It is concluded that DES exercises its oxidative activity through nitroxyl oxidizing radicals capable of efficient hydrogen abstraction, dehydrogenating either rubin to the corresponding verdin. A diradical derivative of DES (bearing two nitroxyl radicals in the same molecule) may be involved in the oxidation of verdins to red pigments, through concerted dehydrogenation and adduct formation. These results shed further light on the redox properties of bilirubin, DES and Trolox, and their interactions. They provide further evidence of the pro‐oxidant activity of DES and suggest a more general biological significance, as rapid removal of bilirubin by bleaching or dehydrogenation may have pharmacological/toxicological implications in severe jaundice. Copyright © 2008 John Wiley & Sons, Ltd.     

Thin-Layer Chromatographic Separation of 14C-Labeled Metabolites from Photosynthate

Abstract

A method for separating ¹⁴C-labeled metabolites (including key intermediates of the glycolate pathway) from plant extracts by thin-layer chromatography is reported. The method provides for rapid and convenient determination of the ¹⁴C-content of metabolites in leaf samples obtained during kinetic investigations of photosynthesis with ¹⁴CO₂.     

Rapid Determination of Methotrexate and 7-Hydroxymethotrexate in Serum and Cerebrospinal Fluid by Radial Compression Liquid Chromatography

Abstract

A rapid, specific and sensitive radial compression reverse phase liquid chromatographic method for the analysis of methotrexate and 7-hydroxymethotrexate in serum and cerebrospinal fluid is reported. A mobile phase consisting of acetonitrile-methanol-pH 3 phosphate (8:15:77) at 6 ml/min flow rate was employed. The U.V. detector was set at 317 nm, and folic acid was used as an internal standard. A rapid extraction of methotrexate and 7-hydroxymethotrexate was performed using Sep-Pak cartridges with high extraction efficiency for both compounds. Patients serum and cerebrospinal fluid samples were analyzed by the described method and the concentrations of methotrexate were compared to those obtained by an enzyme immunoassay. No interference from other metabolites or anticancer drugs in the described assay was observed.     

Solid-Phase Extraction of Carbamazepine and Two Major Metabolites from Plasma for Analysis by HPLC

Abstract

A rapid, sensitive and simple to operate HPLC method for the simultaneous determination of carbamazepine, carbamazepine 10,11-epoxide and 10,11-dihydro-10,11-trans-dihydroxycarbamazepine in plasma is described. The drug and its metabolites are extracted from plasma using commercially available reversed-phase octadecylsilane bonded-silica columns (Bond Elut C₁₈, 2.8 ml capacity). Separation was achieved by reversed-phase chromatography, using a mobile phase consisting of acetonitrile - methanol - water (19:37:44) at a flow-rate of 1.8 ml/min in conjunction with a Waters Assoc. Nova-Pak C₁₈ column. The analytical column, in Radial-Pak cartridge form, was used in combination with a Waters Assoc. Z-module RCSS and protected by a Waters Assoc. Guard-Pak precolumn module containing a Guard-Pak μBondapak C₁₈ insert. Using ultraviolet detection at 214 nm, levels in the region of 50–100 ng/ml for CBZ and its metabolites can be measured with only 250 μl of plasma. The method has been used to determine steady-state concentrations of the drug and its metabolites in paediatric patients.     

A Novel Method for the Quantitation of Warfarin and its Metabolites in Plasma

Abstract

A procedure for the rapid, quantitative recovery of warfarin and its metabolites (diastereoisomeric alcohol, 4′-, 6-, 7-, 8-benzylic-hydroxywarfarin and dehydrowarfarin) from plasma with Sep-Pak C₁₈ cartridges has been developed. A solution of warfarin and its metabolites in plasma was acidified with NH₄OAc buffer (pH 4.85), adsorbed on the Sep-Pak C₁₈ resin, washed free of polar constituents and eluted with methanol. Dilution of the eluate with buffer followed by gradient high performance liquid chromatography permitted accurate quantitation of the desired compounds when detected at 313 nm. The recovery of warfarin and each metabolite was greater than 95% over an investigated range of 0.5–10.0 μg/ml of plasma and the limit of quantitation by the assay was 0.1 μg/ml of plasma. For more rapid quantitation of warfarin, without simultaneous analysis of metabolites, the chromatographic parameters were modified so that elution of warfarin occurred within 13 minutes, and the sensitivity of the assay increased to 0.03 μg of warfarin/ml of plasma. The quantitative recovery of warfarin and its metabolites coupled with the chromatographic versatility of the method make it ideally suited for either detailed pharmacokinetic studies or routine plasma analysis of warfarin.     

HPLC Measurement of Cyclosporine in Blood Plasma and Urine and Simultaneous Measurement of its Four Metabolites in Blood

Abstract

A high performance liquid chromatographic assay has been developed for the estimation of cyclosporine and its four major metabolites in blood and for cyclosporine alone in plasma and urine samples. This assay employs a rapid and very reproducible solid-liquid extraction system. Isocratic chromatographic conditions allow the simultaneous measurement of cyclosporine and its four major metabolites in blood. The method is linear up to 2500 ng/ml and the minimum quantifiable limit for cyclosporine is 30 ng/ml, when 1 ml of sample is analyzed.     

Studies on Mercury Pollution: Microdetermination of Mercury in Biological Materials by Cold Vapour Atomic Absorption Spectrometry

Abstract

A simple, rapid, precise and accurate method for the determination of mercury in biological material is described. Biological samples were digested with nitric acid and acidified potassium permanganate and determined by cold vapour analyser. The proposed method was successfully employed for the determination of mercury in samples of fish, hair and blood.     

Metabolite Identification of Myricetin in Rats Using HPLC Coupled with ESI-MS

Myricetin, a naturally occurring flavonol, shows multifarious pharmacological activities, e.g., antidiabetic, antioxidant, anti-inflammatory, antitumor, and liver protection effects. In order to obtain an understanding of the myricetin’s metabolism in vivo, a rapid and sensitive method by high-performance liquid chromatography coupled with electrospray-ionization mass spectrometry (HPLC-MSⁿ) techniques was employed to investigate the biotransformation in rats after oral administration of myricetin. Recognition and structural exposition of the metabolites were operated by comparing the changes in molecular mass (ΔM) and MSⁿ spectra with the parent drug. As a result, the parent compound and seven metabolites were found in rat plasma, urine, and feces. In addition, besides 3,5-dihydroxyphenylacetic acid (M1) and 3,4,5-trihydroxyphenylacetic acid (M2), five other compounds were first discovered in the metabolite research of myricetin. These results indicated that, besides ring-fission, there were methylate (M3, M4, M5) and glucuronide (M6, M7) biotransformations of myricetin occurring in vivo.

     

A Rapid and Sensitive Method for The Determination of Diclofenac Sodium in Plasma By High-Performance Liquid Chromatography

Abstract

A rapid and sensitive high-performance liquid chromatographic method for the determination of diclofenac sodium in plasma has been developed. The method is specific and free of interference from metabolites and common anti-inflammatory agents. The UV detector (215 nm) response was linear over a range of 5-1000 ng/ml. Day-to-day and within-day calibration curves were reproducible. The method was validated by analysis of spiked human plasma samples, partly in a blind fashion. The accuracy and precision of the method are satisfactory over the range of 5-1000 ng/ml. The method was cross-checked with the GC method. Results show a correlation coefficient of 0.983 and a slope of 1.04. The method is suitable for the routine analysis of large numbers of plasma samples usually obtained in bioavailability and pharmacokinetic studies.     

Separation of Hydroxylated Metabolites of Fatty Acids (C10-C18) on a μPorasil Silica Column Using an Isocratic HPLC System

Abstract

A simple, versatile, and rapid normal-phase isocratic HLPC system is described for the analysis of the major (omega and omega-1) metabolites of C₁₀-C₁₈ chain length fatty acids formed upon incubation with rat liver microsomes and NADPH. Quantitation was achieved by radiometric detection. Chromatographic separation was performed by elution of the fatty acids and their omega and omega-1 metabolites from a 10μ silica column (μPorasil) with hexane:2-propanol:acetic acid (96.5:2.5:1.0). Retention times for these metabolites ranged from 10 to 13 minutes for stearic acid and from 16 to 21 minutes for capric acid. Recovery of the fatty acids and their metabolites from the column was greater than 95 percent. Relative quantitative conversion of the fatty acid substrates to omega and omega-1 metabolites was in the following order: myristic acid > capric acid=lauric acid=palmitic acid ? stearic acid. The omega products were formed preferentially over the omega-1 products of all the fatty acids except lauric acid. The method proved suitable for routine determination of NADPH-dependent fatty acid hydroxylase activities in rat liver microsomes.