Separation of Ribose-5-phosphate,Ribose-1-phosphate,Deoxyribose-1-phosphate by High Performance Liquid Chromatography and Spectrophotometric Determination Using 2-Cyanoacetamide

Abstract

A simple procedure for separation of ribose-5-phosphate, deoxyribose-1-phosphate and ribose-1-phosphate is based on high performance liquid chromatography using reversed phase 4 × 300 mm “μ Bondapak/NH₂” column. The column is equilibrated with 0.13 M borate buffer (pH 7.5) followed by gradient elution of ribose-5-phosphate, deoxyribose-1-phosphate and ribose-1-phosphate using water, 0.05 M borate buffer containing 0.1 M MgCl₂ (pH 9.6) and 0.05 M sodium acetate-acetic acid buffer containing 0.1 M MgCl₂ (pH 5.0) as eluants respectively. Eluates of borate complex “μ Bondapak/NH₂” column are brought to pH 9.6 by the addition of 1 N KOH and enzymatically hydrolysed with alkaline phosphatase (EC 3.1.3.1) to release the free pentoses. The free pentoses are mixed with a reagent solution prepared from aqueous solution of 2% cyanoacetamide and 0.6 M borate buffer (pH 9.6), and the mixture is boiled for 10 minutes and the absorbance of the product is measured at 276 nm using a spectrophotometer.     

The Determination of Folic Acid (Pteroylmonoglutamic Acid) in Fortified Products by Reversed Phase High Pressure Liquid Chromatography

Abstract

A reversed phase HPLC method was developed for the separation and determination of pteroylglutamic acid (PGA) in fortified foods. Extraction was carried out by heating with phosphate-citrate buffer, pH 8.0 containing ascorbate, and incubation with papain at 40°C for 4 hrs. The extracts were purified and concentrated on a short DEAE column which was rinsed with phosphate buffer, pH 7.0, of increasing molarity. PGA was eluted with 0.1M phosphate buffer, pH 7.0, containing 0.5M NaCl. The eluants were chromatographed on a Spherisorb ODS 10 μm column (250 × 4.6 mm) using a 30 min linear gradient of 2% to 30% acetonitrile in 0.1M acetate buffer, pH 4.0, at 1 ml/min and an absorbance detector at 280 nm. The coefficients of variation on analysis of 8 replicate samples of a milk and soy protein based infant formulas were 5.9% (at 4.6 ng/50 μl inject) and 6.8% (at 1.8 ng/50 μl inject) respectively.     

High Performance Liquid Chromatographic Analysis of Penicillin V Solid Dosage Forms

Abstract

An isocratic high performance liquid chromatographic (HPLC) method for the determination of Penicillin V in solid dosage forms is described. A reverse phase RP-8 column and a mobile phase of 52% methanol in 0.05 M phosphate buffer (pH 3.3) were employed. Detection was effected at 254 nm. The results obtained are compared with those from the iodometric method.     

Differential preconcentration of arsenic(III) and arsenic(V) with thionalide loaded on silica gel

2-Mercapto-N-2-naphtylacetamide (thionalide) on silica gel is used for differential preconcentration of μg l^?1 levels of arsenic(III) and arsenic(V) from aqueous solution. In batch experiments, arsenic(III) was quantitatively retained on the gel from solutions of pH 6.5–8.5, but arsenic(V) and organic arsenic compounds were not retained. The chelating capacity of the gel was 5.6 μmol g^?1 As(III) at pH 7.0. Arsenic retained on teh column was completely eluted with 25 ml of 0.01 M sodium borate in 0.01 M sodium hydroxide containing 10 mg l^?1 iodine (pH 10). The arsenic was determined by silver diethyldithiocarbamate spectrophotometry. Arsenic(V) was subsequently determined after reduction to arsenic(III) with sulphite and iodide. Arsenic(III) and arsenic(V) in sea water are shown to be < 0.12 and 1.6 μg l^?1, respectively.     

Rapid screening method for the determination of diethylstilbestrol in edible animal tissue by column liquid chromatography with electrochemical detection

A rapid and sensitive screening method for the determination of residues of diethylstilbestrol in edible animal tissue is described. The analyte was extracted from the tissue with tert.-butyl methyl ether, reextracted with 1 M sodium hydroxide and further cleaned up by solid-phase extraction with C18 cartridges. Analysis was performed by isocratic elution with a phosphate-buffered mobile phase, methanol-0.05 M phosphate buffer pH 3.5 (67:33), on a Nucleosil 5-microns C18 column with electrochemical detection at +0.90 V. The average recovery of trans-diethylstilbestrol in spiked samples is 66%, with a standard deviation of 14% (n = 22) in the range 0.5-2.0 microgram/kg. The detection limit is 0.1-0.2 microgram/kg, although at this level other compounds may interfere and give rise to false positive results.     

Determination of arsenic species by capillary zone electrophoresis with large-volume field-amplified stacking injection.

Determination of arsenic species by large-volume field amplified stacking injection-capillary zone electrophoresis (LV-FASI-CZE) is reported in this paper. Whole column injection was employed. The optimum buffer pH for the separation of weak acids was discussed. It was found that the optimum buffer to analyze the stacked arsenate (As(V)), monomethylarsonate (MMA), and dimethylarsinate (DMA) was 25 mM phosphate at pH 6.5. However, the optimum buffer to analyze the concentrated arsenite (As(III)) was 20 mM phosphate - 10 mM borate at pH 9.28. The limits of detection of the method developed were 0.026 mg/L for As(III), 0.023 mg/L for As(V), 0.043 mg/L for MMA, and 0.018 mg/L for DMA. An enrichment factor of 34-100 for several arsenic species was obtained. In the end, this method was applied to determine the arsenic concentration in the environmental reference materials to show the usefulness of the method developed.     

High Performance Liquid Chromatographic Determination of Oxamniquine in Plasma Samples

Abstract

A sensitive and reliable liquid chromatographic assay procedure for the quantitation of oxamniquine in plasma or urine was developed. Chromatographic separation was achieved on a reversed-phase phenyl colum using U.V. Detection at 254 nm. The eluting solvent was the mixture of 0.05 M acetate buffer pH 5 and acetonitrile (3:7). With this mobile phase the drug and its external standard were well separated from the interference of the blank samples. The average recovery of oxamniquine from 3 or more replicate dog plasma samples of different concentration (0.125 ? 4.00 μg/ml) was 95.5% and its coefficient of variation was 4.17%. The reproducibility of the assay was confirmed by the analysis of variance test for the slopes of the three standard plots obtained from plasma samples at three different occasions (F=4.2, p > 0.01). The detection limit for plasma samples was approximately 20 ng/ml. The method was applied to measure the plasma level vs, time profile of this drug following a single bolus intravenous dose of 16 mg/kg to a dog.     

High-performance liquid chromatographic determination of rifapentine in serum using column switching.

A high-performance liquid chromatographic method with column switching has been developed for the determination of rifapentine in serum. The serum samples were injected onto a precolumn packed with Corasil RP C18 (37-50 microns) after simple dilution with an internal standard in a 1% ascorbic acid solution. Polar serum components were washed out using 0.05 M phosphate buffer. After valve switching, the concentrated drugs were eluted in the back-flush mode and separated by a mu Bondapak C18 column with acetonitrile-tetrahydrofuran-0.05 M phosphate buffer (pH 7.0) (42:5:53, v/v/v) as the mobile phase. The method showed excellent precision with good sensitivity and speed, and a detection limit of 0.1 microgram/ml. The total analysis time was less than 25 min and the mean coefficients of variation for intra- and inter-assay were less than 4.8%. The method has been successfully applied to serum samples from dogs after the oral administration of rifapentine.     

Development and comparison of HPLC and MEKC methods for the analysis of cyclic sulfur mustard degradation products

In this study, novel, fast, and simple methods based on RP‐HPLC and MEKC with DAD are developed and validated for the qualitative and quantitative determination of five cyclic sulfur mustard (HD) degradation products (1,4‐thioxane, 1,3‐dithiolane, 1,4‐dithiane, 1,2,5‐trithiepane, and 1,4,5‐oxadithiepane) in water samples. The HPLC method employs a C18 column and an isocratic water‐ACN (55:45, v/v) mobile phase. This method enables separation of all five cyclic compounds within 8 min. With the CE method, the baseline separation of five compounds was achieved in less than 11 min by applying a simple BGE composed of a 10 mM borate buffer and 90 mM SDS (pH 9.15). Both methods showed good linear correlation (R ² > 0.9904). The detection limits were in the range of 0.08–0.1 μM for the HPLC method and 10–20 μM for MEKC. The precision tests resulted in RSDs for migration times and peak areas less than 0.9 and 5.5%, respectively, for the HPLC method, and less than 1.1 and 7.7% for the MEKC method, respectively. The developed methods were successfully applied to the analysis of five cyclic HD degradation products in water samples. With the HPLC method, the LODs were lowered using the SPE for sample purification and concentration.     

Rapid Purification of the Unstable Enzyme Carbamoyl Phosphate Synthase by High Pressure Liquid Chromatography

Abstract

Extracts of soluble proteins obtained from rat liver mitochondria by freeze-thawing and subsequent diafiltration were fractionated by HPLC on a I 250 protein column. The column was eluted either with 0.05 M phosphate buffer pH 6.85 or 0.1 M acetate buffer pH 7.15. Specific fractions obtained by elution with either phosphate or acetate buffer showed a 6.1-fold or 5.5-fold increase in the specific activity of Carbamoyl phosphate synthase when compared with that of crude mitochondrial preparations. The purification and the molecular weight of carbamoyl phosphate synthase were verified by sodium dodecyl sulphate-polyacrylamide gel electrophoresis.     

Determination of palladium,platinum, and rhodium by HPLC with online column enrichment using 4-carboxylphenyl-thiorhodanine as a precolumn derivatization reagent

In the present work, 4-carboxylphenyl-thiorhodanine (CPTR) was synthesized. A new method for the simultaneous determination of palladium, platinum, and rhodium ions as metal-CPTR chelates was developed using rapid column high-performance liquid chromatography equipped with an online enrichment capability. Palladium, platinum, and rhodium ions were precolumn-derivatized with CPTR to form colored chelates. The Pd-CPTR, Pt-CPTR, and Rh-CPTR chelates can absorbed onto the front of the enrichment column (ZORBAX Stable Bound, 4.6 × 10 mm, 1.8 μm) when they are injected with a buffer solution of 0.05 M sodium acetate-acetic acid (pH 3.5) as mobile phase. After the enrichment had finished, by switching the six-port switching valve, the retained chelates were back-flushed by mobile phase and moved towards the analytical column. The chelate separation on the analytical column (ZORBAX Stable Bound, 4.6 × 50 mm, 1.8 μm) was achieved with 46% acetonitrile (containing 0.05 M of pH 3.5 sodium acetate-acetic acid buffer and 0.01 M tritonX-100) as mobile phase. The palladium, platinum, and rhodium were separated completely within 2 min. The detection limits (S/N = 3) of palladium, platinum, and rhodium are 1.4, 1.6, and 2.0 ng/L, respectively. The method was applied to the determination of palladium, platinum, and rhodium in water, urine, and soil samples with good results. The text was submitted by the authors in English.     

Fluorimetric assay of dopamine, norepinephrine and their 3-O-methyl metabolites by using fluorescamine.

Fluorescamine was subjected to reaction with dopamine and norepinephrine (catecholamines) and with 3-methoxytyramine and normetanephrine (3-methyl metabolites of catecholamines) in phosphate or borate buffer. Catecholamines gave the highest fluorescent intensity at pH 8.0 in phosphate buffer but lower fluorescence in borate buffer. The fluorophores produced in phosphate or borate buffer were the same but the fluorescence intensities were suppressed in borate buffer. The dopamine and norepinephrine fluorophores were separated by high-pressure liquid chromatography on Hitachi 3011 gel with methanol-0.10 M Tris buffer of pH 8.0 (7:3). They were measurable at the 100-pmole level. The metabolites were also measurable by the same chromatography. By using methanol-0.15 M borate buffer of pH 8.0, cate-chol-O-methyltransferase activity might be assayed.     

Further studies on the reaction of amines and proteins with 4-fluoro-7-nitrobenzo-2-oxa-1,3-diazole

The reaction of glycine with NBD-F (4-fluoro-7-nitrobenzo-2-oxa-1,3-diazole) is investigated to establish conditions that provide a high formation rate of NBD-glycine and a low hydrolysis rate of the reagent. The reaction rate increases with higher temperature, larger contents of organic solvent and a sodium borate buffer. The use of borate buffer decreases ther ate of hydrolysis of the reagent. For low-molecular-weight amines, condition for a suitable liquid chromatographic postcolumn reactor include a high content of acetonitrile and 0.1 M sodium borate (pH 8.0–8.5). For proteins, separated by molecular-exclusion chromatography, water is needed for sensitive reactions. Suitable postcolumn reactor conditions include borate buffer (pH 7.9) containing 0.1 M potassium chloride, a 0.02% (w/v) NBD-F solution in acetonitrile with reaction at 50°C for about 45 s. The detection limits for human serum albumin, β-lactoglobulin and myoglobin are 6.6 pmol, 8.4 pmol and 11 pmol, respectively.     

Quantitation of Indomethacin in Serum by HPLC Using Fluorescence Detection

Abstract

An improved, sensitive and accurate HPLC procedure using fluorescence detection for quantitation of indomethacin in serum has been developed. After addition of an equal volume of phosphate buffer, pH 6.6 to serum along with the internal standard, the samples were extracted with methylene chloride. Prior to chromatography, the extracted indomethacin was deacylated to its fluorescent product (DBI) in 0.01 N-NaOH. The mobile phase consisted of methanol and pH 4 acetate buffer (3:7 V/V) and the separation was achieved on a C18 reversed phase column. The retention times of DBI and the internal standard were 7.5 and 16.0 min. respectively. The fluorometric excitation and emission wavelengths were 278 and 358 nm, respectively. The sensitivity of the assay was 1 ng/ml of serum and the CV at this concentration was 2.46%. The standard plot was linear (r > 0.999) for indomethacin concentrations between 1 and 500 ng/ml. The inter-and intra-day studies showed high reproducibility (CV = 2.8%, F = 0.89, p > 0.05). The method was used to determine the complete serum level vs. time profiles of indomethacin in animals.     

Extraction and Spectrophotometric Determination of Neomycin Sulfate in Pharmaceutical Oral Suspensions

Abstract

The conditions of neomycin extraction were studied in pharmaceutical oral suspensions to permit its determination by spectrophotometry after reaction with 2, 4-dinitrofluorobenzene. The best recovery of neomycin was obtained with centrifugation employing water as the extraction agent. The spectrophotometric analysis was carried out in 0.02 M borate buffer (pH 9.0), under ambient conditions after 50 minutes of reaction. The absorbance of the yellow product was measured at 365 nm.     

Ternary Complex Nickel(II)/3-(4′,5′-Dimethyl-2′-Thiazolylazo)-2,6-Dihydroxybenzoic Acid/Cyanide. Spectrophotometric Determination of Nickel

Abstract

A spectrophotometric method for nickel has been developed based on the formation of a ternary complex in the system Ni(II)/3-(4′,5′-dimethyl-2′-thiazolylazo)-2,6-dihydroxybenzoic acid/cyanide at pH 9.2 (borate buffer), which allows the determination of 0.05–0.47ppm of nickel (ε = 3.53×10⁴ 1.mol^?1. cm^?1) at 538nm. Interferences have been studied and the method applied to the determination of nickel in low alloy steels.     

Separation of Xanthine Derivates by High Pressure Liquid Chromatography and Application to Plasma Analysis

Abstract

High pressure liquid chromatography (HPLC) methods were developed for separation and plasma analysis of ten xanthine derivates. Separation was evaluated on silica column and on three different reverse phase columns, with optimum conditions obtained on C₆ spherisorb column using isocratic elution with phosphate buffer 10^?2 M, pH 2.7 - acetonitrile mixture (80/20 V/V). Determination of these xanthine derivates in plasma for therapeutic control was studied.     

Determination of triazine compounds in ground water samples by micellar electrokinetic capillary chromatography

In this work, a capillary electrophoresis (CE) method for the determination of a group of eleven triazine compounds by micellar electrokinetic capillary chromatography (MEKC) with diode array detection was developed. The eleven herbicides studied were: desethylatrazin-2-hydroxy (DEA), simazine, prometon, atrazine, simetryn, ametryn, propazine, prometryn, trietazine, terbutylazine, and terbutryn The separation of these compounds was optimised as a function of buffer concentration and pH, concentration of sodium dodecyl sulphate (SDS) and voltage applied. To increase the selectivity of the separation and the resolution of the solutes, different organic solvents were tested as buffer additives, obtaining the best results when 1-propanol was used. The optimised buffer (24 mM of sodium borate, 18 mM of disodium hydrogen phosphate, 25 mM of SDS, pH 9.5, and 5% of 1-propanol) provides the best separation in terms of resolution and migration time. This method allowed the determination of these compounds at concentrations of 0.05 μg l⁻¹ in ground water samples pretreated using solid-phase extraction (SPE).     

Determination of aluminium,copper, iron and manganese in biological and other samples as 8-quinolinol complexes by high-performance liquid chromatography with electrochemical and spectrophotometric detection

A range of methods based on reverse-phase high-performance liquid chromatography is described for determining Al, Cu, Fe and Mn. The simplest method for determining Fe, Cu and Al involves direct formation and separation of the 8-quinolinol complexes on the column, with 1:1 acetonitrile/water containing 5 × 10^?3 M 8-quinolinol, 0.4 M potassium nitrate and 0.02 M acetate buffer (pH 6.0) as the mobile phase, followed by electrochemical detection at ?0.5 V vs. Ag/AgCl and/or spectrophotometric detection at 400 nm. Electrochemical detection enables < 2 ng Cu and < 1 ng Fe to be quantified for injection volumes of 20 μ1. Spectrophotometric detection allows simultaneous determinations of Al, Cu and Fe with lower sensitivity. The method is applied to the determination of Cu, Fe and Al in bovine liver and oyster tissue. Down to 1 ng of manganese (in the 20 μ1 injected) can be determined in biological samples by liquid chromatography with a mobile phase containing 1 mM Tris buffer (pH 8.8) after injection of an externally prepared 8-quinolinol complex. Preconcentration on Sep-Pak cartridges after dichloromethane extraction is used for the determination of low concentrations of iron in water. A sensitive determination of aluminium based on detection at 254 nm is also reported.     

Separation of Nucleobases Using High‐performance Liquid Chromatography Coupled with Voltammetric Scanning

In this paper, a method based on chromatographic separation of analytes and their quantification using on‐line cyclic voltammetry is reported. The method based on high performance liquid chromatography on reverse phase column was optimized using free nucleobases‐guanine, adenine, thymine, and cytosine. The optimal separation of nucleobases was detected when using 0.05 M borate buffer (pH 9.0) as the mobile phase, at isocratic flow rate 1 mL min⁻¹, and at separation column temperature of 30 °C. The accurate timing of the cyclic voltammetry enabled us to quantify the concentrations of individual nucleobases by oxidation on glassy carbon electrode.