Determination of Nitric Oxide-Derived Nitrite and Nitrate in Biological Samples by HPLC Coupled to Nitrite Oxidation

Nitrite and nitrate are main stable products of nitric oxide, a pivotal cellular signaling molecule, in biological fluids. Therefore, accurate measurement of the two ions is profoundly important. Nitrite is difficult to be determined for a larger number of interferences and unstable in the presence of oxygen. In this paper, a simple, cost-effective and accurate HPLC method for the determination of nitrite and nitrate was developed. On the basis of the reaction that nitrite is oxidized rapidly to nitrate with the addition of acidic potassium permanganate, the determination of nitrite and nitrate was achieved by the following strategy: each sample was injected twice for HPLC analysis, i.e. the first injection was to measure nitrate, and the second injection was to measure total nitrate including initial nitrate and the nitrate from the conversion of nitrite with the addition of acid potassium permanganate in the sample. The amount of nitrite can be calculated as difference between injections 2 and 1. The HPLC separation was performed on a reversed phase C₁₈ column for 15 min. The mobile phase consisted of methanol–water (2:98 by volume); the water in the mobile phase contained 0.60 mM phosphate salt (potassium dihydrogen and disodium hydrogen phosphate) and 2.5 mM tetrabutylammonium perchlorate (TBAP). The UV wavelength was set at 210 nm. Additionally, we systemically investigated the effects of the concentration of phosphate salt and TBAP in the mobile phase, the pH of the mobile phase, and the amount of acidic potassium permanganate added to the sample on the separation efficacy. The results showed that the limits of detection (LOD) and the limit of quantitation (LOQ) were 0.075 and 0.25 μM for nitrate (containing the oxidized nitrite), respectively. The linear range was 1–800 μM. This developed approach was successfully applied to assay nitrite/nitrate levels in cell culture medium, cell lysate, rat plasma and urine.

     

Determination of Nitrate and Nitrite Ions in Human Plasma by Ion Exchange-High Performance Liquid Chromatography

Abstract

Acetonitrile precipitation of plasma samples followed by injection of supernatant onto a reverse phase precolumn coupled to an anion exchange column allowed ultraviolet detection (214 nm) of eluting nitrate and nitrite ions. Sensitivity in plasma is about 0.01 mM for both ions and linearity is excellent from 0.02 to 1.0 mM. Nitrite accuracy assessed by diazotization coupling was good. Reproducibility studies demonstrated withinrun coefficients of variation of < 4%. Interferences were few. Random endogenous serum nitrate concentrations (0.03–0.12 mM) were determined. Serum nitrite and nitrate concentrations were measured in a patient following an overdosage of isobutyl nitrite. The method is applicable for nitrite/nitrate studies in plasma at these concentrations.     

Rapid Analysis of Nitrate and Nitrite by Ion-Interaction Chromatography on a Monolithic Column

Ion-interaction chromatography with direct conductivity detection has been used for analysis of nitrate and nitrite. Chromatographic separation was performed on a monolithic silica-based C₁₈ column dynamically modified with tetrabutylammonium (TBA⁺). Using the optimized mobile phase, containing 2.0 mmol L^?1 TBA⁺ and 0.8 mmol L^?1 citrate (pH 6.0), delivered at a flow rate of 6.0 mL min^?1, separation of five anions (chloride, nitrite, bromide, nitrate, and sulfate) was achieved in only 40 s at a column temperature of 30 °C. The detection limits for nitrate and nitrite were 0.74 and 0.92 mg L^?1, respectively. The relative standard deviation (RSD, n = 5) of the retention times of nitrate and nitrite was 0.1% and RSD of chromatographic peak areas were 0.4 and 0.2%, respectively. The method was successfully used for analysis of the anions in groundwater. Recovery of nitrate and nitrite was 99.1 and 105%, respectively.     

Simultaneous LC–UV Determination of 5-Methyl-1-(3-fluorophenyl)-2-(1H)- pyridone and Its Two Metabolites in Rat Plasma

A simple, rapid, and reproducible isocratic reverse-phase HPLC method was developed to simultaneously determine AKF-PD and its two oxidized metabolites in rat plasma. 5-Carboxyl-1-phenyl-2-(1H)-pyridone and phenacetin were used as internal standards to ensure the precision and accuracy of the method. The analytes were separated on a C₁₈ reversed-phase column with methanol—phosphate buffer (20 mM, pH 2.5) as mobile phase. The limits of detection for AKF-PD and its two oxidized metabolites was 0.1 μg mL^?1. The method is applicable for the pharmacokinetic studies of AKF-PD and its metabolites in rats.     

Simultaneous LC–UV Determination of 5-Methyl-1-(3-fluorophenyl)-2-(1H)- pyridone and Its Two Metabolites in Rat Plasma

A simple, rapid, and reproducible isocratic reverse-phase HPLC method was developed to simultaneously determine AKF-PD and its two oxidized metabolites in rat plasma. 5-Carboxyl-1-phenyl-2-(1H)-pyridone and phenacetin were used as internal standards to ensure the precision and accuracy of the method. The analytes were separated on a C₁₈ reversed-phase column with methanol—phosphate buffer (20 mM, pH 2.5) as mobile phase. The limits of detection for AKF-PD and its two oxidized metabolites was 0.1 μg mL⁻¹. The method is applicable for the pharmacokinetic studies of AKF-PD and its metabolites in rats.

     

Direct determination of nitrite traces in high ionic-strength samples by electrostatic ion chromatography using diluted acid solutions as eluent

An ion-chromatographic (IC) system with high selectivity for separation of nitrite is described. It is analogous to the EIC (electrostatic IC) previously reported and was established using 3-(N,N-dimethylstearylammonio)propanesulfonate (C23H49NO3S, a sulfobetaine type of zwitterionic surfactants) as the stationary phase and dilute aqueous HCl solutions as the mobile phase. Five inorganic anions, sulfate, chloride, bromide, nitrate, and nitrite were chosen as the model analytes and were analyzed using this EIC system. Sulfate was always eluted first, followed by chloride, bromide and nitrate. Nitrite, however, could be eluted either before or after nitrate, depending on the concentration of HCl in the eluent. An elution order nitrate< nitrite was always obtained simply by using >3 mmol L(-1) HCl as the eluent. For nitrite the detection limit was better than 2.1 x 10(-7) mol L(-1) (100 microL sample injection volume, S/N=3, UV at 210 nm). Bromide and nitrate could also be separated under these HPLC conditions. The detection limit for bromide was 7.2 x 10(-8) mol L(-1) and for nitrate 6.5 x 10(-8) mol L(-1). Both nitrite and nitrate in real seawater samples were successfully determined with direct sample injection using this EIC system.     

Nitrite and nitrate measurement in human urine by capillary electrophoresis.

Nitrite and nitrate have been widely used as markers for nitric oxide (NO) formation in vivo and represent the major NO oxidation products in biological fluids. In the present study, the use of capillary electrophoresis (CE) in the measurement of nitrite and nitrate in human urine is described. Urine samples were electrophoresed in an extended light path fused-silica capillary (104 cm; 75 microm ID) at an applied negative potential of 30 kV, and UV detection at 214 nm. Using electrokinetic sample injection (-6 kV x 20 s), we found that urine concentration, pH, sodium and chloride interfered with nitrite and nitrate detection. The detection of nitrite and nitrate was decreased when hydrodynamic sample injection was used (30 mbar x 60 s). However, basal levels of urinary nitrite (0.25 +/- 0.05 microM) and nitrate (591 +/- 115 microM) were detected and no interference by variations in urine concentration and pH was noted when hydrodynamic sample injection was used. Thus, hydrodynamic sample injection is convenient for the measurement of urinary nitrite and nitrate and avoids the effect of variations in urine matrices and pH on nitrite and nitrate detection.     

Flow Injection Biamperometric Determination of Nitrite and Nitrate

Abstract

A simple and efficient FIA method was used with good results to determine nitrite in residual waters and nitrate in natural waters. Nitrite determination is based on the reaction with iodide occurring in acidic medium and biamperometric detection of the formed iodine at two platinum electrodes polarised at a potential of 100 mV. Nitrate is similarly determined after its previous reduction to nitrite in a cadmium column. The method does not need the solution deaeration. However, the calibration graphs present two regions of linearity owing to the catalytic effect of the dissolved oxygen on the iodide oxidation by nitrite.     

Spectrophotometer Determination of Nitrite Using Salbutamol sulphate as a Reagent

Abstract

A simple spectrophotometric method for the trace determination of nitrite (NO^? ₂) is described. Nitrite is reacted with Salbutamal sulphate in acidic medium which gives a yellow colour in alkaline medium (?pH 7) and can be determined in the presence of several cations and anions. Beer's law is obeyed in the range of 1.8 to 27.6 ppm of nitrite with the molar absorptivity 1.8 × 10³ 1 × mole^?1 × cm^?1 at 4l0 nm. The proposed method can also be utilized for the determination of nitrate (NO^? ₃) after its reduction to nitrite. The method has been applied for the determination of various samples containing traces of nitrite.     

Determination of Nitrate,Nitrite, and Phosphate at 214 NM by Reverse PhaseHPLC

Abstract

Nitrate and nitrite can be determined by reverse phase HPLC, using 1:1 methanol-water at pH 3.0 as the mobile phase and UV detection at 214 nm. Phosphate can be determined using 1:1:1 methanol-water-isopropyl alcohol at pH 3.0. At a flow rate of 1.0 mL/min, these anions elute within 5 min. A comparison of the mobile phases 1:1 methanol-water and Low UV PIC A reagent, indicates that 1:1 methanol-water yields 10 fold greater sensitivity to nitrate and 2 fold less to nitrite. The use of 1:1 methanol-water for the extraction of nitrate and nitrite from soil results in 19% higher recovery than in the case of water alone.     

Quantification of Suramin by Reverse-Phase Ion-Pairing High-Performance Liquid Chromatography

Abstract

A specific and sensitive method has been developed for the separation and quantification of suramin and trypan blue (internal standard) in human plasma. Plasma samples were extracted by centrifugation after the addition of ion-pairing reagent (tetra-butylammonium phosphate, TRAP) and methanol. Extracts were injected directly onto a reverse-phase ion-pairing HPLC system with 5 mM TBAP in the mobile phase. There was nearly 100% extraction efficiency after 3 cumulative extracts of each sample. The limit of quantitation was 0.5 μg/ml at a detection wavelength of 313 nm. Analysis of 3 post-therapy samples from a patient with AIDS was used to determine a plasma half-life for suramin of at least 3 weeks.     

The Use of Ultrasound for the Analytical Determination of Nitrite on Diamond Electrodes by Square Wave Voltammetry

Abstract

This work describes an analytical methodology for the determination of nitrite ions in aqueous solutions using boron‐doped diamond electrodes and square wave voltammetry associated with ultrasound radiation. The nitrite ions were oxidized to nitrate ions in Britton‐Robinson buffer solutions 0.1 M, pH 2.0 at 1.0 V versus Ag/AgCl. The voltammetric response of nitrite in the presence of ultrasound showed a peak current five times higher than the obtained in silent conditions. Thus, the detection limit obtained in the presence of radiation was 17 nM (0.782 µg l^?1), a small value if compared with that obtained in the absence of ultrasound: 140 nM (6.44 µg l^?1).     

Simultaneous determination of nitrite and nitrate in dew, rain, snow and lake water samples by ion-pair high-performance liquid chromatography

A simple, fast, sensitive and accurate reversed-phase ion-pair HPLC method for simultaneous determination of nitrite and nitrate in atmospheric liquids and lake waters has been developed. Separations were accomplished in less than 10 min using a reversed-phase C₁₈ column (150 mm × 2.00 mm i.d., 5 μm particle size) with a mobile phase containing 83% 3.0 mM ion-interaction reagent tetrabutylammonium hydroxide (TBA-OH) and 2.0 mM sodium phosphate buffer at pH 3.9 and 17% acetonitrile (flow rate, 0.4 mL/min). UV light absorption responses at 205 nm were linear over a wide concentration range from 100 μg/mL to the detection limits of 10 μg/L for nitrite and 5 μg/L nitrate. Quantitation was carried out by the peak area method. The relative standard deviation for the analysis of nitrite and nitrate was less than 3.0%. This method was applied for the simultaneous determination of nitrite and nitrate in dew, rain, snow and lake water samples collected in southeast Massachusetts. Nitrate was found being present at 4.79-5.99 μg/mL in dew, 1.20-2.63 μg/mL in rain, 0.32-0.60 μg/mL in snow and 0.12-0.23 μg/mL in lake water. Nitrite was only a minor species in dew (0.62-0.83 μg/mL), rain (<0.005-0.14 μg/mL), snow (0.021-0.032 μg/mL) and lake water (0.12-0.16 μg/mL). High levels of nitrite and nitrate observed in dew water droplets may constitute an important source of hydroxyl radicals in the sunny early morning.     

Kinetic Spectrophotometric Determination of Nitrite with Tropaeolin 00-Bromate System

A simple accurate kinetic spectrophotometric method was developed for the determination of nitrite based on its catalytic effect on the redox reaction between tropaeolin 00 and bromate in acid medium. Nitrite was determined by measuring the decrease in the absorbance of tropaeolin 00 at 530 nm by a fixed time method, after 30 s from the initiation of the reaction. The calibration graph was linear in the range 6–500 ng mL^?1 of nitrite and the detection limit was 2 ng mL^?1. The proposed method is selective and is useful for the determination of nitrite in drinking water samples.     

Comparison of HPLC and MEEKC for Miconazole Nitrate Determination in Pharmaceutical Formulation

A simple solid phase extraction (SPE) method coupled with high performance liquid chromatography (HPLC) using UV detector and microemulsion electrokinetic chromatography (MEEKC) has been developed and compared for the quantitative determination of miconazole nitrate in pharmaceutical formulation. For HPLC method, two parameters were optimized, namely, the wavelength and the mobile phases. The optimized condition was at the 225 nm wavelength and the mobile phase of ACN:MeOH (90:10 v/v). There are seven MEEKC parameters that were optimized, in this research, which were applied to voltage, temperature, wavelength, sodium dodecyl sulfate (SDS) concentration, buffer pH, buffer concentration and butan-1-ol concentration. The optimum MEEKC condition was obtained using 86.35 % (w/w) 2.5 mM borate buffer pH 9, 0.25 % (w/w) SDS, 0.8 % (w/w) ethyl acetate, 6.6 % w/w butan-1-ol and 6.0 % (w/w) acetonitrile. The combination of SPE using a diol column with HPLC–UV and the MEEKC methods were successfully applied for the determination of miconazole nitrate in a pharmaceutical formulation with the recovery percentage of 98.35 and 92.50 %, respectively.

     

Comparison of Ion-Pairing and Reversed Phase Liquid Chromatography in Determination of Sulfamethoxazole and Trimethoprim

Abstract

Two simple, rapid, and sensitive HPLC methods have been developed for the simultaneous determination of sulfamethoxazole and trimethoprim in their pure and dosage forms, one utilizing reversed phase HPLC and the other ion-pair HPLC. In the reversed phase HPLC method (A) the mobile phase consists of 0.05% aqueous solution of formic acid with pH adjusted to 4.5±0.2 with triethylamine : acetonitrile:tetrahydrofuran 50 : 49 : 1 (v/v), and the mobile phase pumped at flow rate of 1.0 ml min^?1. An Appolo LC18 column (5.0 µm), 250 mm length × 4.6 mm diameter, was utilized as the stationary phase. Detection was affected spectrophotometrically at 254 nm. In the ion-pair HPLC method (B) the mobile phase consisted of methanol : buffer 35 : 65 (v/v) with the buffer composed of potassium dihydrogen phosphate 0.3 M and sodium heptan sulfonic acid 5.0 mM. To 500 ml of buffer was added 2.0 ml triethylamine, and then the pH was adjusted to 5.0 with phosphoric acid, and the mobile phase was pumped at a flow rate of 1.2 ml min^?1. A Hypersil C₁₈ column (5.0 µm), 150 mm length × 4.6 mm diameter, was utilized as the stationary phase. Detection was affected spectrophotometrically at 254 nm. Linearity ranges for sulfamethoxazole and trimethoprim were 1.0–110 and 1.5–98 µg ml^?1, respectively, with method A and 0.5–100 and 1.0–125 µg ml^?1, respectively, with method (B). Minimum detection limits obtained were 0.1969 and 0.3451 µg ml^?1 for sulfamethoxazole and trimethoprim, respectively, with method A, and 0.1377 and 0.2454 µg ml^?1 with method (B). The proposed methods were further applied to the analysis of tablets containing the two drugs, and the results were satisfied.     

Comparison of HPLC and MEEKC for Miconazole Nitrate Determination in Pharmaceutical Formulation

A simple solid phase extraction (SPE) method coupled with high performance liquid chromatography (HPLC) using UV detector and microemulsion electrokinetic chromatography (MEEKC) has been developed and compared for the quantitative determination of miconazole nitrate in pharmaceutical formulation. For HPLC method, two parameters were optimized, namely, the wavelength and the mobile phases. The optimized condition was at the 225 nm wavelength and the mobile phase of ACN:MeOH (90:10 v/v). There are seven MEEKC parameters that were optimized, in this research, which were applied to voltage, temperature, wavelength, sodium dodecyl sulfate (SDS) concentration, buffer pH, buffer concentration and butan-1-ol concentration. The optimum MEEKC condition was obtained using 86.35 % (w/w) 2.5 mM borate buffer pH 9, 0.25 % (w/w) SDS, 0.8 % (w/w) ethyl acetate, 6.6 % w/w butan-1-ol and 6.0 % (w/w) acetonitrile. The combination of SPE using a diol column with HPLC–UV and the MEEKC methods were successfully applied for the determination of miconazole nitrate in a pharmaceutical formulation with the recovery percentage of 98.35 and 92.50 %, respectively.     

New Validated Methods for the Simultaneous Determination of Two Multicomponent Mixtures Containing Guaiphenesin in Syrup by HPLC and Chemometrics‐Assisted UV‐Spectroscopy

Abstract

High pressure liquid chromatographic (HPLC) and spectrophotometric methods are developed for the determination of two multicomponent mixtures containing guaiphenesin, dextromethorphane hydrobromide, and sodium benzoate together with either phenylephrine hydrochloride, chlorpheniramine maleate, and butylparaben (mixture 1) or ephedrine hydrochloride and diphenhydramine hydrochloride (mixture 2). The HPLC method depended on using an ODS column with mobile phase consisting of acetonitrile ?10 mM potassium dihydrogen phosphate, pH 2.7 (40∶60 v/v) containing 5 mM heptane sulfonic acid sodium salt (for mix 1) and a cyanopropyl column with mobile phase consisting of acetonitrile ?12 mM ammonium acetate, pH 5 (40∶60 v/v) (for mix 2) and UV detection at 214 nm. The cyanopropyl column is much less hydrophobic, less sterically restricted to the penetration of bulky solute molecules into the stationary phase, and has weaker hydrogen‐bond acidity than the ODS column. So the cyanopropyl column is more suitable for separation of components of mix 2. The chemometric‐assisted spectrophotometric method with, principal component regression (PCR) and partial least squares (PLS‐1) was used. For the chemometric method a calibration set of the mixture consisting of each compound in each mixture was prepared in distilled water. The absorbance data in the UV spectra were measured in the spectral region (210–240 or 210–224 nm for mix 1 and mix 2, respectively, as this range provided the greatest amount of information about the two mixture components). The spectrophotometric method does not require a separation step. The proposed methods were successfully applied for the analysis of the two multicomponents combinations in laboratory‐prepared mixtures and in commercial syrups, and the results were compared with each other.     

Focused Microwave-Assisted Extraction and LC Determination of Ketoprofen in the Presence of Preservatives in a Pharmaceutical Cream Formulation

A simple and rapid open-vessel focused microwave-assisted extraction (FMAE) method followed by LC analysis was developed for the determination of ketoprofen lysine salt in the presence of methyl p-hydroxybenzoate and propyl p-hydroxybenzoate preservatives in topical cream. Extraction were performed in acetone/potassium dihydrogenphosphate (25 mM, pH 3.0) (70:30 v/v) by reaching a target temperature of 65 °C in a 10 min linear ramp. The chromatographic separation was performed on a Discovery RP-Amide C16 column (250 × 4.6 mm I.D., 5 μm particle size). The optimal mobile phase consisted of acetonitrile/potassium dihydrogen phosphate 25 mM adjusted to pH 3.0 with phosphoric acid (50:50 v/v). The complete analytical procedure was validated with regard to limit of quantification, linearity, precision and accuracy. The method was linear over the concentration range of 0.08–0.12 mg mL⁻¹; the relative standard deviations of intra- and inter-day assays were 1.9–2.3 and 1.8% respectively. The limit of quantification was 0.54 μg mL⁻¹. The proposed method shows many advantages as short extraction time, little solvent consumption without requiring further sample clean-up steps before liquid chromatographic analysis and is proposed for vast scale screening of cream dosage forms aimed to the detection of counterfeit and substandard drugs.

     

A simple isocratic LC method for quantification of trace-level inorganic degradation impurities (ferricyanide,ferrocyanide, nitrite,and nitrate) in sodium nitroprusside injection and robustness by quality using design approach

This study developed and validated a trace-level quantification inorganic impurities method using reversed-phase HPLC and performed the robustness check using quality-by-design approach by varying the multiple factors simultaneously. This method is economical and simple and exhibits its stability-indicating nature [for the determination of ferrocyanide ([Fe(CN)₆]^4–), ferricyanide ([Fe(CN)₆]³⁻), nitrate (NO₃^–), and nitrite (NO₂^–)] in sodium nitroprusside (SNP) drug substance and liquid dosage form. Chromatographic separation was achieved using a USP L43 column (ACE PFP, 150 × 4.6 mm, 3 μm) with a simple isocratic elution. The buffer consists of potassium dihydrogen phosphate (50 mM), tetrabutylammonium hydrogen sulfate (9 mM), and tetrabutylammonium hydroxide (25 mM). The buffer pH was adjusted to 7.2 with tetrabutylammonium hydroxide. The mobile phase was mixed with the buffer and acetonitrile (68:32 v/v). The flow rate was 0.8 mL/min, column temperature was maintained at 30°C, and injection volume was 5.0 μL. The SNP impurities were monitored at 225 nm using a UV detector. Further, the method was validated per the International Council for Harmonisation (ICH) guidelines, and forced degradation studies were carried out under different stress conditions. The detector responses were plotted against concentrations, and correlation was linear (r > 0.999) over the range of 0.8–7.5 μg/mL for ferricyanide; 1.0–37.5 μg/mL for SNP; and 0.2–7.5 μg/mL for ferrocyanide, nitrite, and nitrate. The method repeatability was established for all the impurities with relative standard deviation (%), and the results were found to be less than 2.0.