Kinetic fluorimetric determination of carbamazepine in serum by the stopped-flow technique

Summary A simple, fast method for the determination of carbamazepine in serum is reported for the first time. It is based on the fluorescent reaction of this drug with cerium(IV) in an acid medium. A stopped-flow mixing module coupled to a conventional spectrofluorimeter is used for this purpose. The linear range of the proposed method is 0.04–140 g ml^–1 of carbamazepine and the detection limit is 0.01 g ml^–1. The within- and between-assay precision data and selectivity results show the method to be adequate for the determination of carbamazepine in serum by including a preliminary extraction step with dichloromethane. Analytical recoveries from different serum samples are reported.     

A flow-injection ultrafiltration sampling chemiluminescence system for on-line determination of drug–protein interaction

A flow-injection ultrafiltration sampling chemiluminescence system for on-line determination of cimetidine–bovine serum albumin (BSA) interaction is proposed in this paper. Cimetidine can be oxidized by N-bromosuccinimide (NBS) and sensitized by fluorescein to produce high chemiluminescence emission in basic media. The concentration of cimetidine is linear with the CL intensity in the range 3×10^–7–1×10^–4 mol L^–1 with a detection limit of 1×10^–7 mol L^–1 (3). The drug and protein were mixed in different molar ratios in 0.067 mol L^–1 phosphate buffer, pH 7.4, and incubated at 37 °C in a water bath. The ultrafiltration probe was utilized to sample the mixed solution at a flow rate of 5 µL min^–1. The data obtained by the proposed ultrafiltration flow-injection chemiluminescence method was analyzed with Scrathard analysis and a Klotz plot. The estimated association constant (K) and the number of the binding site (n) on one molecule of BSA by Scrathard analysis and Klotz plot were 3.15×10⁴ L mol^–1 and 0.95, 3.25×10⁴ L mol^–1 and 0.92, respectively. The proposed system proved that flow-injection chemiluminescence analysis coupled with on-line ultrafiltration sampling is a simple and reliable technique for the study of drug–protein interaction.     

Microdetermination of Proteins with the 1,10-Phenanthroline–H2O2–Cetyltrimethylammonium Bromide–Cu(II) Chemiluminescence System

Proteins can enhance the chemiluminescence (CL) intensity of the 1,10-phenanthroline–H₂O₂–cetyltrimethylammonium bromide (CTMAB)–Cu(II) system because unsaturated complexes of Cu(II) with protein have a much stronger catalytic effect on the CL reaction than does Cu(II). On this basis, a new flow injection analysis method for detection of some proteins was established. The method gives linear responses over two orders of magnitude and detection limits at the 0.02–0.05 μg ml⁻¹level for bovine serum albumin, human serum albumin, γ-globulin, and egg albumin. The method was used for determination of proteins in human serum with satisfactory results.     

Kinetic-Spectrophotometric Determination of Trace Quantities of Thiocyanate Based on Its Landolt Effect on the Reaction of Bromate with Hydrochloric Acid1

A new method for the rapid and sensitive determination of trace quantities of thiocyanate based on its Landolt effect on the bromate-hydrochloric acid reaction was developed. The induction period of the reaction is proportional to the SCN^– concentration. The decolorization of methyl orange by the reaction products was used to monitor the reaction spectrophotometrically at 525 nm. We were able to determine thiocyanate in the range 2 × 10^–7–4 × 10^–5 M by this method. The relative standard deviation for 10 determinations of 1.5 × 10^–6 M thiocyanate ion is 0.19% and the detection limit of the method was 7.00 × 10^–8 M. The method was applied to the determination of thiocyanate in human blood serum and of saliva samples with satisfactory results.     

Direct determination of trace refractory elements in human serum by ETV–ICP–MS with in-situ matrix removal

A method for in-situ removal of matrix is proposed for direct determination of trace refractory elements in human serum by ETV–ICP–MS with the use of poly(tetrafluoroethylene) (PTFE) as fluorinating reagent. Attention has been paid to investigating the vaporization behavior both of refractory elements of interest and of matrix elements (Na, K, Ca, Mg, Cl, S, and P) in a graphite furnace with the PTFE modifier present or not. It was shown that potential interferences from the organic and inorganic matrices in the serum sample could be eliminated or reduced to a negligible level by appropriate dilution of the serum and deliberate optimization of the ETV temperature program. The proposed method has been applied to the direct simultaneous determination of V, Cr, Mo, Ba, La, Ce, and W in human serum. The limits of detection for fivefold diluted serum were 0.18 (V), 0.229 (Cr), 0.050 (Mo), 0.328 (Ba), 0.031 (La), 0.038 (Ce), and 0.019 ng mL^–1 (W), respectively, and the relative standard deviations of the method were in the range 4–15% (2 ng mL^–1 in serum, n=3).     

Voltammetric study of glibenclamide at carbon paste and Sephadex-modified carbon paste electrodes

The oxidative behaviour of the antidiabetic agent glibenclamide on a bare carbon paste electrode (CPE) and a Sephadex-modified carbon paste electrode (SMCPE) was explored by cyclic and differential pulse voltammetry (DPV). The analysis procedure consisted of an open circuit accumulation step in stirred sample solution of Britton-Robinson buffer (0.04 mol L^–1, pH 2.0). This was followed by medium exchange to a clean solution of Britton-Robinson buffer (0.04 mol L^–1, pH 5.0), and subsequently an anodic potential scan was effected to obtain the voltammetric peak. The glibenclamide oxidation peak current obtained by DPV was proportional to the concentration of the glibenclamide in the range of 1.0×10^–9 mol L^–1 to 5.0×10^–8 mol L^–1 for 180 s accumulation time, with a detection limit of 4.0×10^–10 mol L^–1. A method was developed for the determination of glibenclamide in formulation and spiked human serum. Moreover, the proposed procedure was used to estimate the serum concentrations after oral administration of a 5 mg tablet of glibenclamide to three diabetic subjects.     

The International Conference on Harmonisation Guidance in Practice: Stress Degradation Studies on Lamivudine and Development of a Validated Specific Stability-Indicating HPTLC Assay Method

A sensitive, selective, precise and stability-indicating high-performance thin-layer chromatographic method of analysis of lamivudine both as a bulk drug and in formulations was developed and validated. The solvent system consisted of carbon tetrachloride – methanol – chloroform - acetonitrile (7.0: 3.0: 2.0: 1.5, v/v/v/v). Densitometric analysis of lamivudine was carried out in the absorbance mode at 275 nm. This system was found to give compact spots for lamivudine (R_F value of 0.36 ± 0.02) following double development of chromatoplates with the same mobile phase. Lamivudine was subjected to acid and alkali hydrolysis, oxidation, dry heat and wet heat treatment and photo degradation. The drug undergoes degradation under acidic, basic conditions, oxidation, wet heat and photo degradation. Also the degraded products were well resolved from the pure drug with significantly different R_F values. Linearity was found to be in the range of 50 – 1000 ng spot^–1 with significantly high value of correlation coefficient. The linear regression analysis data for the calibration plots showed good linear relationship with r² = 0.9994 ± 0.05 in the working concentration range of 300 ng spot^–1 to 1000 ng spot^–1. The mean value of slope and intercept were 0.11 ± 0.08 and 10.47 ± 1.21, respectively. The method was validated for precision, robustness and recovery. The limit of detection and quantitation were 15 ng spot^–1 and 40 ng spot^–1 respectively. As the method could effectively separate the drug from its degradation products, it can be employed as a stability indicating one. Moreover, the proposed HPTLC method was utilized to investigate the kinetics of acid degradation process. Arrhenius plot was constructed and activation energy was calculated.     

Difference spectrophotometric determination of some pharmaceutically important thioxanthene derivatives in dosage forms

A Spectrophotometric method is described for the rapid determination of four thioxanthene derivatives, namely chlorprothixene, thiothixene, flupenthixol hydrochloride and clopenthixol hydrochloride. The method is based on measuring the first derivative spectrum (D ₁) of the oxidized drug relative to a solution of the underivatized drug. At the wavelength of maximum difference in first derivative (range 285–315 nm), only the oxidation products have an appreciable difference in first derivative and the oxidizing agent has no absorbance. The oxidation products (assumed to be the thioxanthone sulphoxides) are formed rapidly at room temperature by the addition of peroxyacetic acid, prepared by the slow reaction of hydrogen peroxide and glacial acetic acid. The first derivative of the absorbance is proportional to the concentration of the drugs in solution over the ranges 2–14 g ml^–1 for chloroprothixene, 2–20 g ml^–1 for clopenthixol hydrochloride, 2–24 g ml^–1 for thiothixene and 4–40 g ml^–1 for flupenthixol hydrochloride. The method is specific for the intact drug and can be adopted in the presence of oxidative and photochemical decomposition products and tablet excipients. The recoveries ranged from 99.7 ± 1.3 to 100.2 ± 1.5%. The validity of the method was tested by analysing synthetic samples of thioxanthenes and some dosage forms containing the drugs; the results were in accordance with those given by the official methods.     

Simultaneous isolation of six fluoroquinolones in serum samples by selective molecularly imprinted matrix solid-phase dispersion

A simple and sensitive method for the simultaneous determination of six fluoroquinolones from serum samples was developed by selective molecularly imprinted matrix solid-phase dispersion (MI-MSPD) coupled with chromatographic separation. By using ethylene glycol dimethacrylate as crosslinker and reformative methanol–water system as reaction medium, the improved water-compatible imprinted polymers were synthesized which show higher affinity to template and its analogues in aqueous environment. The molecularly imprinted polymers (MIPs) were applied as the selective dispersant of matrix solid-phase dispersion (MSPD) could selectively extracted the six fluoroquinolones from serum, while interferences originated from serum matrices were eliminated simultaneously. Good linearity was obtained in a range of 0.05–100 μg mL⁻¹ with the correlation coefficients >0.999. The average recoveries of the six fluoroquinolones at four different spiked levels (0.25–10 μg mL⁻¹) were ranged from 72.2% to 114.1% with the relative standard deviations less than 6.6%. This method is simple and sensitive, and can be used as an alternative tool to the existing HPLC methods for analyzing the residues of fluoroquinolones in biological samples.     

Ion-pair adsorption film colorimetry of iron (III) in water samples and human serum

The anionic chelate of iron(III)-2,2-dihydroxyazobenzene (H₂L), [FeL₂]^–, formed 1 1 ion-pair with crystal violet cation (CV⁺), CV⁺ [FeL₂]^–, and was adsorbed on a surface of transparent polyvinyl chloride (PVC) film plasticized with di-n-octyl phthalate. Enrichment of the blue violet species of the ion-pair onto the transparent PVC film has enabled a highly sensitive and simple method for the determination of iron(III). The detection limits are 1 × 10^–8 mol dm^–3 (0.6 ppb) by spectrophotometry at 592 nm, and 4 × 10^–8 mol dm^–3 (2 ppb) by visual colorimetry. The method has been successfully applied to the determination of iron in water samples and human serum. No preparatory procedures for the separation of serum protein and other coexisting substances are required, since ion-pair adsorption process provides a new method to prevent interference of serum matrix.     

Polarographic behaviour and determination of beclomethasone dipropionate

The polarographic behaviour of beclomethasone dipropionate in Britton-Robinson buffers containing 40% methanol as a solubilizer has been studied. Over the pH range 1.8–12, a cathodic wave was produced, which was characterised as being irreversible, diffusion controlled and free from adsorption phenomena. The number of electrons involved in the reduction was found through comparative study with spironolactone. Using direct current polarographic mode, the limiting current concentration plot is rectilinear over the range 2.5 × 10^–5 to 4 × 10^–4 mol/1 with a detection limit of 2.5 × 10^–6 mol/1. A method has been developed for the determination of the drug in aerosols and creams, the results being in agreement with those obtained by the official method.     

Determination of ultra trace amounts of protein by 4-chlorosulfo-(2′-hyaroxylphenylazo)-rhodanine-Ti(IV) complex [ClSARP-Ti(IV)] as the fluorescence spectral probe in AOT microemulsion

Experiments indicated that protein can enhance the fluorescence of the 4-chlorosulfo-(2′-hydroxylophenylazo)-rhodanine-Ti(IV) complex [ClSARP-Ti(IV)] in the presence of bis(2-ethylhexyl)sulfosuccinate sodium salt (AOT) microemulsion. Based on this, a sensitive and reproducible fluorometric method for the determination of micro amount protein was developed. The calibration curves of four proteins were given. Under the optimum experimental conditions, the enhanced fluorescence intensity of the system was in proportional to the concentration of protein in the range of 0.1–11 μg mL⁻¹ for bovine serum albumin (BSA), 1.0–10 μg mL⁻¹ for human serum albumin (HSA), 1.0–50 μg mL⁻¹ for ovalbumin (Ova) and 2.5–18 μg mL⁻¹ for γ-globulins (γ-G). Their detection limits were 0.070, 0.071, 0.33 and 0.22 μg mL⁻¹, respectively. The ClSARP-Ti(IV) complex as a spectral probe can be used to the determination of protein in milk powder and oatmeal yielding with satisfactory results. Therefore, the proposed method is one of the most sensitive methods available. In addition, the interaction mechanism of this system is studied by multi-techniques.     

Determination of oxytetracycline in urine and human serum by differential pulse polarography

Summary A differential pulse polarographic method for the determination of oxytetracycline in urine and human serum in acid media (HClO₄ of pH 2) is proposed. The effects of the amount of sample taken and the concentration of HClO₄ present were investigated. The detection limit was 5.5×10^–6 mol/l. The standard deviation of the determination of 5.5×10^–5 mol/l of oxytetracycline in 2 ml of urine was 1.7×10^–6 mol/l and that of the determination of 5.5×10^–5 mol/l of oxytetracycline in 2 ml of human serum was 1.9×10^–6 mol/l.

---

Bestimmung von Oxytetracyclin in Urin und Humanserum durch Differential-Pulspolarography

     

Voltammetric behaviour and determination of moxifloxacin in pharmaceutical products and human plasma

The oxidative behaviour of moxifloxacin was studied at a glassy carbon electrode in different buffer systems using cyclic, differential pulse, and Osteryoung square-wave voltammetry. The oxidation process was shown to be irreversible over the entire pH range studied (2.0–10.0) and was diffusion-controlled. The methods were performed in Britton–Robinson buffer and the corresponding calibration graphs were constructed and statistical data were evaluated. When the proposed methods were applied at pH 6.0 linearity was achieved from 4.4×10^–7 to 1.0×10^–5 mol L^–1. Applicability to tablets and human plasma analysis was illustrated. Furthermore, a high-performance liquid chromatographic method with diode-array detection was developed. A calibration graph was established from 4.0×10^–6 to 5.0×10^–5 mol L^–1 moxifloxacin. The described methods were successfully employed with high precision and accuracy for estimation of the total drug content of human plasma and for pharmaceutical dosage forms of moxifloxacin.     

Fluorimetric determination of tetracycline and anhydrotetracycline

Summary A rapid fluorimetric method employing the complexes of Al³⁺ with tetracycline (TC) and anhydrotetracycline (ATC) has been used for the measurement of the concentrations of TC and ATC in about 10^–7–10^–6 mol/l. The assay offers simplicity and rapidly compared with other methods. The recoveries in the determination of synthetic samples are in the range of 95–103% for TC and 101–120% for ATC. Several determinations of TC and ATC in serum and urine have been carried out with satisfactory results.     

Spectrophotometric determination of some pharmaceutically-important aminoquinoline antimalarials

A simple and rapid spectrophotometric method for the assay of amodiaquine hydrochloride, chloroquine phosphate and primequine phosphate is described. The method is based on the interaction of the drug with tetracyanoethylene to give a stable charge transfer complex. The spectra of the complex show maxima at 413, 415 and 415nm, respectively, with high apparent molar absorptivities. Beer's law is obeyed in the concentration ranges 2–12, 1–8 and 2–12 g ml^–1 of the three drugs studied. The proposed method is applied to the determination of these drugs in certain formulations and the results are favourably comparable to the official methods.     

Development of an acetylene black–dihexadecyl hydrogen phosphate composite-modified glassy-carbon electrode,and its application in the determination of lovastatin in dosage drug forms

An electrochemical method has been established for the determination of lovastatin (LV). It is based on the enhanced oxidation of lovastatin at a novel acetylene black–dihexadecyl hydrogen phosphate composite-modified glassy-carbon electrode (AB–DHP/GCE) in the presence of Triton X-100. This electrode was prepared by dispersion of acetylene black particles in an aqueous suspension of DHP and the formation of a stable film of the resulting AB–DHP composite on the surface of a glassy carbon electrode (GCE). As a result of modification of the AB–DHP composite, the electrochemical response of lovastatin at GCE was apparently enhanced; this was apparent as amplification of the oxidation current and the negative shift of the oxidation potential. The oxidation current can be further increased in the presence of a trace amount of Triton X-100. The enhanced oxidation of lovastatin at AB–DHP/GCE was due to enlargement of the effective electrode area, catalysis of lovastatin oxidation by AB, and accumulation of lovastatin at the hydrophobic surface of the DHP layer, which would be enhanced by the coherence with Triton X-100. The effects of some working conditions on the oxidation current of lovastatin were tested and the calibration plot was examined. The result showed that the oxidation current was a linear function of lovastatin concentration in the range 2.5×10^–8–1.0×10^–6 mol L^–1 and a low detection limit of 4.0×10^–9 mol L^–1 was obtained under optimum conditions. This electrode system was applied to the determination of lovastatin in dosage drug forms and the results were in accordance with the ultraviolet–visible spectroscopy method.     

A study on terbium sensitized chemiluminescence of ciprofloxacin and its application

A novel rapid flow injection method with chemiluminescence (CL) detection was established for the determination of ciprofloxacin (CPLX), which is an antibiotic commonly used. The method is based on CL of Ce(IV)–SO₃²⁻ sensitized by Tb³⁺–CPLX, and showed the intensive bands characteristic of Tb³⁺ (⁵D₄→⁷F₅). The optimum conditions for CL emission were investigated. The linear relationship between the relative CL intensity and the concentration of CPLX is in the range of 9.0×10⁻⁹–1.0×10⁻⁶ mol/l with a detection limit of 3.1×10⁻¹⁰ mol/l. The relative standard deviation is 2.8% (n=11) for a level of 5.0×10⁻⁸ mol/l. The method was applied to the analysis of CPLX in human serum and urine samples with satisfactory results. The possible mechanism for this sensitized CL reaction is also discussed.     

Simplified Solid-Phase Extraction Procedure and Liquid Chromatographic Determination of Celecoxib in Rat Serum

A simplified solid phase extraction method, eliminating a preliminary protein precipitation has been developed for the determination of celecoxib in rat plasma. The technique included a solid phase extraction of the serum samples on a [poly (divinylbenzene-co-N-vinylpyrrolidone)] sorbent. After conditioning, the cartridge was loaded with 0.5 mL of acidified serum containing internal standard. Elution was made with 1 mL of a mixture of acetonitrile and methanol (1/1, v/v). After evaporation of the eluate to dryness and reconstitution with methanol, the samples were analyzed on an octadecyl bonded phase with several mobile phases containing acetonitrile and a phosphate buffer. Detection was carried out using a Photodiode Array Detector. Full validation of the proposed method was provided (linearity range: 0.01–2 mg. L^–1, average extraction efficiency: 92.4%; average intra-day variability: 4.6% with an accuracy of 94.8%; average interday variability: 5% with an accuracy of 95.3%, limit of detection: 0.005 mg. L^–1, limit of quantification: 0.002 mg. L^–1). The proposed method was successfully utilised to quantify celecoxib in rat plasma for a pharmacokinetic study.Revised: 26 January and 23 April 2004     

Ion chromatographic determination of iodide in urine and serum using a tubular ion-selective electrode based on a homogeneous crystalline membrane

The use of a laboratory-made iodide ion-selective electrode with tubular configuration and based on a crystalline membrane (AgI/Ag₂S) as the detector for ion chromatographic determination of iodide in urine and serum is described. A CIS reversed-phase column was coated withN-cetylpyridinium chloride to prepare a low-exchange-capacity analytical column and with hexadecyltrimethylammonium bromide to prepare a concentrator pre-column. A 2.0 ml min^–1 flow rate of deionized water and 0.1 mol 1^–1 KNO₃ solution was used for the pre-concentration and for the chromatographic separation, respectively. For optimum performance of the detector a background level of iodide was added into the column effluent. A linear relationship (r = 0.9997) between tubular electrode potential (as peak height) and iodide concentration in the range 5–400 g 1^–1 and a detection limit of 1.47 g 1^–1 were obtained. The method shows good reproducibility for both peak height (2.2% RSD) and retention time (1.3% RSD). Recoveries on its application to the samples were 93.0–100.9% for urine and 91.4–106.0% for serum.