Polarography of disodium pentacyanonitrosylferrate(II): Part 2. Determination at Therapeutic Levels in Serum,Plasma, and Whole Blood

Disodium pentacyanonitrosylferrat(II) (sodium nitroprusside) is determined at therapeutic (ng ml^?1) levels in plasma, serum and blood with conventional and high-performance differential pulse polarography (d.p.p. and h.p.d.p.p.) at a dropping mercury electrode or a static mercury drop electrode. Serum or plasma (3 ml) is treated with perchloric acid containing 1 mg ml^?1 potassium hexacyanoferrate(II), centrifuged for 10 min and subjected to polarography. For spiked serum, calibration graphs are linear over the range 30–1000 ng ml^?1 sodium nitroprusside, regardless of the polarographic technique; the estimated detection limit is 15 ng ml^?1 (5 × 10^?8 M). Calculated therapeutic levels range from 100 to 1000 ng ml^?1. Similar results were obtained for spiked plasma. A similar procedure is suitable for whole blood and was used to study the in-vitro degradation of sodium nitroprusside (200 ng ml^?1) on incubation at 37°C. The in-vitro loss is rapid (t_{$\text{1}\text{2}$} ≈ 6 min) but meaningful in-vivo levels can be obtained when the blood is collected in a 0.9% sodium chloride solution at 0°C. Thiocyanate, the main metabolite of nitroprusside, and thiosulphate, which is a potential antidote for cyanide, do not interfere.     

Determination of Arsenic and Phosphorus in Doped Polysilicon Layers

Abstract

The method is based on polysilicon dissolution with a water-hydrofluoric-nitric acid etchant mixture followed by matrix volatilization as hexafluorosilicic acid. Losses of arsenic through volatilization are avoided by its oxidation with permanganate. Phosphorus is determined by the molybdenum blue method with direct addition of a mixed reagent to the residue. Spectrophotometric evaluation at 882 nm provides a detection limit of 10 ng P ml^?1 with a precision better than 3%. Arsenic is determined by reducing As(V) to electroactive As(III) on addition of sulphite in 2 M hydrochloric acid. Differential-pulse polarography of this solution provides a precision of 2% and a detection limit of 20 ng As ml^?1.     

Dosage direct du paracetamol dans les milieux biologiques par polarographie sinusoidale

(The direct determination of paracetamol in biological fluids by a.c. polarography). Paracetamol can be determined rapidly in biological fluids (blood serum and urine) by a.c. polarography. After elimination of protein by perchloric acid, followed by reaction with nitrous acid in acidic medium, the nitro derivative is measured at pH 10. As little as 4 × 10^-6 M paracetamol (0.6 μg ml^-1) in serum can be determined.     

Determination de la Silice Par Polarographie en Courant Alternatif en Milieu Nitrate

Abstract

In 1 M ammonium nitrate supporting electrolyte, alternating current polarography of the α and β forms of molybdosilic acids yielded a single common peak. That peak provides a means for the determination of silicon in silicate solutions. The dynamic range of the method extends from 0.6 to 20 μg.mL^?1 of silicon.     

Electrochemical Behaviour of Loprazolam and its Determination in Pharmaceutical Formulations

Abstract

The electrochemical behaviour of Loprrzoiam has been determined in aqueous solution at 37 > Cusing DC polarography, differential pulse polarography and voltammetry and linear sweep cyclic voltammetry. Loprazolam can be quantitavely determined up to 3.9 10^?6 M at pH 6.5 using DP polarography, the detection limit being established at 1.6 10^?7 M. The method developed was applied to the determination of the compound in its formulations, Somnovit 1 mg, obtaining errors lower than 4%.     

Colorimetric Determination of Propofol in Bulk form,Dosage Form and Biological Fluids

ABSTRACT

Propofol is coupled with 2, 6-dichloroquinone-4-chlorimide (DCQ) in a reaction buffered at pH 9.6 to give a colored product having an analytically useful maximum at 635 nm. The factors affecting the color generation were optimized and incorporated in the procedure. The reacted propofol has a molar absorptivity of 3.9 × 10^?4 L mol^?1 cm^?1, and Beer's law is obeyed for concentrations 1-5 μg ml^?1 with detection limit 0.25 μg ml^?1. The method was found applicable to biological fluids (plasma and urine) spiked with propofol at concentration levels 1-5 μg ml^?1 for plasma and 1-5 μg 0.5 ml^?1 urine (less sensitivity is obtained with urine volumes above 0.5 ml) with detection limits 0.28 μg ml^?1 for plasma and 0.4 μg 0.5 ml^?1 urine. The average recovery for the commercial preparation (1% w/v propofol emulsion intravenous injection for infusion) was 99.54% with an RSD of 1.05%. The method was validated by an adopted HPLC method. The results obtained by the HPLC method for the commercial preparation were statistically compared with the proposed method and evaluated at the 95% confidence limits.     

Determination of tin in the ng g−1 range differential pulse polarography

A sensitive determination method of tin by differential pulse polarography is described. Addition of tropolone to acetate supporting electrolyte at about pH 4.7 provides a 30-fold signal enhancement, giving a sensitivity comparable to that obtained in anodic stripping voltammetry, but without the need for enrichment by pre-electrolysis. The response is linear over more than three orders of magnitude (1 ng ml^?1?5 μg ml^?1 Sn), allowing measurements within a wide concentration range without changes in sample preparation or measuring conditions. Large amuonts of Ti, W, Cr or Mo interfere, but can be removed completely by pre-separation of tin based on extraction with tropolone/toluene and back-extraction into the supporting electrolyte. Results for tin in water and fruit juice are consistent with those obtained by other techniques.     

Etude Polarographique De La Marcellomycine

Abstract

Polarographic study of marcellomycine.

d.c., a.c. and d.p. polarography and cyclic voltammetric techniques were used to investigate the electrochemical properties of marcellomycine. These are found to be quite similar to those of aclacinomycine or carminomycine, the main reversible two-electron wave being attributed tot he reduction of the quinonic structure. The molecule undergoes a degradation process starting in acidic medium and giving rise to the formation of two small irreversible waves at more negative potentials. This process is time, illumination and pH dependent. Important adsorption phenomena interfere in the investigated pH range but are lowered in very acidic medium. Quantitative measurements have been carried out at pH 1 and 6 in a 10^?3 to 10^?5 M concentration range using d.c. polarography. d.p. technique allows determinations in a restricted 10^?5 to 10^?4 M range. A detection limit of 1 · 10^?5 M has been fixed at pH 1.     

Kinetic Spectrophotometric Determination of Vanadium (V) Based on its Inhibitory Effect on the Thionine – Ascorbic Acid Reaction

ABSTRACT

A simple and sensitive kinetic method for the determination of vanadium(V) based on its inhibitory effect on the reduction of thionine by ascorbic acid at pH=5 is described. The reaction rate is monitored spectrophotometrically by measuring the decrease in absorbance of thionine at 598 nm after a fixed time (10 min). The calibration graph is linear in the range of 10 ? 120 ng ml^?1 of vanadium(V) and the detection limit is 6 ng ml^?1. The relative standard deviation (RSD) for 80 ng ml^?1 of V(V) was 0.96% (n=10). The method was successfully applied to the determination of vanadium in a certified reference sample.     

Differential pulse polarographic determination of cyanuric chloride

Cyanuric chloride (2,4,6-trichloro-1,3,5-triazine) can be determined by fastscan differential pulse polarography in methanolic acetate buffer solution at pH 5.6 at a hanging mercury drop electrode. At positive potentials, the insoluble salt formed between cyanuric chloride and mercury(I) is adsorbed on the mercury surface and the d.p.p. current is enhanced. The detection limit is 0.2gmg ml^?1. Cyanuric chloride in air can be determined after absorption in methanol.     

Ion-Associates of Alkaloids and Synthetical Psychopharmaca With Cresol Red.

Abstract

Ethylmorphine, morphine, codeine, cocaine, sernyl (PCP), LSD, 3-quinuclidinyl benzilate (BZ) provide, together with Cresol Red, ion-associates that are extractable by chloroform. The extracts of the ion-associates prove the absorption maxima in the interval 405 to 415 nm. Maximum extraction of the analytes of the ion-associates is reached after 4 minutes, taking readings of different pH values in 4 intervals of 1.5. This method allows detect of alkaloids and synthetical psychopharmaca row of quantities between 0.45 μg.ml^?1 and 1.55 μg.ml^?1 and to determine 1.05 μg.ml^?1 to the amount 2.99 μg.ml^?1 of the analytes in the aqueous solutions.     

FLOW - Injection Determination of Traces of Sulfide by the Brilliant Green - Sulfide Reaction with Spectrophotometry Detection

Abstract

A flow injection system is proposed for the rapid and sensitive determination of trace amounts of sulfide based on the addition reaction of sulfide with Brilliant Green at pH 7 and 25 C°. The effect of important parameters, such as reagent concentration, pH, reagent flow rate, sample volume, temperature and length of the reaction coil are reported. Sulfide in the range of 40 - 2000 ng·ml^?1 can be determined at a rate of 40 ± 5 samples per hour. The limit of detection was obtained as 2.0 ng of sulfide. The relative standard deviation for the determination of 100 ng·ml^?1 of sulfide is 0.8%. A system is proposed for elimination of potential interferences. The method was applied to the determination of sulfide in synthetic samples and in spring water.     

Spectrophotofluorimetric Determination of Trace Amounts of Aluminium with 2,2′-Dihydroxy-3,3′-dicarboxy-1, 1′-Dinaphthylmethane (Pamoic Acid)

Abstract

Fluorescence properties of 2,2′-dihydroxy-3,3′-dicarboxy -1,1′-dinaphthylmethane (pamoic acid) and of its aluminium 1:1 complex are described. The fluorescence of the latter, as measured from a water-dioxane (3:7, v/v) solution, at pH 5.05–5.20, at room temperature, is used as a basis for a new method of aluminium determination at submicrogram level. Limit of quantification of the proposed procedure is 0.028 ng.ml^?1, range of applicability goes up to 1.7 ug.ml^?1, RSD is 1% at 0.47 ug.ml^?1 level (concentrations, given refer to HCl solution which is measured) Tolerance ratios for several interferent metal ions are given. A comparison is made with Kirkbright's method which uses 3-hydroxy-2-naphthoic acid as complexing agent: stability with time of the readings and freedom from Fe(III) interference are the main advantages of the proposed procedure. The new method is applied to the aluminium determination in atmospheric aerosol samples.     

Determination of Methimazole and Carbimazole Using Polarography and Voltammetry

Abstract

Anodic waves of methimazole (I) (1-methylimidazole-2-thiol) and carbimazole (II) (1-ethoxycarbonyl-3-methyl-2-thio-4-imidazoline) on mercury electrodes correspond to mercury salt formation. Both compounds form in the thiono form a soluble complex at pH < 6, compound (I) at higher pH-values a slightly soluble salt of the thiol form. Electrode processes involving the thiol form are complicated by adsorption. Oxidation at solid electrodes occurs only at potentials more than 0.5 V more positive. For compound (I) spectrophotometry indicated pK_a=12.0 ± 0.2. By d.c. polarography in 0.1 M H₂SO₄ containing 10% ethanol the determination of both compounds is possible between 4 × 10^? and 1 × 10^?3 M, by differential pulse polarography between 1 × 10^? and 1 × 10^?4 M, by differential pulse voltammetry at HMDE between 5 × l0^?7 and 6 × 10^? M.     

Fluorescent Complexes of Nucleic Acids/8-Hydroxyquinoline/Lanthanum(III) and the Fluorometry of Nucleic Acids

Abstract

The ternary fluorescent complexes of nucleic acids/8-hydroxyquinoline/ lanthanum (III) were studied. Nucleic acids in the study involve natured and thermally denatured calf thymus DNA, fish sperm DNA and yeast RNA. In the range of pH 8.0–8.4 (controlled by NH₃-NH₄Cl buffer) ternary fluorescent complexes are formed which emit at 485.0 nm for calf thymus DNA and at 480.0 nm for yeast RNA (when excited at 267.0 nm) and emits at 483.0 nm for fish sperm DNA when excited at 265.0 nm. Based on the fluorescence reactions sensitive fluorometric methods for nucleic acids were proposed. Using optimal conditions, the calibration curves were linear in the range of 0.4–3.6 μg˙ml^?1 for calf thymus DNA, 0.4–4.0 μg-ml^?1 for fish sperm DNA and 0.4–4.0 μg˙ml^?1 for yeast RNA, respectively. The limits of determination (3σ) were 0.076 μg˙ml^?1 for calf thymus DNA, 0.068 μg˙ml^?1 for fish sperm DNA and 0.329 μg˙ml^?1 for yeast RNA, respectively. Five synthetic samples were determined with satisfaction.

     

Cyclodextrin Enhanced Spectrofluorimetric Determination of Melatonin in Pharmaceuticals and Urine

ABSTRACT

Melatonin forms a 1:1 inclusion complex with methyl-β-cyclodextrin with an association constant of 139 ? 30 M^?1 at 20 °C. The effect of several cyclodextrins and derivatives on the fluorescence spectra of melatonin was studied with a great increase of fluorescence signal when methyl-β-cyclodextrin was employed. Optimal conditions of the method were: [methyl-β-cyclodextrin] = 0.01 M and temperature 20 °C; the pH does not affect the luminescence emission. The linear dynamic range (LDR) was 50-3000 ng ml^?1 and a limit of detection of 10 ng ml^?1 of melatonin was obtained with a relative standard deviation (RSD) of 0.77% (at 0.3 μg ml^?1 level). This simple method was satisfactorily applied to the determination of melatonin in pharmaceutical preparations and urine.     

Determination of Steroids in Human Urine by Micellar Liquid Chromatography

Abstract

A simple and sensitive method for the determination of steroids using micellar liquid chromatography is described. The steroids, including hydroxycorticosterone. corticosterone, northisterone, testosterone, mexdroprogesterone acetate and progesterone, were separated by reversed-phase using a micelles mobile phase following UV detection at 245 nm. The parameters affecting retention of the test solutes such as the concentration of sodium dodecyl sulfate (SDS) and n-butanol-1 in the mobile phase were investigated. It was found that the retention of the solutes was dependent on the composition of mobile phase. The linear calibration plots range from 0.1 to 10 μg ml^?1 in mobile phase containing 5.0 × 10^?2 mol l^?1 SDS/9 % n-butanol-1 at pH 6.0, and the detection limit in order of 0.1 μg ml^?1 was obtained. The proposed method was used for the determination of steroids in urine using direct injection of samples without previous treatment.     

2-(2-Thiazolylazo)-p-cresol(TAC) as a Reagent for the Spectrophotometric Determination of Lead(II)

Abstract

The reaction between lead(II) and 2-(2-Thiazolylazo)-p-Cresol(TAC) in the presence of TERGITOL NPX (4 mg/ml) at an apparent pH 9.0–10.0 results in an intensely colored complex which is stable for at least 4 hr.

The composition of the complex is 1:2 cation: TAC and the log of the formation constant is 11.92 ± 0. 40. Beer's law is obeyed up to 6.0μg.ml^?1 of lead(II) at 650nm.

The apparent molar absorptivity at 650 nm is 2.07 × 10⁴ 1. mole^?1.cm^?1 and the detection limit was obtained as 10.0 ng.ml^?1 of lead(II).

The method is applied to determination of lead(II) in copper-base alloy.     

Direct Spectrophotometric Determination of Calcium in Human Serum and Cerebrospinal Fluids with Amino G Acid Chlorophosphonazo

ABSTRACT

A novel spectrophotometric method based on amino G acid chlorophosphonazo (AGCPA) has been developed for measuring calcium in human serum and cerebrospinal fluids. The effects of experimental factors including pH, reagent concentrations, and interfering species on calcium determinations were investigated. In a neutral reaction media of pH 7.0, AGCPA reacts rapidly with calcium to form a stable and greenish blue complex, whose absorption maximum is at 670 nm. The molar absorptivity (?) of the complex is 7.2x10⁴ 1 mol^?1cm^?1, and the molar ratio of calcium to AGCPA in the complex is found to be 1:2. Beer's law is obeyed over the range 0.02-0.8 μg ml^?1 of calcium. No interferences were observed from the commonly coexisting species present in serum and cerebrospinal fluids. Compared to the reported and currently often used methods based on o-cresolphthalein complexone, arsenazo III and methylthymol blue, the proposed method in this work provides better analytical characteristics such as high sensitivity, good selectivity and neutral reaction media. In addition, the present method is simple and can be applied to the direct determination of calcium in human serum and cerebrospinal fluid samples with satisfactory results.     

Pyrocatechol-1-Aldehyde 2-Benzothiazolylhydrazone As Reagent for the Spectrofluorimetric Determination of Nanogram Amounts of Gallium in Urine and Blood Serum

Abstract

A method is developed for the spectrofluorimetric determination of 1–80 ng.ml^?1 of gallium with pyrocatechol-1-aldehyde 2-benzothiazolylhydrazone, in a 50% (v/v) DMSO-Water medium at apparent pH 4.0 (monochloracetic/monochloracetate buffer). Λ_ex = 400nm, Λ_em = 504 nm (corrected). Interferences have been evaluated and the method applied to the determination of gallium in human urine and blood serum samples.