Simultaneous determination of histamine and spermidine by second-derivative synchronous fluorescence spectrometry

The method is based on formation of the fluorescent condensation products with o-phthaldialdehyde; 0.5–2000 ng ml^?1 histamine and 3–700 ng ml^?1 spermidine can be quantified, with relative standard deviations of 2–3%. Histamine/spermidine ratios of 2.5:1–1:30 can be handled. A selectivity study is reported.     

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 trace levels of heavy metals in waters by extraction with ammonium tetramethylenedithiocarbamate and hexamethyleneammonium hexamethylenedithiocarbamate into xylene followed by inductively-coupled plasma emission spectrometry

The determination of Cd, Co, Cr, Cu, Fe, Mn, Mo, Ni, Pb, V and Zn in river and sea water by inductively-coupled plasma emission spectrometry after extraction with a mixture of ammonium tetramethylenedithiocarbamate (APDC) and hexamethyleneammonium hexamethylenedithiocarbamate into xylene is described. All these elements are simultaneously concentrated 100-fold in a single extract and directly introduced into the plasma. The pH dependences of the extraction and the stabilities of the complexes are reported. The limits of detection of the method range from 0.017 ng ml^?1 (cadmium) to 0.5 ng ml^?1 (lead). With 100-fold concentration factors, calibration graphs are linear up to 30 ng ml^?1 or more.     

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.     

2-(α-pyridyl)thioquinaldinamide: a novel fluorimetric reagent in inorganic trace analysis. : Part 2. A simple selective determination of selenium(IV) at Ultratrace Levels

The very sensitive fluorimetric determination of selenium(IV) is based on its oxidation of the non-fluorescent 2-(α-pyridyl)thioquinaldinamide in slightly acidic solution (0.05–0.15 M sulphuric acid). The excitation and emission wavelengths are 350 nm and 500 nm, respectively. Linear calibration graphs are obtained for different ranges of selenium concentration between 0.01 ng ml^?1 and 0.5 μg ml^?1. Over sixty ions either do not interfere or can be masked in the determination of 1 ng ml^?1 Se(IV). The method is applied successfully to various synthetic mixtures and to a native sulphur sample. The reaction is fast and the fluorescent system is stable for 24 hours.     

Flame atomic absorption spectrometric determination of Cd(II), Ni(II), Co(II) and Cu(II) in tea and water samples after simultaneous preconentration of dithizone loaded on naphthalene

A simultaneous preconcentration procedure for the determination of Cd(II), Ni(II), Co(II) and Cu(II) by atomic absorption spectrometry is described. The method is based on solid phase extraction of the metal ions on dithizone loaded on naphthalene in a mini-column, elution with nitric acid and determination by flame atomic absorption spectrometry. The sorption conditions including NaOH concentration, sample volume and the amount of dithizone were optimized in order to attain the highest sensitivity. The calibration graph was linear in the range of 0.5–75.0 ng ml^?1 for Cd(II), 1.0–150.0 ng ml^?1 for Ni(II), 1.0–150.0 ng ml^?1 for Co(II) and 1.0–125.0 ng ml^?1 for Cu(II) in the initial solution. The limit of detection based on 3S_b was 0.13, 0.32, 0.33 and 0.43 ng ml^?1 for Cd(II), Ni(II), Co(II) and Cu(II), respectively. The relative standard deviations (R.S.D) for ten replicate measurements of 20 ng ml^?1of Cd(II), 100 ng ml^?1 of Ni(II), Co(II) and 75 ng ml^?1 of Cu(II) were 3.46, 2.43, 2.45 and 3.26%, respectively. The method was applied to the determination of Cd(II), Ni(II), Co(II) and Cu(II) in black tea, tap and river water samples.     

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.     

1,2-Diamino-4,5-ethylenedioxybenzene as a highly sensitive fluorogenic reagent for aromatic aldehydes

1,2-Diamino-4,5-ethylenedioxybenzene is shown to be a highly sensitive reagent for aromatic aldehydes, especially for benzaldehydes having a hydroxy group. The reagent reacts selectively with aromatic aldehydes at pH 3.0 (phosphate buffer) within 30 min at 60°C; the products fluoresce most intensely at pH 11. In the manual method, the lower limits of detection vary from 6 pmol ml^?1 to 7 nmol ml^?2. The fluorescent derivatives of aromatic aldehydes can be separated by reversed-phase high-performance liquid chromatography. The fluorescent product from 4-hydroxybenzaldehyde is shown to be 2-(4-hydroxyphenyl)-5,6-ethylenedioxybenzimidazole.     

Inductively-coupled plasma atomic emission spectrometric determination of boron based on generation of methyl borate

Boron is converted to methyl borate, distilled and condensed, and selectively volatilized at 50°C into the plasma without interference from methanol, which quenches the plasma. The 3σ detection limit is 40 ng ml^?1 boron, the calibration graph is linear up to 10 μg ml^?1 and the r.s.d. 3.0% for 2.0 μg ml^?1 (n = 10). Boron is determined in plant-tissue and steel standards.     

Determination of prednisolone and prednisone in plasma by liquid chromatography with fluorescence detection

After a single-step extraction from plasma (250 μl) with dichloromethane, the drugs and dexamethasone (internal standard) are oxidized by copper(II) acetate to the corresponding glyoxal and converted into the fluorescent quinoxalines by reaction with 1,2-diamino-4,5-methylenedioxybenzene. The quinoxalines are separated within 55 min by reversed-phase liquid chromatography with isocratic elution. The detection limits for prednisolone and prednisone added to plasma are 3 ng ml^?1 in plasma (signal-to-noise ratio=3).     

The double radio-isotope derivative technique for the assay of drugs in biological material: Part II. The simultaneous determination of opipramol and its deshydroxyethyl metabolite

The neuroleptic drug opipramol and its deshydroxyethyl metabolite can be determined simultaneously in the same biological sample. Known amounts of ¹⁴C-labelled opipramol and ¹⁴C-labelled metabolite are added to the sample to serve as internal standards. After suitable extraction, both compounds are acetylated by ³H-labelled acetic anhydride. Together with μg-amounts of carrier compounds, the O-acetyl derivative of opipramol and the N-acetyl derivative of the metabolite are purified and separated by two-dimensional thin-layer chromatography. Each of the derivatives is isolated and counted for ¹⁴C-and ³H-activity. The ¹⁴C-activities recovered serve to determine the overall yield of the opipramol and metabolite, and to convert the measured ³H-activity to 100 % theoretical yield. From analyses of standard samples, the specific ³H-activities of the acetyl derivatives were calculated, and these values were used to convert the measured ³H-activities from biological samples to concentrations of original opipramol and metabolite. For both compounds the standard deviations of blank samples were ±1 ng ml^?1. For concentrations up to 100 ng ml^?1 the standard deviation was ±3 ng ml^?1.     

Spectrophotometric Catalytic Determination of Trace Amounts of Selenium Based on the Reduction of Azurea by Sulphide

ABSTRACT

A sensitive catalytic kinetic spectrophotometric method for determining ng ml^?1 concentrations of selenium is described. The method, based on the catalytic effect of Se (IV) on the reduction of azureA by sulphide, is monitored spectrophotometrically at 600 nm. The linearity range of the calibration graph is dependent on the concentration of sulphide. The variables affecting the rate of the reaction were investigated and the optimum conditions were established. The method is simple, rapid, precise, sensitive, free from many interferences and is widely applicable. The limit of detection is 2.5ng ml^?1 of Se. The relative standard deviation of seven determinations of 100 ng ml^?1 Se was 1.5%. The method was applied to the determination of selenium in spiked water, Kjeldahl tablets, synthetic samples and health care products.     

Enhancement of ruthenium determination by inductively coupled plasma/atomic emission spectrometry by addition of periodic acid

A sensitive method for the determination of ruthenium involving the formation of volatile species in solution and subsequent nebulization for inductively coupled plasma/atomic emission spectrometry is proposed. The sensitivity of the determination of ruthenium was increased by a factor of 70 with the addition of 1×10^?2 M periodic acid as an oxidizing agent. The detection limit was 5 ng ml^?1 of ruthenium and the calibration was linear over the range 0.01–0.5 μg ml^?1 of ruthenium. Serious interferences were not found except from reducing agents.     

Determination of Biacetyl by Sensitized Photochemical Kinetic Fluorimetry

Abstract

A new in-situ photochemical kinetic fluorimetric method was proposed for the determination of biacetyl (BI). It is based on the sensitization of BI on the photochemical reaction of amaranth (AM). AM, a nonfluorescent compound was converted into an intensively fluorescent compound in a slightly alkaline medium by the sensitized photochemical reaction, and BI was indirectly determined by monitoring the change of the fluorescence intensity. The determination can be carried out by fixed-time method or tangent method. The kinetic behavior of the reaction and the effects of some experimental conditions were investigated and discussed. The calibration graph was rectilinear from 1.0 μg ml^?1 to 10.0 μg ml^?1 of BI (r = 0.999), the limit of detection was 1.0 ng ml^?1, and the coefficient of variation was 0.44% for 0.90 μg ml^?1 of BI (n = 6). The mechanism for the sensitization of BI was examined and the triplet-triplet energy transfer, in which BI acted as the energy donor and AM as the energy acceptor, was suggested to be the main cause. Its application to real samples has been tested.     

Determination of mitomycin C in human blood plasma and urine by high-performance differential pulse polarography

High-performance differential pulse polarography is used for determining the antitumor antibiotic mitomycin C in human blood plasma and urine. The limit of determination (2-ml samples) is 25 ng ml^?1 when the substance is isolated by means of Amberlite XAD-2, and 200 ng mo_?1 when samples are not pretreated. The method was applied in a pharmacokinetic experiment; no metabolites of mitomycin C were observed in urine or plasma.     

Determination of urinary chromium levels for healthy men and diabetic patients by electrothermal atomic absorption spectrometry

Urinary chromium levels for healthy and diabetic men were determined by direct graphite-furnance atomic absorption spectrometry. The average values were 0.72 ± 0.31 ng ml^?1 for 23 healthy men aged 23 to 35, 0.39 ± 0.19 ng ml^?1 for 19 healthy men aged 47 to 69, and 1.0 ± 0.9 ng ml^?1 for 23 diabetic patients aged 13 to 79. Some urines of diabetic patients exhibit values > 1.3 ng ml^?1, which are never found in healthy men. The proposed method involves direct injection of 20 μl of urine inot a pyrolytically-coated graphite tube, and a standard addition calibration procedure involving a pooled urine sample. The results are compared with those obtained by a liquid-liquid extraction method.     

Determination of uranium in marine sediment pore waters by isotope dilution inductively coupled plasma mass spectrometry

Inductively coupled plasma mass spectrometry (ICP-MS) was used in an isotope dilution mode to assay small-volume (0.25 ml) sediment pore waters for their uranium contents, using ²³⁶U as the spike. The only pretreatment required was a simple dilution by a factor of 20, which gave sufficient volume for three replicate analyses per sample. Rapid and accurate results were obtained for a variety of samples and standards, ranging in concentration from 0.05 to 10 ng U ml^?1. A suite of 30 samples can be analysed in less than 6 h by this method. The relative standard deviation was better than 1.9%, with a detection limit, based on 3σ background, of 2 pg U ml^?1 in solution (40 pg ml^?1 in samples). Sea water is a difficult matrix for ICP-MS and thus the method is generally suitable for uranium determinations in many other sample solutions.     

Extraction-spectrofluorimetric determination of cadmium with diethyldithiocarbamate and calcein in non-aqueous media

Cadmium (7–80 ng ml^?1) is extracted with diethyldithiocarbamate into chloroform from aqueous media, at pH 11–12 and the fluorescent complex is developed by addition of a calcein solution in dimethylformamide. The method is applied to the determination of cadmium in waste waters, high-purity metals and zinc ores.     

Direct determination of biacetyl in fats by sensitized room temperature phosphorescence

A direct method for the determination of biacetyl in butter and margarine by sensitized room temperature phosphorescence (SRTP) is described. After dissolution of the sample in hexane, biacetyl is isolated by distillation, and its native phosphorescence is sensitized by a non-polar linear furocoumarin, 4′5′-dihydro-3-carbethoxypsoralen. The limit of detection is 0.05 ng ml^?1 biacetyl, with a linear response from 1 × 10^?4 to 1 μg ml^?1 (r = 0.999). The RSD is 3.5% at 100 ng ml^?1.     

Indirect determination of fluoride in waters with lanthanum alizarin complexone and inductively-coupled plasma emission spectrometry

Fluoride is determined indirectly by measurement of the La II 333.75-nm line in the lanthanum/alizarin complexone/fluoride complex. The ternary complex is extracted into hexanol containing N,N-diethylaniline and the extract is introduced directly into the plasma. Related to water samples, the detection limit (3σ, concentration factor 5) is 0.59 ng ml^?1 fluoride, calibration is linear up to 1.2 μg ml^?1 and the relative standard deviation for 0.04 μg ml^?1 is 2.6%. Alkali, alkali elements and most anions do not interfere. The method is applied in the analysis of river water, coastal seawater and drinking water.