Determination of terbinafine in pharmaceuticals and dialyzates by capillary electrophoresis

A capillary electrophoresis method has been developed for the separation and determination of terbinafine (TER) in various pharmaceutically relevant matrices. Capillary zone electrophoresis (CZE) separation and UV absorbance photometric detection were carried out in a 160 mm capillary tube with a 300 μm i.d., hydrodynamically (membrane) closed. The influences of pH, carrier cation and counterion on migration parameters of TER were studied and the following conditions were selected: a 20 mmol l⁻¹ glycine running buffer adjusted to pH 2.7 with acetic acid, 0.2% (w/v) methylhydroxyethylcellulose (m-HEC) as an electro-osmotic flow (EOF) suppressor, a 250 μA driving current, and 20 °C. The optimized separation conditions were convenient for the determination of TER in commercial tablets and spray and in dialyzates. Here, the dialysis was used to investigate in vitro permeation of TER through the skin from the gel. The samples of dialyzates were examined with and without simple extraction procedure and the results were compared. A permeation profile of the drug present in the gel of given composition was obtained analyzing pretreated samples. The proposed electrophoretic method was successfully validated. It was suitable for the simple, sensitive, rapid and highly reproducible assay of TER. CZE analysis was completed within 5.5 min. The detection limit of TER was 1.73 μmol l⁻¹ at a 224 nm detection wavelength. The intra- and inter-laboratory precisions over the concentration range 6.0-60.0 μmol l⁻¹ were between 0.32-0.69% and 1.04-1.44% including R.S.D. of migration times and peak areas, respectively. The mean absolute recoveries of drugs from samples were found to be 98.34 (tablets) and 99.47% (spray). It is suggested that there are potentialities to determine TER present in unpretreated complex samples, as CZE in a hydrodynamically closed separation system may be easily on-line combinable with purification and preconcentration CE modes (e.g., isotachophoresis, ITP).     

Determination of terbinafine (Lamisil) in human hair by microbore liquid chromatography/tandem mass spectrometry

An analytical method for the determination of terbinafine (Lamisil(R)) in human hair was developed and validated. Human hair (10 mg) was hydrolyzed in 0.50 mL of 5.0 N sodium hydroxide for 1.5 h. The aqueous layer was extracted with 1.5 mL of n-hexane. The organic layer was separated and re-extracted with 0.20 mL of formic acid (12.5%)/2-propanol (85:15, v/v). The aqueous layer was separated and 0.010 mL of the aqueous extract was injected onto a reversed-phase microbore (50 x 1.0 mm i.d.) column for analysis by liquid chromatography/tandem mass spectrometry (LC/MS/MS). The instrument was equipped with an electrospray ionization (ESI) interface and operated in the positive ion mode of detection. Interday and intraday accuracy and precision were assessed from the relative recoveries of spiked samples analyzed on three different days. The method showed excellent specificity and ruggedness with a lower limit of quantitation of 10 ng/g (i.e., 10 ppb) using 10 mg of human hair.     

Determination of hydroxyproline in tissues and the evaluation of the collagen content of the tissues

The concentrations of hydroxyproline (an amino acid specific of collagen) in a number of connective tissues were determined. Two procedures were compared. In one of them, amino acids were preseparated by chromatography and then determined on a standard amino acid analyzer. In the other procedure, hydroxyproline was selectively oxidized without amino acid separation and determined by a spectrophotometric reaction with Ehrlich’s reagent. Data obtained for purified collagen preparations in accordance with the two procedures were consistent with each other. The results can be somewhat different in unpurified preparations and tissues because of the presence of polysaccharide components in the tissues.     

Determination of neomycin in animal tissues by liquid chromatography

Tissue samples are digested under hot alkaline conditions after initial conditioning at room temperature with phosphate-buffered saline. The cooled digest is deproteinated with concentrated perchloric acid. After centrifugation and pH adjustment, the clear supernatant is applied to an ion-exchange cartridge, and after the cartridge is washed, the neomycin is eluted with dilute perchloric acid. This eluate is derivatized with 9-fluorenylmethyl chloroformate prior to liquid chromatography using a wide-pore spherical silica C4 column and fluorescence detection. Recovery and repeatability are calculated from tissue extract standard calibration curves produced from the same assay. Recoveries ranged from 80 to 120% for fortifications of 0.25-1.00 mg/kg for muscle tissue and from 80 to 100% for fortifications of 0.50-10.0 mg/kg for kidney tissue. Limits of quantitation were 0.25 and 0.50 mg/kg, respectively, for muscle and kidney tissues. Limits of detection were 0.125 and 0.20 mg/kg, respectively, for muscle and kidney tissues.     

Determination of dehydrodiisoeugenol in rat tissues using HPLC method

Dehydrodiisoeugenol (DDIE) is a bioactive neolignan from the seeds of Myristica fragrans Houtt., which exhibits good anti-inflammatory activity. A rapid and simple high-performance liquid chromatographic (HPLC) method has been developed for the determination of DDIE in rat tissues after intravenous administration. The tissue samples were processed by liquid-liquid extraction. The analyses were successfully carried out on a Diamonsiltrade mark ODS C18 column (250 x 4.6 mm i.d., 5 microm) equipped with a C18 guard column (8 x 4.6 mm i.d., 5 microm). The mobile phase was the system of methanol-water (4:1, v/v). The UV detection was set at 270 nm. The calibration curves were linear from 0.4 to 200.0 microg/g with the correlation coefficients (r(2)) greater than 0.998. The intra- and inter-day precisions in quality control samples were less than 10% and the accuracies were in the range 85.4-110.3%. The average recoveries from all the tissues were between 84.4 and 106.0%. This assay method has been successfully used to study the tissues distribution of DDIE in rats after intravenous administration. The result suggests that DDIE is distributed to rat tissues rapidly with possibly greater initial concentrations in liver and brain than in other tissues.     

Determination of selenium in human tissues by atomic absorption spectrometry

A simple method is described for the determination of selenium in human tissues without the use of perchloric acid. Digestion with nitric and sulphuric acids is followed by hydride generation and atomic absorption spectrometry. Results for NBS bovine liver and IAEA horse kidney reference materials were in good agreement with assigned concentrations, as was also achieved with the perchloric acid digestion. Recovery of added selenium was >90%, and the relative standard deviation was 5.5% for within-batch and 6.9% for between-batch analyses. The values of selenium in heart tissue were 0.9–1.3 μg g^?1 dry weight.     

Determination of vanadium in animal tissues by PIXE and AAS

Proton induced X-ray emission (PIXE) and atomic absorption spectroscopy (AAS) were used for vanadium determination in animal tissues. The vanadium concentration levels were determined in blood, kidneys and livers taken from rats. Two groups of the animals were treated with different diets. The diet for the first group was supplemented with vanadium compounds while the diet for the second one was assumed to be a normal diet. The second group was treated as control. In order to achieve the best minimum detectable limit (MDL)¹ the samples were subject to a special sample preparation procedure. Blood and kidneys were mineralized with an APDC compound. The mineralization process was performed according to the procedure described previously.² The application of PIXE³ is very useful for different types of samples. PIXE measurements were performed with a proton beam at the Institute of Nuclear Physics in Cracow, Poland while the AAS measurements were done at the Institute of Molecular Biology, Jagiellonian University, Poland. The concentration levels of vanadium in blood and kidneys are compared and discussed. There were no significant statistical differences between results of vanadium concentration levels determined by the abovementioned techniques. The PIXE technique had the advantage over the AAS technique of giving a broad spectrum of trace elements analyzed in a single measurement. Therefore with the help of sample preparation procedure the application of the PIXE method seems to be suitable for such analyzes.     

Determination of gallium in tumour-affected tissues by means of spectroscopic techniques

A comparative investigation was carried out on the suitability of atomic absorption spectrometry and of emission spectrography with arc and hollow-cathode excitation sources for determination of gallium (μg g^-1) in biological samples. The three methods give reliable results. Hollow-cathode emission spectrography was found to be influenced to a lesser extent by matrix effects and to be more precise than the other two techniques.     

OasisTM小柱用于腐败生物组织中吗啡检测的研究

应用新型亲水亲酯的Oasis^TM固相柱，并使用Zymark全自动固相萃取仪，检测了腐败生物组织中的吗啡。与传统的Cl8固相柱相比，Oasis^TM固相柱具有选择范围广、吸附能力强的特点，其方法操作简单、快速、重现性好及回收率高。所建立的方法适合大批量腐败生物检材的标准化分析测定，并已成功应用于一些案例的检测工作，取得了良好的效果。     

固相萃取-高效液相色谱法测定鱼组织中吡喹酮和克螨特残留

近年来,为了防治水产品中血吸虫、螨虫等寄生虫病,各种抗生素、抗菌素等渔药被广泛使用.吡喹酮(Praziquantel,PZQ)和克螨特(Propargite,CO-MIT)均是新型的高效、低毒、广谱的抗寄生虫药物,在水产养殖中被广泛应用于防治血吸虫、螨虫等寄生虫疾病,其中原本主要用于果树、蔬菜等农作物寄生螨类防治的克螨特由于防治效果好、成本低,近年来在国内外开始作为PZQ的渔药复配剂应用.由于水产养殖生产中渔药使用量、使用频次大、半衰期长,休药期短,而药物主要残留于可食用的动物肌肉、肝、肾中,这使得水产品药物残留和食品安全问题日趋严峻.为了研究PZQ和COMIT渔药复配剂对水产品养殖产生的影响,控制渔药在水产品中的残留,服务于生产,有必要建立一种简便有效的分离检测方法.     

Determination of elements in bovine tissues by instrumental neutron activation analysis

Instrumental neutron activation analysis was carried out to obtain the normal concentration of trace elements in bovine tissues (heart, liver, kidney, spleen, lymph nodes) and serum. Concentrations of 17 elements were determined. In this paper, concentrations of Al, Br, Cs, In and Rb are given and correlations of concentrations are discussed between Cl and Br and between K and Cs or Rb. Significant positive correlations have been found between Cl and Br concentrations in all tissues, between K and Cs concentrations in tissues excluding kidney, and between K and Rb concentrations in tissues excluding liver.     

气相色谱-质谱法同时检测动物组织中多种激素类兽药的残留量

建立了不同动物基质(肌肉、肝脏、肾脏)中己烷雌酚、己烯雌酚、己二烯雌酚、还原尿睾酮、表睾酮、雌酮、雌二醇、炔雌醇和雌三醇激素残留量的气相色谱-质谱联用(GC-MS)检测方法。以乙腈为提取溶剂,固相萃取柱净化,微波辅助衍生化,用双(三甲基硅烷基)三氟乙酰胺(BSTFA)与甲基氯硅烷(TMCS)(体积比为99 :1)的硅烷化试剂在吡啶存在下进行衍生化反应。实验结果表明,9种激素的检出限为0.1～1 μg/kg。3种动物基质中9种激素的平均回收率为68.8%～93.1%,实验室内相对标准偏差(RSD)为4.1%～22.3%,实验室间RSD为3.1%～17.9%。方法的技术指标满足动物组织中激素类兽药残留分析的要求。     

Determination of terbinafine in human plasma using UPLC–MS/MS: Application to a bioequivalence study in healthy subjects

A high‐throughput and sensitive ultra‐performance liquid chromatography–tandem mass spectrometry (UPLC–MS/MS) method has been developed for the determination of terbinafine in human plasma. The method employed liquid–liquid extraction of terbinafine and terbinafine‐d7 (used as internal standard) from 100 μL human plasma with ethyl acetate–n‐hexane (80:20, v/v) solvent mixture. Chromatography was performed on a BEH C₁₈ (50 × 2.1 mm, 1.7 μm) column using acetonitrile–8.0 mm ammonium formate, pH 3.5 (85:15, v/v) under isocratic elution. For quantitative analysis, MS/MS ion transitions were monitored at m/z 292.2/141.1 and m/z 299.1/148.2 for terbinafine and terbinafine‐d7, respectively, using electrospray ionization in the positive mode. The method was validated according to regulatory guidance for selectivity, sensitivity, linearity, recovery, matrix effect, stability, dilution reliability and ruggedness with acceptable accuracy and precision. The method shows good linearity over the tested concentration range from 1.00 to 2000 ng/mL (r² ≥ 0.9984). The intra‐batch and inter‐batch precision (CV) was 1.8–3.2 and 2.1–4.5%, respectively. The method was successfully applied to a bioequivalence study with 250 mg terbinafine in 32 healthy subjects. The major advantage of this method includes higher sensitivity, small plasma volume for processing and a short analysis time.     

Determination of210Pb and210Po in human tissues of Japanese

To determine the levels of²¹⁰Pb and²¹⁰Po in human tissues of people in Japan, various tissue samples were obtained at autopsy from the cadavers of 22 oncologic cases, mainly in Niigata Prefecture in northern Japan, from 1986 to 1988.Wet ashing, followed by electrochemical deposition and alpha spectrometry were used to separate and determine the²¹⁰Pb and²¹⁰Po present. Among the tissues analyzed, the highest concentrations of²¹⁰Pb and²¹⁰Po were observed in bone (sternum), liver, and kidneys. The total body burden of²¹⁰Pb and²¹⁰Po was found to be approximately 427 pCi and 514 pCi, respectively. This estimated²¹⁰Po value did not differ significantly from values found in populations in the U.S.A. and European countries.     

Determination of vinca alkaloids in mouse tissues by high-performance liquid chromatography.

A high-performance liquid chromatographic method is described for the determination of vinblastine in various normal mouse tissues, such as lung, heart, liver, kidney and muscles, and in implanted MO4 tumours. Vincristine was used as the internal standard. Freshly obtained mouse tissue or tumour tissue was frozen at -20 degrees C and then lyophilized. After lyophilisation, the dry tissues were pulverized and homogeneously mixed, and an aliquot was suspended in 0.1 M hydrochloric acid. The drugs of interest were then isolated from this suspension using ion-pair extraction at pH 3 with octylsulphate as counter-ion. The obtained extracts were analysed on a reversed-phase system with a cyanopropyl stationary phase. The detection limit was 1 ng/l in plasma and 10 ng/g in tissue. The extraction recoveries of vincristine and vinblastine were between 45 and 67%, and there were no interferences from blank components. Preliminary pharmacokinetic data for different mouse tissues and tumour implanted in muscle tissue are presented.