Characterization and identification of ascorbyl methylsilanol pectinate for cosmetic formulations application

The ascorbyl methylsilanol pectinate (AMP) presents the same functional properties of ascorbic acid (AA). Besides antioxidant and depigmentant activity, the AMP presents silanol in its chemical structure. The aim of this work was to characterize and indentify the AMP alone and in cosmetic formulations. The following techniques were employed: Fourier Transform Infrared Spectrophotometry, particle size distributions, in vitro antioxidant activity with 2.2-diphenyl-1-picrylhydrazyl (DPPH) and Oxigen Radical Absorbance Capacity Assay and High Performace Liquid Chromatography (HPLC) (developed and validated method) for the active ingredient; Microscopy, HPLC and Normal Stability Assay (NSA) for the emulsions. Particle size distributions results showed that the average size of AMP was 1.0 µm and polydispersity index was 0.1. In DPPH assay AA and AMP were statistically the same. The value of ORAC obtained for AMP was 0.74 and for AA in the literature was 0.95. In the NSA the formulations were stable in conditions of 5.0 and 45.0 ± 2.0 ºC for 90 days. Adequate stability at ambient temperature out of reach of light was also observed. Thus, this works presented an acceptable method for quantification of AMP alone and in cosmetic formulations. AMP was an adequate choice for the incorporation in emulsions with antioxidant efficacy.

Simultaneous determination of abamectin homologs H 2 B 1a and H 2 B 1b in gel formulation by high performance liquid chromatography

ABSTRACT Abamectin is a drug with antiparasitic properties used in several pharmaceutical formulations. The objective of this research was to develop and validate a high performance liquid chromatographic (HPLC) method for quantification of the two abamectin homologs (H2B1a and H2B1b) in gel formulation. This HPLC method was validated using a LichroCart(r) 100 RP-18 (125 x 4 mm, 5 µm) column. The mobile phase contained of acetonitrile and water (95:5 v/v) with 1% acetic acid. The flow rate was 1.0 mL min-1 and UV detection was performed at 245 nm. Mobile phase solutions were prepared containing a nominal concentration 185.2 µg mL-1 H2B1a and 9.6 µg mL-1 H2B1b. The method displayed good linearity in the concentration range of 148.1 - 222.3 µg mL-1 and 7.7 - 11.5 µg mL-1, for H2B1a and H2B1b, respectively, with a correlation coefficient of (r)> 0.99 for both compounds, calculated by the least mean squares method. Detection limits (DLs) were 2.8 µg mL-1 and 1.2 µg mL-1 and quantitation limits (QLs) were 8.6 µg mL-1 and 3.8 µg mL-1, for H2B1a and H2B1b, respectively. The method is simple, economical and efficient for the quantitative determination of abamectin H2B1a and H2B1b homologs in pharmaceutical preparations.

Simultaneous determination of ethinyl estradiol and drospirenone in oral contraceptive by high performance liquid chromatography

A simple, rapid, economical and reliable high performance liquid chromatographic method has been developed and successfully applied in simultaneous determination of ethinyl estradiol and drospirenone in coated tablets. The HPLC method was performed on a LiChroCART® 100RP column (125x4 mm i.d., 5 µm) with acetonitrile:water 50:50 (v/v) as mobile phase, pumped at a flow rate of 1.0 mL.min-1. The fluorescence detection for ethinyl estradiol was made at λex= 280 nm and λem= 310 nm and a UV detection for drospirenone was made at 200 nm. The elution time for ethinyl estradiol and drospirenone were 4.0 and 5.7 min, respectively. The method was validated in accordance to USP 34 guidelines. The proposed HPLC method presented advantages over reported methods and is suitable for quality control assays of ethinyl estradiol and drospirenone in coated tablets.

Um método simples, rápido, econômico e confiável foi desenvolvido empregando a cromatografia líquida de alta eficiência para a determinação simultânea de etinilestradiol e drospirenona em comprimidos revestidos. O método foi realizado utilizando coluna LiChroCART® 100RP (125 x 4 mm d.i., 5 µm), a fase móvel constituída de acetonitrila:água, 50:50 (v/v) com vazão de 1,0 mL.min-1. A detecção foi realizada empregando fluorescência em λex= 280 nm e λem= 310 nm para o etinilestradiol e na região de UV em 200 nm para a drospirenona. O etinilestradiol e a drospirenona tiveram tempo de retenção de 4,0 e 5,7 min, respectivamente. O método foi validado de acordo com as diretrizes da USP 34. O método proposto apresentou vantagens sobre os relatados na literatura e pode ser considerado adequado para o controle de qualidade do etinilestradiol e da drospirenona em comprimidos revestidos.

Stability evaluation of tocopheryl acetate and ascorbyl tetraisopalmitate in isolation and incorporated in cosmetic formulations using thermal analysis / Estabilidade de avaliação de acetato de tocoferol e ascorbil tetraisopalmitato isoladamente e incorporados em formulações de cosméticos por meio de análise térmica

In view of the increase in the number of cosmetic preparations containing antioxidant vitamins, chiefly, due to their action in preventing the process of skin aging, there is a need to develop pre-formulation studies and to validate analytical methods in order to obtain high quality products. Thus, the objective of this research was to evaluate and compare the thermal behavior of tocopheryl acetate and ascorbyl tetraisopalmitate as raw materials, and incorporated into a base cream. Thermogravimetry (TG / DTG) and differential scanning calorimetry (DSC) were used for this purpose. Both vitamins were found to be stable up to 250ºC. The base cream (placebo) and the sample (base cream containing the vitamins) presented different weight loss. Thermal analysis has shown itself to be an excellent tool for the characterization of these vitamins and can be used in routine analysis for quality control of this type of cosmetic formulation.

Considerando o potencial antioxidante das vitaminas utilizadas em produtos cosméticos, seu uso na prevenção do processo de envelhecimento da pele e a necessidade de estudos de pré-formulação que garantam o desenvolvimento de cosméticos de qualidade, foi objetivo deste trabalho avaliar e comparar o comportamento térmico dos ativos acetato de tocoferila e tetraisopalmitato de ascorbila, matérias-primas, isoladamente e incorporados em creme base. As técnicas termogravimetria/termogravimetria derivada (TG/DTG) e calorimetria exploratória diferencial (DSC) foram utilizadas para tal finalidade. Verificou-se que as vitaminas mantiveram-se estáveis até a temperatura de, aproximadamente, 250 ºC, observando-se diferença na perda de massa entre o creme base e o creme base associado às vitaminas. Assim sendo, a análise térmica mostrou-se como excelente ferramenta para caracterização das vitaminas e do creme base, podendo ser empregada em análises de rotina no controle de qualidade deste tipo de formulação cosmética.

Determination of atropine enantiomers in ophthalmic solutions by liquid chromatography using a Chiral AGP column.

Many therapeutic agents are commercialized under their racemic form. The enantiomers can show differences in the pharmacokinetic and pharmacodynamic profile. The use of a pure enantiomer in pharmaceutical formulations may result in a better therapeutic index and fewer adverse effects. Atropine, an alkaloid of Atropa belladonna, is a racemic mixture of l-hyoscyamine and d-hyoscyamine. It is widely used to dilate the pupil. To quantify these enantiomers in ophthalmic solutions, an HPLC method was developed and validated using a Chiral AGP column at 20 degrees C. The mobile phase consisted of a buffered phosphate solution (containing 10 mM 1-octanesulfonic acid sodium salt and 7.5 mM triethylamine, adjusted to pH 7.0 with orthophosphoric acid) and acetonitrile (99 + 1, v/v). The flow rate was 0.6 ml/min, with UV detection at 205 nm. In the concentration range of 14.0-26.0 microg/mL, the method was found to be linear (r > 0.9999), accurate (with recovery of 100.1-100.5%), and precise (RSD system < or = 0.6%; RSD intraday < or = 1.1%; RSD interday < or = 0.9%). The method was specific, and the standard and sample solutions were stable for up to 72 h. The factorial design assures robustness with a variation of +/- 10% in the mobile phase components and 2 degrees C of column temperature. The complete validation, including stress testing and factorial design, was studied and is presented in this research.

Development and validation of sensitive methods for determination of sibutramine hydrochloride monohydrate and direct enantiomeric separation on a protein-based chiral stationary phase.

Sibutramine hydrochloride monohydrate, chemically 1-(4-chlorophenyl)-N,N-dimethyl-alpha-(2-methylpropyl) hydrochloride monohydrate (SB.HCI.H20), was approved by the U.S. Food and Drug Administration for the treatment of obesity. The objective of this study was to develop, validate, and compare methods using UV-derivative spectrophotometry (UVDS) and reversed-phase high-performance liquid chromatography (HPLC) for the determination of SB.HCI.H20 in pharmaceutical drug products. The UVDS and HPLC methods were found to be rapid, precise, and accurate. Statistically, there was no significant difference between the proposed UVDS and HPLC methods. The enantiomeric separation of SB was obtained on an alpha-1-acid glycoprotein column. The R- and S-sibutramine were eluted in < 5 min with baseline separation of the chromatographic peaks (alpha = 1.9 and resolution = 1.9).

Development and validation of a method for quantitative determination of econazole nitrate in cream formulation by capillary zone electrophoresis.

A simple, fast, inexpensive and reliable capillary zone electrophoresis (CZE) method for the determination of econazole nitrate in cream formulations has been developed and validated. Optimum conditions comprised a pH 2.5 phosphate buffer at 20 mmol L(-1) concentration, +30 kV applied voltage in a 31.5 cm x 50 microm I.D. capillary. Direct UV detection at 200 nm led to an adequate sensitivity without interference from sample excipients. A single extraction step of the cream sample in hydrochloric acid was performed prior to injection. Imidazole (100 microg mL(-1)) was used as internal standard. Econazole nitrate migrates in approximately 1.2 min. The analytical curve presented a coefficient of correlation of 0.9995. Detection and quantitation limits were 1.85 and 5.62 microg mL(-1), respectively. Excellent accuracy and precision were obtained. Recoveries varied from 98.1 to 102.5% and intra- and inter-day precisions, calculated as relative standard deviation (RSD), were better than 2.0%. The proposed CZE method presented advantageous performance characteristics and it can be considered suitable for the quality control of econazole nitrate cream formulations.

Quantitative determination of dimethylaminoethanol in cosmetic formulations by nuclear magnetic resonance spectroscopy.

A nuclear magnetic resonance (NMR) spectroscopic method was validated for the quantitative determination of dimethylaminoethanol (DMAE) in cosmetic formulations. The linearity in the range from 0.5000 to 1.5000 g (DMAE salt/mass maleic acid) presents a correlation coefficient > 0.99 for all DMAE salts. The repeatability (intraday), expressed as relative standard deviation, ranged from 1.08 to 1.44% for samples and 1.31 to 1.88% for raw materials. The detection limit and quantitation limit were 0.0017 and 0.0051 g for DMAE, 0.0018 and 0.0054 g for DMAE bitartrate, and 0.0023 and 0.0071 g for DMAE acetamidobenzoate, respectively. The proposed method is simple, precise, and accurate and can be used in the quality control of raw materials and cosmetic gels containing these compounds as active substances.

Comparative study on two rapid and sensitive methods for quantitative determination of tenoxicam in tablets

Tenoxicam, a piroxicam analogue, is an NSAID (Non-Steroid Antinflamatory Drug). It is used in the symptomatic management of musculoskeletal and joint disorders such as osteoarthritis and rheumatoid arthritis, and also in the short-term management of soft-tissue injury. Its quantitative determination in pharmaceutical formulations is important to guarantee the desired therapeutic effects. The objective of this research was to develop, validate and compare spectrophotometric and chromatographic methods in the quantitative determination of tenoxicam in tablet preparations. In this work, tablets containing 20.0 mg of tenoxicam from different origins were analyzed. The spectrophotometric method was validated using 0.1 mol/L NaOH as solvent and a signal at 368 nm was taken. The HPLC method was validated using Synergi Hydro-RP® C18 column (250x4.6 mm, 4 µm). The mobile phase was constituted of methanol-water (61:39 v/v) with pH adjusted to 2.5 with formic acid, at a flow rate of 1.0 mL/min. UV detection was made at 375 nm. All analyses were performed with a column temperature of 25 ºC ± 1. The calibration curves were linear over a concentration range from 4.0-24.0 µg/mL with a correlation coefficient better than 0.9999. The detection limit (DL) and quantitation limit (QL) were 0.25 µg/mL and 0.90 µg/mL for UV method and 0.35 µg/mL and 1.20 µg/mL for HPLC method respectively. The intra-day and inter-day precision expressed as RSD were below 2 percent for both methods. The mean recovery of tenoxicam was found to be in the range of 98.5-101.25 percent for UV method and 99.01-101.93 percent for HPLC method. The UV and HPLC methods were found to be rapid, precise and accurate. Statistically there was no significant difference between proposed UV spectrophotometric and HPLC methods.

Tenoxicam, um análogo de piroxicam, é um AINE (Antiinflamatório Não-Esteróide). ë usado no tratamento sintomático de doenças musculoesqueléticas das juntas, tais como osteoartrite e artrite reumatóide, e, também, no tratamento de danos dos tecidos moles. Sua determinação quantitativa em formulações farmacêuticas é importante para garantir os efeitos terapêuticos desejados. O objetivo dessa pesquisa foi desenvolver, validar e comparar métodos espectrofotométrico e cromatográfico na determinação quantitativa de tenoxicam em comprimidos. Neste trabalho, comprimidos contendo 20,0 mg de tenoxicam de diferentes procedências foram analisados. O método espectrofotométrico foi validado utilizando-se 0,1 mol/L de NaOH como solvente e se obteve sinal a 368 nm. O método por CLAE foi validado utilizando-se coluna Synergi Hydri-RP® C18 (250x4,6 nm, 4µm). A fase móvel constitui-se de metanol-água (61:39 v/v), com pH ajustado para 2,5 com ácido fórmico, e velocidade de fluxo de 1,0 mL/minuto. A detecção por UV foi efetuada a 375 nm. Todas as análises foram realizadas com temperatura de coluna a 25 ºC ± 1. As curvas de calibração foram lineares na faixa de concentração de 4,0 a 24,0 µg/mL, comcoeficiente de correlação melhor que 0,9999. O limite de detecção (LD) e o limite de quantificação (LQ) foram 0,25 µg/mL e 0,90 µg/mL e 1,20 µg/mL por CLAE, respectivamente. A precisão intra e inter-dia, expressa como RSD, foi abaixo de 2 por cento para ambos os métodos. A média de recuperação do tenoxicam ficou na faixa de 98,5 a 101,25 por cento para o método de UV, e 99,01 a 101,93, para a CLAE. Os métodos de UV e de CLAE mostraram-se rápidos, precisos e exatos. Estatisticamente, não se observou diferença significativa entre os métodos espectrofotométricos (UV) e CLAE.

Determination of optimum wavelength and derivative order in spectrophotometry for quantitation of hydroquinone in creams

UV derivative spectrophotometry was used for quantitative determination of hydroquinone in creams. The aim of this work was to investigate optimum wavelength and order of derivative, and to validate the proposed spectrophotometric method. The results of standard curves were calculated and statistically analyzed through the least squares method in the interval from 10.0 to 26.0 µg/mL, in the first, second, third and fourth order derivatives. The quantitative determination was carried out by using the zero-crossing (Z-C) and zero-peak (Z-P) methods. The proposed method is simple, of low cost and provides reliable results in order to be used in quality control of creams containing hydroquinone as active substance.

A espectrofotometria derivada no UV foi usada para a determinação quantitativa de hidroquinona em cremes. O objetivo desta pesquisa foi investigar o melhor comprimento de onda e a ordem da derivada, bem como validar o método proposto. Os resultados das curvas analíticas foram analisados estatisticamente pelo método dos mínimos quadrados no intervalo de 10,0 a 26,0 µg/mL, na primeira, segunda, terceira e quarta ordens da derivada. As determinações quantitativas foram realizadas utilizando os métodos "zero-crossing (Z-C)" e zero-pico (Z-P). O método proposto é simples, de baixo custo e fornece resultados confiáveis podendo ser usado no controle de qualidade de cremes contendo hidroquinona como substância ativa.

Quantitative determination and sampling of azathioprine residues for cleaning validation in production area.

Cleaning validation is an integral part of current good manufacturing practices in any pharmaceutical industry. Nowadays, azathioprine and several other pharmacologically potent pharmaceuticals are manufactured in same production area. Carefully designed cleaning validation and its evaluation can ensure that residues of azathioprine will not carry over and cross contaminate the subsequent product. The aim of this study was to validate simple analytical method for verification of residual azathioprine in equipments used in the production area and to confirm efficiency of cleaning procedure. The HPLC method was validated on a LC system using Nova-Pak C18 (3.9 mm x 150 mm, 4 microm) and methanol-water-acetic acid (20:80:1, v/v/v) as mobile phase at a flow rate of 1.0 mL min(-1). UV detection was made at 280 nm. The calibration curve was linear over a concentration range from 2.0 to 22.0 microg mL(-1) with a correlation coefficient of 0.9998. The detection limit (DL) and quantitation limit (QL) were 0.09 and 0.29 microg mL(-1), respectively. The intra-day and inter-day precision expressed as relative standard deviation (R.S.D.) were below 2.0%. The mean recovery of method was 99.19%. The mean extraction-recovery from manufacturing equipments was 83.5%. The developed UV spectrophotometric method could only be used as limit method to qualify or reject cleaning procedure in production area. Nevertheless, the simplicity of spectrophotometric method makes it useful for routine analysis of azathioprine residues on cleaned surface and as an alternative to proposed HPLC method.

Cromatografia líquida com fase quiral aplicada na separação enantiomérica de fármacos cardiovasculares / Applied chiral phase liquid chromatography in enantiomeric separation of cardiovascular drugs

A maioria dos agentes terapêuticos, freqüentemente prescritos, é formulada e comercializada sob a forma racêmica, embora, para alguns deles, já tenha sido demonstrado que os efeitos farmacológicos e/ou tóxicos estejam relacionados apenas a um dos enantiômeros. Além disso, é conhecido o fato de que os enantiômeros podem apresentar perfis farmacocinéticos e farmacodinâmicos diferentes. Neste trabalho foram selecionados compostos que fazem parte de um importante grupo de fármacos muito empregados na terapêutica. São fármacos freqüentemente prescritos em doenças cardiovasculares. As separações enantioméricas diretas do atenolol, betaxolol, metoprolol e nadolol foram obtidas utilizando-se fase estacionária quiral do tipo carbamato de celulose tris-3,5-dimetilfenil, Chiralcel OD®, (250 x 4.6 mm, 10 æm). Os enantiômeros do pindolol foram separados com fase estacionária quiral derivada de dinitrobenzoil (DNB), a-Burke 2®, (250 x 4.6 mm, 10 æm). Os fármacos foram cromatografados à temperatura ambiente, com volume de injeção de 20 æL. A detecção foi efetuada em 276 nm exceto para o pindolol, que foi detectado em 220 nm. Os métodos propostos neste trabalho empregando CLAE-FEQs oferecem vantagens sobre as técnicas clássicas de separação de enantiômeros e podem ser empregados na análise quantitativa dos enantiômeros em preparações farmacêuticas e amostras biológicas.

The majority of frequently prescribed therapeutic agents are formulated and commercialized in the racemic form, even though, for some of them, it has already been demonstrated that the pharmacological and/or toxicological effects are associated only with one of the enantiomers. Moreover, it is well known that these antipodes can present different pharmacokinetic and pharmacodynamic profiles. In this work we selected drugs that belong to an important group of pharmaceuticals, frequently prescribed in the treatment of cardiovascular disorders. The direct enantiomeric separations of atenolol, betaxolol, metoprolol and nadolol were obtained using the chiral stationary phase cellulose tris-3,5-dimethylphenyl-carbamate, Chiralcel OD® (250 x 4,6 mm, 10 æm). The enantiomers of pindolol were separated with the chiral stationary phase derived from dinitro-benzoyl (DNB) (S, S) alpha-Burke 2® (250x4.6 mm, 10 æm). The drugs were chromatographed at room temperature, with injection volumes of 20 æL. The detention was made at 276 nm except for pindolol, which was detected at 220 nm. The proposed methods in this work using HPLC-CSP offer advantages over contemporaneous techniques of enantiomeric separation, being rapid and efficient, and can be used in the simultaneous quantitative analysis of referred enantiomers in pharmaceutical preparations and biological samples.

First-derivative ultraviolet spectrophotometric and high performance liquid chromatographic determination of ketoconazole in pharmaceutical emulsions

Foram desenvolvidos e padronizados métodos por espectrofotometria no ultravioleta (UV) por derivada de primeira ordem (Método I) e cromatografia líquida de alta eficiência (CLAE) (Método II) para a determinação quantitativa de cetoconazol em formulações farmacêuticas sob a forma de emulsão obtida no comércio e formulada em laboratório. A espectrofotometria no UV por derivada de primeira ordem foi padronizada usando-se o método do zero pico a 257 nm, utilizando metanol como solvente. A cromatografia líquida foi realizada empregando-se uma coluna LiChrospher® 100 RP-18 (5 µm). A fase móvel utilizada foi a mistura de trietilamina em metanol (1:500) e solução de acetato de amônio em água (1:200) na proporção de 75:25 v/v, com vazão de 1 mL/min e detecção no UV de 225 nm. O tempo de retenção do cetoconazol foi de 3,9 min e do terconazol de 5,9 min, este último utilizado com padrão interno. As curvas analíticas mostraram linearidade dentro das concentrações de 5,0 a 30,0 µg/mL para o Método I e 20,0 a 80,0 µg/mL para o Método II, com coeficientes de correlação linear de 0,9997 e 0,9981, respectivamente.O desvio padrão relativo (DPR) foi de 0,56% e 0,41% para a amostra simulada e comercial, respectivamente, empregando-se o Método I. Para o Método II, os valores foram de 2,13% e 1,25%, respectivamente. A porcentagem de recuperação foi de 100,1% para o Método I e 100,4% para o Método II. Os excipientes não interferiram nas análises. Os resultados mostraram que os dois métodos podem ser usados para a determinação rápida de cetoconazol em formulações de emulsões com precisão, exatidão e especificidade.

Determination of alpha-hydroxy acids in cosmetic products by capillary electrophoresis.

In this work, a simple and reliable method for the simultaneous analysis of alpha-hydroxy acids such as tartaric, glycolic and lactic acids in cosmetic products was developed using capillary electrophoresis with indirect UV detection at 254 nm. A buffer solution containing 10 mmoll(-1) potassium phthalate (pH 4.1) and 0.5 mmoll(-1) cetyltrimethylammonium bromide as electroosmotic flow modifier allowed baseline resolution of the analytes in approximately 3 min. A few validation parameters of the proposed method include: good linearity for all compounds in the range from 10 to 100 mgl(-1) with coefficients of correlation larger than 0.9999. The average recoveries of tartaric, glycolic and lactic acids in commercial samples were 99.12, 99.41 and 99.43%, respectively. The method presented acceptable precision with average relative standard deviation of 0.54% (assay of commercial samples), 0.44% (peak area) and 0.16% (migration time).

Validação de um método analítico para a determinação de substâncias ativas em formulações farmacêuticas empregadas em ®peelings¼ químicos / Validation of analytical methods for the determination of active substances in pharmaceutical preparations used in chemical peelings

Nos "peelings" químicos utilizam-se formulações esfoliantes, empregadas na terapêutica de queratoses actínicas, rugas, discromias pigmentares, acne vulgar e rosácea. Na presente pesquisa, foram empregadas como amostras, a solução de Jessner (SJ) composta por resorcinol (RS) 14 por cento e ácido láctico (AL) 14 por cento em solução alcoólica e géis de AS a 20 por cento e RS a 30 por cento. As técnicas utilizadas foram a espectrofotometria derivada no UV de primeira e segunda ordens em etanol absoluto para o AS e RS, respectivamente na SJ, e a espectrofotometria derivada no UV de primeira ordem em ácido sulfúrico 0,1 N para o AS e RS nos géis. Para o AS na SJ, o coeficiente de correlação (r) foi de 0,9999, a precisão expressa pela média dos desvios padrão relativos (DPR) de 0,68 por cento e a exatidão expressa pela recuperação média de 100,5 por cento...

Determination of sun protection factor (SPF) of sunscreens by ultraviolet spectrophotometry

The aim of this research was to determine the sun protection factor (SPF) of sunscreens emulsions containing chemical and physical sunscreens by ultraviolet spectrophotometry. Ten different commercially available samples of sunscreen emulsions of various manufactures were evaluated. The SPF labeled values were in the range of 8 to 30. The SPF values of the 30 por cento of the analyzed samples are in close agreement with the labeled SPF, 30 por cento presented SPF values above the labeled amount and 40 por cento presented SPF values under the labeled amount. The proposed spectrophotometric method is simple and rapid for the in vitro determination of SPF values of sunscreens emulsions

Eletroforese capilar: teoria e aplicaçöes na análise de medicamentos / Capillary electrophoresis: theory and applications in drug analysis

Como quase todas as boas idéias, a eletroforese capilar (CE) é fácil e eficiente. O equipamento é constituído por componentes simples e perfeitamente controlados, proporcionando a reprodutibilidade e a confiabilidade requeridas para a validação dos métodos analíticos empregados no controle de qualidade de medicamentos. Para muitas moléculas importantes, a CE proporciona ótimos resultados quando comparada com outras técnicas. Para a separação de alguns compostos com estruturas muito complexas, tais como princípios ativos altamente polares, enantiômeros e compostos básicos, a CE oferece vantagens muito significativas em relação à cromatografia a líquido de alta eficiência. A CE permite, ainda, fácil validação de ensaios quantitativos para determinação de traços de impurezas, assim como para a determinação quantitativa de vários compostos em fluidos biológicos

Acido glicólico: agente despigmentante e rejuvenescedor / Glycolic acid: depigmenting agent and rejuvenating

A pigmentaçäo da pele, causada pela irradiaçäo da luz ultravioleta, como defesa contra a açäo carcinogênica da luz solar, pode levar ao envelhecimento precoce da pele e a uma hipercromia, cujo tratamento requer o uso de fotoprotetores, despigmentantes e rejuvenescedores. Recentemente, têm sido usadas várias substâncias para previnir e/ou tratar o envelhecimento cutâneo, bem como para diminuir a pigmentaçäo da pele. O hidroxiáxido mais comumente empregado em preparaçöes cosméticas e dermatológicas tem sido o ácido glicólico, pelas propriedades despigmentantes e rejuvenescedoras e pela eficácia que apresenta, em diferentes concentraçöes, quando incorporado a vários tipos de excipientes.

Identificação do amido de milho por espectroscopia no infravermelho próximo / Corn starch identification through near infrared spectroscopy

Utilizou-se a espectroscopia no infravermelho próximo (Near Infrared Spectroscopy - NIR) para o estabelecimento de um método de identificação para o amido de milho. Para tal, criou-se um banco de dados contendo espectros no NIR da substância e utilizou-se o mesmo como referência para a qualificação de novos lotes do material. O banco de dados formado (biblioteca) foi validado para uso de acordo com os parâmetros de correlação e distância conforme estabelecido pelo ®software¼, NSAS, módulo IQ², do espectrofotômetro. O método elaborado mostrou-se simples, rápido e eficiente, podendo-se otimizar os processos de controle de qualidade através da sua aplicação devido à redução de tempo e, conseqüentemente, de custos

Determination of acetylsalicylic acids in effervescent tablets by high performance liquid chromatography and UV-multicomponent spectrophotometry

The simultaneous determination of acetylsalicylic acid (ASA) and its degradation product, salicylic acid (SA) in effervescent tablets by high performance liquid chromatography (HPLC) and UV-multicomponent spectrophotometric (MCS) methods is described. In HPLC method, the analytes were extracted with a mixture of acetic acid and methanol (1:99v/v) and aliquots of these solutions appropriately diluted were injected on a reversed-phase C-18 column using a mobile phase consisting of methanol, water and acetic acid, isocratic elution and detection at 283nm. Recoveries ranging from 98.43 to 101.48 por cento and from 99.13 to 102.80 por cento were obtained from commercial samples for ASA and SA, respectively. Relative standard deviations ranged from 0.94 to 1.31 por cento for ASA and from 1.83 to 2.50 por cento for SA. In MCS method, a mixture of acetic acid and chloroform (1:99v/v) was used as solvent. Analyte solutions were measured at 280 and 310nm. Recoveries ranging from 98.30 to 102.02 por cento and from 98.50 to 103.20 were obtained from commercial samples for ASA and SA, respectively. Relative standard deviations ranged from 0.40 to 0.73 por cento for ASA and from 0.86 to 0.93 por cento for SA. Results were compared statistically by F and t tests. On the basis of precision, accuracy, time saving and economy, MCS method was found to show advantages over the HPLC method and can be applied for routine analysis of commercial samples in quality control laboratories.