Utility of Derivative Spectrophotometry in the Determination of Carbochromen Hydrochloride and Dipyridamole in the Presence of Their Oxidative Degradation Products

Abstract

Direct spectrophotometric methods for the determination of carbochromen hydrochloride and dipyridamole, each in the presence of its oxidative degradation products, are presented. the methods are based on the first derivative (D₁) and second derivative (D₂) spectrophotometric measurement (absolute trough, U) at 336 nm and (Peak-trough, Y) at 309–342 nm for carbochromen hydrochloride and at 240–260 nm(U) and 246–268 nm(Y) for dipyridamole. Plots of D₁ or D₂ versus concentration were linear over the concentration range of 8.00–16.00 μg/ml for carbochromen hydrochloride and 4.00–12.00 μg/ml for dipyridamole. Oxidative degradation of these drugs has been optimized with respect to hydrogen peroxide concentration. Determining the intact in coexistence with its oxidative degradation product, the proposed derivative spectrophotometric methods proved to be of high potential in correcting the systematic error appearing in the results of the A_max method due to the latter. Assaying the commercial tablets, the proposed method gave results of high accuracy and reproducibility.     

First Derivative Spectrophotometric Determination of Phenytoin

Abstract

The first derivative curve (D₁) of absorption spectrum of Phenytoin in buffer pH 10 develos negative peaks at 244, 263 and 270 nm. D₁ at 244 nm was found linearly related to concentration over a range 0.4 ? 1.4 mg per 100 ml and highly reproducible (C.V. %=0.62). Tablets and capsules have been analyzed using D₁ at 244 nm and the mean percentage found were 99.7 ± 0.81 and 103.3 ± 0.44, respectively. The B.P. method gave 100.9 and 103.8 %, respectively.     

Application of Difference and Derivative Ultraviolet Spectrometry for the Assay of Some Benzodiazepines

Abstract

Differential (δ A), second derivative (D₂) and differential second derivative (δ D₂) ultraviolet spectrophotometric methods have been described for the quantitiative estimation of clonazepam, diazepam and medazepam in pharmaceutical formulations such as drops, tablets and capsules. Interferences due to excipients and diluents are thereby avoided. Accuracy of the analyses with the proposed procedures is significantly greater than the conventional spectrophotometric and official methods.     

Spectrophotometric Determination of Chlorzoxazone in pure State and Formulations Through Oxidative Coupling of its Hydrolysis Product

ABSTRACT

Three simple and sensitive procedures (Methods A, B and C) for the assay of chlorzoxazone (CZZ) in pure form and in formulations are described. The methods are based on the oxidative coupling reaction of the hydrolysis product of chlorzoxazone (HCZZ) with 3-methyl-2-benzothiazolinone hydrazone (MBTH) in the presence of Fe (III) (Method A, λ_max 445 nm), N, N-dimethyl-p-phenylene diamine (DMPD) in the presence of periodate (IO₄) (method B, λ_max 605 nm) and 2, 6-dichloroquinone chlorimide (DCQC) (Method C, λ, _max 560 nm). The Beer's law limits were found to be 5.0 to 25.0 μg/ml in the case of methods A and B and 2.0 to 12.0 μg/ml in the case of method C. The results are statistically validated and the reactions involved are presented.     

Different chromatographic methods for simultaneous determination of diloxanide furoate,metronidazole and its toxic impurity

TLC densitometric and RP-HPLC methods are innovative chromatographic methods used for determination of diloxanide furoate, metronidazole and its impurity, 4-nitroimidazole. In the developed TLC densitometric method, appropriate separation was achieved using silica gel 60 F₂₅₄ TLC plates and ethyl acetate/acetone/hexane/ammonia solution (9.5:0.5:0.3:0.3, by volume), as a developing system and the separated bands were UV-scanned at 276 nm. While the developed RP-HPLC method depended on separation of components on C8 column using deionized water containing 0.05 % TEA: methanol (40:60, v/v) as a mobile phase at constant flow rate of 1 mL/min with UV detection at 276 nm. Variables affecting performance of the developed methods were studied and optimized. Regression analysis showed acceptable correlation coefficients in the selected ranges with excellent percentage recoveries. The methods showed no significant interferences from dosage form excipients, and the validity of the proposed methods was further assessed by applying standard addition technique. In addition, results obtained by applying the proposed methods were statistically compared to those obtained by applying the reported method and no significant difference was found between them. The suggested methods were successfully applied for the determination of the cited drugs in bulk powder, laboratory prepared mixtures and commercial tablets.     

Lanthanide(III) Complexes of Two Novel N 3 O 4 -donor Macrocycles Derived from 3,6-Dioxa-1,8-Octanediamine

Cyclodextrins are a group of cyclic oligosaccharides which have shown to improve pharmaceutical properties of drugs, such as solubility and stability, by forming inclusion complexes. Diloxanide furoate has direct amoebicide action on the intestinal lumen and little solubility in water. In this work, solubility, NMR, fluorescence techniques, and kinetic methods were used to determine the equilibrium constant for the formation of the -cyclodextrin–diloxanide furoate complex, K_1:1. It is shown that the kinetic approach is the best method for such a determination.     

High Performance Liquid Chromatogrphy of Fat-Soluble Vitamins. III. Determination of Vitamin D3 in Pharmaceutical Preparations and in Blood

Abstract

A reversed phase high-performance liquid chromatographic method (HPLC) is described for separation and determination of colecalciferol (Vitamin D₃) in Vitamin preparations and in biological materials. Vitamin D₃ is extracted from the formulations and from the blood in a fully automated electronically controlled extraction apparatus. For HPLC a column of lichrosorb RP18 and methanol as eluent are used. The extraction, separation and determination of vitamin D₃ needs about 10–20 minutes. The described extraction and HPLC methods allow the detection of 1–2 ng per injection and are well reproduced with a maximum coefficient of variation of < 3,5%. Vitamin A-acetate is used as internal standard.     

Synthesis and Characterization of Gold Nanoparticles with Surface Ligands Derived from a Primary Phosphine

Reduction of HAuCl₄ · 3H₂O with NaBH₄ in THF/H₂O in the presence of the primary phosphine PH₂Mes* (Mes* = 2,4,6-(t-Bu)₃C₆H₂) gave a mixture of ca. 1.3 nm diameter gold nanoparticles (1) and the known oligomers [Au(PHMes*)]_n (2). Nanoclusters 1 might contain phosphido (PHMes*) or phosphinidene (PMes*) surface ligands, or both; they were characterized by elemental analysis, TGA, XPS, TEM, NMR, IR, and UV–Vis spectroscopies, and by their reactions with dodecanethiol, which gave PH₂Mes*. Solid-state ³¹P-NMR cross-polarization studies of 1 and 1D (prepared using NaBD₄ and PD₂Mes* in THF/D₂O) were consistent with the presence of phosphinidene surface groups.     

Spegtrophotometrig Determination of α -Tocopherol Acetate in Soft Capsules

Abstract

Two spectrophotometric methods have been described for the determination of α -tocopherol acetate (vitamin E) in soft capsules. The first method applies the orthogonal function method under least squares. The quadratic coefficients calculated over the wavelength range 277 - 304 nm at 4-nm intervals in chloroform were reproducible and independent of ethyl oleate concentration. The second method applies the second derivative (D₂) to correct for irrelevant absorbance due to ethyl oleate The peak trough amplitude at 271 - 287 nm was in linear correlation to the concentration of vitamin E. The recoveries obtained using the proposed methods agreed with those obtained using the official proceduce.     

Determination of Vitamin D3 and 25-Hydroxyvitamin D3 Using Liquid Chromatography with Amperometric Detection

Abstract

The electrochemical behaviour of vitamin D₃ and 25-hydroxyvitamin D₃ (25-OH D₃) in a high performance liquid chromatography system using amperometric detection is described. Separation is carried out using a C18 reversed-phase column and the optimum mobile phase was a 0.1 M LiClO₄ solution in methanol-water (97:3, v/v) at a flow rate of 1.25 ml/min. 25-OH D₃ and vitamin D₃ were eluted with good resolution at retention times of 3 and 6 minutes respectively, and determined by amperometric detection with a glassy carbon electrode at + 1.050 V (vs Ag/AgCl). Calibration graphs for both substances showed good linearity when amounts of vitamin D₃ between 18 and 312 ng and 27 and 412 ng of 25-OH D₃ were injected. Detection limits of 8 ng (vitamin D₃) and 25 ng (25-OH D₃); relative standard deviations of 3.2% (vitamin D₃) and 5.8% (25-OH D₃) were obtained.     

Determination of Vitamins D2 and D3 in Feedingstuffs by High Performance Liquid Chromatography

Abstract

A sensitive and reliable HPLC method for complete separation and quantitation of vitamins D₂ and D₃ in complicated biological mixtures such as feedingstuffs has been developed and described. The method has been applied to the quantitative determination of D₂ and D₃ in feedingstuffs and related matrices at both high premix levels and low feed levels ranging down to a detection limit near 100 IU/1b or 0.22 IU/g sample. The procedures consist of the initial step of sample preparation by extraction; four sample cleanup stages: Sep/Pak/Silica Cartridge Cleanup, Millipore-Teflon Cleanup, Gel Permeation/Sephadex LH-20 Column Cleanup, and HPLC/Partisil-PAC Column Cleanup; and the final step of Reverse-Phase HPLC Separation, Identification, and Quantitation. The analytical Column used was Rainin Accupak 20 cm-3 um C-18 & Guard Columns. The Waters Associates Model 440 Fixed Wavelength UV Detector at 254 nm was used for all measurements. All separations and quantitations were carried out isocratically at room temperature and under subdued lighting. By these procedures, the sensitivity for both D₂ and D₃ is about the same (20 ng), and the resolution is excellent. Normally, the D₂ peak eluted at 30–31 min. and the D₃ peak followed at 2–3 min. later. By using the standard calibration and standard addition methods, the percent recovery ranges from 90.0%–104.8% with the mean value of 97.4%, whereas the accuracy is from 85.3% to 108.9% with the average of 97.8%. The standard deviation is ±5.2% and the coefficient of variation is 5.3%.     

Direct and Convenient Method of Regioselective Benzylation of Methyl α‐D‐Glucopyranoside

A facile and convenient method for the direct preparation of methyl 2,3,6‐tri‐O‐benzyl‐α‐D‐glucopyranoside (2) by the regioselective benzylation of methyl α‐D‐glucopyranoside (1) with benzyl bromide in the presence of mild bases K₂CO₃ and KOH (1∶1) without solvents is reported.     

THE SYNTHESIS,CRYSTAL, MOLECULAR AND ELECTRONIC STRUCTURES OF TRIBROMO(NITROSYL) BIS(TRIPHENYLPHOSPHINE OXIDE) RHENIUM(II) AND TRIBROMO(NITROSYL) BIS(TRIPHENYLPHOSPHINE)RHENIUM(I)

Abstract

Gaseous nitric oxide reacts with a benzene solution of [ReOBr₃(PPh₃)₂] to give [ReBr₃(NO) (OPPh₃)₂] (1). When the reaction is carried out in the presence of an excess of free triphenyl-phosphine, the product is [ReBr₃(NO)(PPh₃)₂] (2). The latter is also isolated in the reaction of 1 with PPh₃. This paper, apart from the synthetic methods, presents spectroscopic and magneto-chemical measurements, and crystal, molecular and electronic structures for 1 and 2.     

A SYNTHETIC ROUTE TO 3-METHYLTHIO-2-ALKANONES STARTING FROM 3-ALKYL-2,4-PENTANEDIONES

Abstract

An efficient preparation of a 3-methylthio-2-alkanone (1) has been realized by the reaction of a 3-alkyl-2,4-pentanedione (8) with one mol-equiv of S-methyl methanethiosulfonate (4) in the presence of excess EtONa in EtOH. Furthermore, treatment of 8 with 4 and K₂CO₃ in refluxing acetone, followed by addition of MeOH and heating the resulting mixture, gave 1 in a high yield. These methods were applied to synthesis of pseudoionone.     

Synthesis,crystal structure,and luminescence properties of [TbGd(NAA)6(phen)2] and [Tb2(NNA)6(phen)2] · 2C3H7NO

Lanthanide(III) heteronuclear and binuclear complexes [TbGd(NAA)₆(phen)₂] (1) and [Tb₂(NAA)₆(phen)₂] · 2C₃H₇NO (2) (NAA = 1-naphthylacetic acid, phen = 1,10-phenanthroline) were prepared and their crystal structures were determined. In 1 and 2, each lanthanide is nine-coordinate by two bidentate-bridging and two tridentate chelating-bridging carboxylate groups, one bidentate chelating carboxylate and one phen molecule in a distorted monocapped square antiprism. The solid-state luminescence behavior and the antibacterial activities were studied. Complexes 1 and 2 exhibited characteristic emission of Tb(III) ion ⁵D₄ → ⁷F_J (J = 6–0) under UV radiation at room temperature. A main excitation peak (359 nm) of 2 appears under red emission of 615 nm. By contrast, all emission peak intensities of 1 were enhanced by addition of gadolinium(III), and the 545 nm band is much stronger than the 615 nm band, attributed to, under perturbation of the ligand field, the probability of ⁵D₄ → ⁷F₃ transition of Tb(III) was greatly enhanced in 2. Because of perturbation of the ligand field by addition of gadolinium(III), the probability of ⁵D₄ → ⁷F₅ transition of Tb(III) was greatly enhanced in 1 and green fluorescence was observed. The antibacterial activity showed that the two complexes were active against Escherichia coli, Staphylococcus aureus and Bacillus subtilis.     

Spectrophotometer Determination of Nitrite Using Salbutamol sulphate as a Reagent

Abstract

A simple spectrophotometric method for the trace determination of nitrite (NO^? ₂) is described. Nitrite is reacted with Salbutamal sulphate in acidic medium which gives a yellow colour in alkaline medium (?pH 7) and can be determined in the presence of several cations and anions. Beer's law is obeyed in the range of 1.8 to 27.6 ppm of nitrite with the molar absorptivity 1.8 × 10³ 1 × mole^?1 × cm^?1 at 4l0 nm. The proposed method can also be utilized for the determination of nitrate (NO^? ₃) after its reduction to nitrite. The method has been applied for the determination of various samples containing traces of nitrite.     

Synthesis of Neu5Ac α-(2→ 8)Neu5Ac α-(2→ 3)Galβ1→ Och2Ch2Ch3, A Determinant Epitope of Gd3 Ganglioside

ABSTRACT

Synthesis of the terminal trisaccharide sequence of the ganglioside GD₃, α-D-Neup5Ac-(2→8)-α-D-Neup5Ac-(2→3)-β-D-Galp-(1→4)-β-D-Glcp-(1→1)-Cer (2) was achieved by employing an α-(2→8) disialyl glycosyl donor (1). Condensation of 1 with the glycosyl acceptor 6, propyl 4,6-O-benzylidene-β-D-galactopyranoside, gave the desired protected trisaccharide 10 (14%) as well as the elimination and hydrolysis products of 6, compounds 8 and 9 respectively. O-Deacetylation and debenzylation of 10 gave the final trisaccharide 11, as its propyl glycoside.     

Application of Crown Ether in Chemical Analysis Extraction of Copper(II)-Zincon Chelate Anion with Crown Ether Complex

Abstract

Crown ether-potassium ion complex extracts selectively copper-zincon anion complex as ion-pairs into chloroform phase in the presence of copper-zincon and zinc-zincon chelate anion, whereas quarternary ammonium ion extracts both anions. By measuring the absorbance of the chloroform phase at 615 nm, copper in the presence of zinc has been determined spectrophotometrically. The composition of extracted species was estimated to be Cu²⁺-zincon^4?-(KL⁺)₂.     

Synthesis,Characterization, and Spectroscopic Properties of Hexa(4-Bromo-2-Formyl-Phenoxy)Cyclotriphosphazene and Hexa(4-Chloro-2-Formyl-Phenoxy)Cyclotriphosphazene and Fully Substituted Cyclotriphosphazene Derivatives Bearing a Schiff Base at Room Temperature

Abstract

Hexa(4-bromo-2-formyl-phenoxy)cyclotriphosphazene (2) and hexa(4-chloro-2- formyl-phenoxy)cyclotriphosphazene (3) were obtained from the reactions of hexachloro- cyclotriphosphazene (1) with 5-bromosalicylaldehyde and 5-chlorosalicylaldehyde in the presence of (C₂H₅)₃N and K₂CO₃ at room temperature, respectively. The new two organocyclotriphosphazenes bearing formyl groups were reacted with 4-cyano aniline, 2-phenyl aniline, 4-aceto aniline, 5-chloro-2-hydroxy aniline, 2-hydroxy aniline, 4-hydroxy aniline, 2-(4-morpholino)ethyl amine, 4-carboxy aniline, 4-carbomoyl aniline, 2-mercapto aniline, and 5-amino isoquonoline to prepare cyclotriphosphazene derivatives containing a Schiff base at room temperature. However, fully phenoxy-substituted cyclotriphosphazenes containing a Schiff base were isolated from the reactions of the compound 2 and 3 with 5-chloro-2-hydroxy aniline, 2-hydroxy aniline, 4-hydroxy aniline, and 2-(4-morpholino)ethyl amine. The structures of the synthesized compounds were characterized by elemental analysis, IR, and NMR (¹H, ¹³C, ³¹P) spectroscopy. According to the results of the analysis, all synthesized compounds were found to be fully substituted organocyclotriphosphazenes, such as hexa[4-bromo-2-(5-chloro-2-hydroxy-pheyliminomethyl)phenoxy]cyclotriphosphaze (2a). All cyclotriphosphazene derivatives synthesized gave fluorescence emission peaks in range between 300 nm and 410 nm.     

Quantitative Determination of Octamethylcyclotetrasiloxane (D4) in Extracts of Biological Matrices by Gas Chromatography-Mass Spectrometry

Abstract

A method was developed and validated to measure octamethylcyclotetrasiloxane (D₄)^? quantitatively by gas chromatography-mass spectrometry (GC-MS) at low level in extracts of several biological matrices that include plasma, liver, lung, feces and fat from rats. The key to the successful determination lay in the use of extracts dried with anhydrous magnesium sulfate. This was necessary in view of the propensity of the methyl siloxane based GC-stationary phase to generate D₄ by its reaction with water present in the extracts. To enable quantiiation of D₄ at parts per billion (μg/L) levels, the base ion m/z 281 resulting from the loss of a methyl group from the parent molecule was selected for monitoring by SIM mode in GC-MS. The recovery of D₄ from any of the biological matrices was determined to be greater than 90% in three extractions. The D₄ response for the standards in GC-MS was linear (R² > 0.9900) and reproducible at concentrations ranging from 1—16,000 ng D₄/g solvent. Precision was less than 5%.