Chiral stability-indicating HPLC method for analysis of arotinolol in pharmaceutical formulation and human plasma

An enantioselective stability-indicating high performance liquid chromatographic method was developed for the analysis of arotinolol in standard solution. The degradation behaviour of arotinolol was investigated under different stress conditions recommended by International Conference on Harmonization (ICH). Resolution of the drug and complete separation from its degradation products were successfully achieved on a Chirobiotic V column, using UV detector set at 315 nm, polar organic mobile phase (POM) consisting of methanol:glacial acetic acid:triethylamine, 100:0.02:0.03, (v/v/v), and a flow rate of 1 ml/min. The drug was subjected to oxidation, hydrolysis, photolysis, and heat to apply stress conditions. The drug was found to degrade in alkaline, acidic, oxidative conditions and when exposed to heat. The drug was stable to sunlight. The method reported here has also been successfully applied to pharmaceutical formulation and to human plasma that spiked with stock solutions of arotinolol enantiomers.Arotinolol enaniomers were recovered from plasma by using liquid–liquid extraction procedure with ethyl ether. The method was highly specific, where degradation products and coformulated compounds did not interfere, and was sensitive with good precision and accuracy and was linear over the range of 50–400 ng/ml (R² > 0.9981) with a detection limit of 20 ng/ml for each enantiomer. The mean extraction efficiency for arotinolol was in the ranges 96–104% for each enantiomer. The mean relative standard deviation (RSD) of the results of within-day precision and accuracy of the drug were ?7.1%. There was no significant difference between inter- and intra-day studies for each enantiomers which confirmed the reproducibility of the assay. The overall recoveries of arotinolol enantiomers from pharmaceutical formulations were in the ranges 97.6–101.8%.     

Gamma radiolytic degradation of fluoranthene and monitoring of radiolytic products using GC–MS and HPLC

Removal of priority pollutant fluoranthene in methanol by gamma-irradiation under varied conditions has been optimized. The influence of applied dose and dose rate on the degradation of fluoranthene under nitrogen has been investigated. The preliminary radiolytic degradation efficiency has been monitored by spectrophotometry. HPLC and GC–MS have been used to study the nature of degradation pattern. It is found that four main degradation products are formed and detected by HPLC. Different reversed phase columns have been used for the separation of degraded products under optimum chromatographic conditions. For 2 kGy dose ⩾80% fluoranthene has been degraded at dose rate 200 Gy/h. However, a dose of 370 Gy/h was more effective and it produces for less degradation products. Radiolytic degraded fluoranthene was also analyzed to detect various degradation products using GC–MS. It was proposed that major products were hydrocarbons and methoxy group containing organic compounds after comparing their mass spectra with the installed NIST mass spectral library.     

Study on the Kinetics of Vitamin C Degradation in Fresh Strawberry Juices

Vitamin C is an essential nutrient needed for maintaining the human health. Strawberry fruit have a relatively high content of vitamin C, which is around 40-70 mg/ 100 g strawberries. However, vitamin C which is also known as ascorbic acid is easily degraded during storage. The objective of this research is to study the kinetics of degradation of vitamin C in fresh strawberry juices upon storage and to investigate the effect of storage temperatures and sugar addition on the ascorbic acid loss in strawberry juices. Four different types of fresh strawberry juices were prepared, namely A, B, C, and D. Juices A and C were stored at a room temperature of 28 °C, while samples B and D were stored at a refrigerated temperature of 8 °C. Furthermore, juices A and B were prepared without sugar addition, while sugar was added to juices C and D. The concentration of ascorbic acid in the juice was analyzed using iodimetric titration method. It was monitored every one hour for 8 hours of storage for the kinetics of ascorbic acid degradation study. The results showed that the degradation reaction of vitamin C followed zero-order kinetic models in all types of juices. The degradation reaction rate constants obtained for juices A, B, C, and D were 4.42; 3.63; 2.32; and 1.85 mg vitamin C/(100 ml. h), respectively. The activation energy for the vitamin C degradation in fresh strawberry juices with sugar and without sugar addition was estimated to be 1.90 kcal/ mol and 1.65 kcal/ mol, respectively. In conclusion, the storage at a lower temperature combined with sugar addition could effectively slow the rate of degradation of vitamin C.     

Analysis of phenanthrene biodegradation by using FTIR,UV and GC–MS

The aim of this paper is to assess the biodegradation of phenanthrene by Flavobacteria FCN2 which was isolated from coke plant sludge via a classical shaken liquid medium enrichment method. The strain FCN2 can decompose phenanthrene (50 mg l^?1) completely within 5 days. The values of pH decrease to 6.7 from 7.2 during degradation periods. And a detailed phenanthrene metabolism was assayed by using FTIR, UV and GC–MS. For FTIR, appearance of new broad absorption bands at 2858 cm^?1, 2927 cm^?1, 2955 cm^?1 and another new strong absorption band at 1734 cm^?1 in metabolites demonstrates that carboxyl group produced during phenanthrene degradation. Besides this, a very strong absorption band appears at 1260 cm^?1. It is ascribed to C–C stretching vibration band in carbonyl group of arone. Two weak adsorption at 334 nm and 349 nm in UV spectra were assigned to the n-π* transition of CO of aldehyde. Two metabolites, phenanthrene-dihydrodiol and naphthalene-1-diol were identified in neutral fraction of phenanthrene degradation by using GC–MS. As a result carboxylic acids and arone were generated during biodegradation of phenanthrene by Flavobacteria FCN2.     

Change in the enzymatic dual function of the peroxiredoxin protein by gamma irradiation

PP1084 protein was exposed to gamma irradiation ranging from 5 to 500 kGy. Native PAGE showed minor structural changes in PP1084 at 5 kGy, and major structural changes at >15 kGy. Size-exclusion chromatography (SEC) showed the formation of a new shoulder peak when the protein was irradiated with 15 and 30 kGy, and a double peak appeared at 100 kGy. The results of PAGE and SEC imply that PP1084 protein is degraded by gamma irradiation, with simultaneous oligomerization. PP1084 chaperone activity reached the highest level at 30 kGy of gamma irradiation, and then, decreased in a dose-dependent manner with increasing gamma irradiation. However, the peroxidase activity significantly decreased following exposure to all intensities of gamma irradiation. The improvement of chaperone activity using gamma irradiation might be promoted by the oligomeric structures containing covalently cross-linked amino acids. Consequently, PP1084 modification using gamma irradiation could elevate chaperone activity by about 3–4 folds compared to the non-irradiated protein.     

Stability-indicating HPLC method for the determination of nicardipine in capsules and spiked human plasma. Identification of degradation products using HPLC/MS

In this stability-indicating, reversed-phase high-performance liquid chromatographic method for nicardipine (NIC), forced degradation has been employed and the formed degradants were separated on a C18 (150 mm × 3.9 mm, 5 μm) analytical column using a mobile phase consisted of 70% methanol: acetic acid containing 0.01 M triethylamine with pH 4. The flow rate was 1.0 mL/min and the photodiode array detection wavelength was 353 nm. Forced degradation of the drug was carried out under acidic, basic, photolytic, and oxidative stress conditions. Chromatographic peak purity data indicated no co-eluting peaks with the main peaks. This method resulted in the detection of seven degradation products. Among these, two major degradation products from basic hydrolysis, one from oxidation by H₂O₂ and four from photolytic stress were identified by mass spectral data. A good linear response was achieved over the range of 0.5–40 μg/mL with a limit of detection (LOD) of 0.011 μg/mL and limit of quantification (LOQ) of 0.036 μg/mL. The suggested method was successfully applied for the analysis of NIC in its commercial capsules, with mean% recovery value of 100.11 ± 2.26%. The method was extended to the in vitro determination on NIC in spiked human plasma samples with mean% recovery of 99.04 ± 5.67%. The suggested method was utilized to investigate the kinetics of photolytic induced degradation.     

Synthesis and characterization of highly-active nickel and lanthanum co-doped SrTiO3

A series of highly-active nickel and lanthanum co-doped SrTiO₃ photocatalysts were synthesized via sol–gel process and their photocatalytic activities were evaluated by degradation of methylene blue (MB). The obtained samples were found by XRD, XPS and UV–vis to have a perovskite structure in which Ni and La atoms were incorporated into SrTiO₃. After Ni and La doped into SrTiO₃, the absorption edge of SrTiO₃ powder was greatly shifted from 380 nm to 700 nm. Under a 100 W incandescent lamp irradiating for 14 h, a 100% of MB was degraded, which is much higher than those of pure SrTiO₃ and commercial Degussa P25. The optimal range of Ni and La dopants is 0.1–1.0 mol%. The formation of a new absorption edge and the large surface area may be the main reasons for the high activity.     

Simultaneous determination of diastereoisomeric and enantiomeric impurities in SSS-octahydroindole-2-carboxylic acid by chiral high-performance liquid chromatography with pre-column derivatization

SSS-Octahydroindole-2-carboxylic acid (SSS-Oic) is a key intermediate used in the synthesis of some angiotensin-converting enzyme (ACE) inhibitors. The separation of diastereoisomers and enantiomers of Oic was performed using a pre-column derivatization chiral HPLC method. Phenyl isothiocyanate (PITC) was used as the derivatization reagent. Three PITC derivatives of Oic stereoisomers were separated on an Ultron ES-OVM chiral column (150 mm × 4.6 mm, 5 μm). Derivatization conditions such as reaction temperature, reaction time and derivatization reagent concentration were investigated. The chromatographic conditions for separation of the three PITC-Oic derivatives were optimized. The method was successfully applied in the diastereoisomeric and enantiomeric purity test of SSS-Oic.     

Thermal degradation and evolved gas analysis: A polymeric blend of urea formaldehyde (UF) and epoxy (DGEBA) resin

A polymeric blend has been prepared using urea formaldehyde (UF) and epoxy (DGEBA) resin in 1:1 mass ratio. The thermal degradation of UF/epoxy resin blend (UFE) was investigated by using thermogravimetric analyses (TGA), coupled with FTIR and MS. The results of TGA revealed that the pyrolysis process can be divided into three stages: drying process, fast thermal decomposition and cracking of the sample. There were no solid products except ash content for UFE during combustion at high temperature. The total mass loss during pyrolysis at 775 °C is found to be 97.32%, while 54.14% of the original mass was lost in the second stage between 225 °C and 400 °C. It is observed that the activation energy of the second stage degradation during combustion (6.23 × 10⁻⁴ J mol⁻¹) is more than that of pyrolysis (5.89 × 10⁻⁴ J mol⁻¹). The emissions of CO₂, CO, H₂O, HCN, HNCO, and NH₃ are identified during thermal degradation of UFE.     

Changes in Secondary Metabolite Contents Following Crude Drug Preparation

Crude drug is commonly prepared by directly drying of freshly harvested plant organ or after slicing. These processes may decrease or maintain the content of the desired metabolites presence in the crude drug. Plant rhizome can be directly sliced followed by drying or after storage at certain period. Certain rhizome can maintain the secondary metabolites after being stored for three months (12 weeks), while others decreased just after being stored for two weeks. Drying process can be performed under the sun or in an air circulated oven with temperature not higher than 60 °C. Phenolic content of crude drugs on the other hand is the lowest if it is dried at 60 °C. Drying at 40 °C, 80 °C and 100 °C produce crude drug with higher phenolic content compared to those dried at 60 °C. This may associated with the activity of peroxidase that has optimal activity at 60° C. At above 60 °C, the activity of peroxidase may decrease due to the degradation of the enzyme. Moist treatment of fresh material may increase the content of the secondary metabolites. Boiling of Cosmos caudatus leaves increased the content of the flavonoid glycoside. However, part of the flavonoid was presence in the aliquot that hamper further step of crude drug preparation. Steaming of potato peels increased the chlorogenic acid content. From these observations, steaming can be considered as one of pre-treatment steps in the preparation of crude drugs prior drying process. The increase of flavonoid glycoside in Cosmos caudatus leaves upon boiling has been confirmed not due to the increase the extractability of the flavonoid. The increase of key enzyme activity that involved in the biosynthetic pathway upon moist-heat treatment need to be further studied     

Influence of thermal treatment on the glass transition temperature of thermosetting epoxy laminate

The influence of accelerated thermal treatment of thermosetting epoxy laminate on its glass transition temperature was studied. Lamplex^® FR-4 glass fibre-reinforced epoxy laminate (used for printed circuit board manufacturing) was used in these experiments. The composite was exposed to thermal treatments at temperatures ranging from 170 °C to 200 °C for times ranging from 10 to 480 h. The glass transition temperature (T_g) was analysed via dynamic mechanical analysis (DMA). It has been proven that the glass transition temperature rapidly decreases in reaction to thermal stress. The obtained T_g data were used for Arrhenius plots for different critical temperatures (T_g-crit. = 105–120 °C). From their slopes (?E_a/R), the activation energy of the thermal degradation process was calculated as 75.5 kJ/mol. In addition to this main relaxation mechanism, DMA also recorded one smaller relaxation process in the most aged samples. Microscopic analysis of the sample structure showed the presence of pronounced small regions of degradation both on the surface and in the inner structure, which are probably the causes of microscopic delamination and the smaller relaxation process.     

Development of a stability-indicating high performance liquid chromatography method for assay of erythromycin ethylsuccinate in powder for oral suspension dosage form

In this study an effective method was developed to assay erythromycin ethylsuccinate for an oral suspension dosage form. The chromatographic separation was achieved on an X-Terra™ C₁₈ analytical column. A mixture of acetonitrile–ammonium dihydrogen phosphate buffer (0.025 mol L^-1) (60:40, V/V) (pH 7.0) was used as the mobile phase, effluent flow rate monitored at 1.0 mL min⁻¹, and UV detection at 205 nm. In forced degradation studies, the effects of acid, base, oxidation, UV light and temperature were investigated showing no interference in the peak of drug. The proposed method was validated in terms of specificity, linearity, robustness, precision and accuracy. The method was linear at concentrations ranging from 400 to 600 μg mL⁻¹, precise (intra- and inter-day relative standard deviations <0.65), accurate (mean recovery; 99.5%). The impurities and degradation products of erythromycin ethylsuccinate were selectively determined with good resolution in both the raw material and the final suspension forms. The method could be useful for both routine analytical and quality control assays of erythromycin ethylsuccinate in commercial powder for an oral suspension dosage form and it could be a very powerful tool to investigate the chemical stability of erythromycin ethylsuccinate.     

Stability of NF membranes under extreme acidic conditions

Two commercial nanofiltration (NF) membranes (FilmTec NF-45 and Desal-5 DK) and two new NF-1 membranes made by BPT (Bio Pure Technology) for the purpose of a European Union funded research project (RENOMEM) were tested under extreme acidic conditions. The polyethersulphone (PES) ultrafiltration (UF) supports used for casting the BPT-NF-1 membranes were also tested under similar conditions. The 006 and 015 UF supports were found to be stable in 5% nitric acid at 20 and 80 °C for 4 and 3 months, respectively. Both supports (006 and 015) showed a significant reduction in flux after immersion in sulphuric acid at both temperatures. The BPT-NF-1 membranes showed excellent resistance to 20% sulphuric acid for up to 4 months at 20 °C but were attacked by the nitric acid solution. The resistance of the two commercial membranes in 20% sulphuric acid at 20 °C was generally lower than that of the BPT-NF-1 membranes. The NF-45 membrane was slightly more stable in 5% nitric acid at 20 °C. Degradation of the membrane occurred only after 2 months while both the Desal-5 DK and BPT-NF-1 membranes degraded during the first month. At the higher temperature of 80 °C in 5% nitric acid all membranes degraded in the first month.The cause of membrane degradation was attributed to oxidation of the thin NF selective skin layer in nitric acid and to acid-catalysed hydrolysis of this layer in sulphuric acid. Knowing the cause of membrane degradation is a step forward in developing a better and more stable nanofiltration membrane.     

Degradation of diazinon contaminated waters by ionizing radiation

Study of degradation of diazinon pesticide by ⁶⁰Co gamma irradiation in a single aqueous solution was conducted on a laboratory scale and the effect of ionizing radiation on the removal efficiency of diazinon residues was investigated. Distilled water solutions at three different concentrations of targeted compound (i.e. 0.329, 1.643 and 3.286 μmol dm⁻³) were irradiated over the range 0.1–6 kGy. The initial concentration of contaminant and irradiation doses play a significant role in the rate of destruction; this was evident from the calculated decay constants of diazinon residue. Gamma radiolysis showed that the absorbed doses from 1.5 to 5.6 kGy at a dose rate of 4.79 kGy h⁻¹ achieved 90% destruction for diazinon with initial concentrations over the range 0.329–3.286 μmol dm⁻³. The radiolytic degradation by-products and their mass balances were qualitative determined with good confidence by using GC/quadrupole mass spectrometry (GC/MS) with EI⁺ or CI in positive and negative ionization mode and diazinon degradation pathways were proposed. Additionally, the final products of irradiation were identified by ion chromatography (IC) to be acetic and formic acid.     

Free radical scavenging and COX-2 inhibition by simple colon metabolites of polyphenols: A theoretical approach

Free radical scavenging and inhibitory potency against cyclooxygenase-2 (COX-2) by two abundant colon metabolites of polyphenols, i.e., 3-hydroxyphenylacetic acid (3-HPAA) and 4-hydroxyphenylpropionic acid (4-HPPA) were theoretically studied. Different free radical scavenging mechanisms are investigated in water and pentyl ethanoate as a solvent. By considering electronic properties of scavenged free radicals, hydrogen atom transfer (HAT) and sequential proton loss electron transfer (SPLET) mechanisms are found to be thermodynamically probable and competitive processes in both media. The Gibbs free energy change for reaction of inactivation of free radicals indicates 3-HPAA and 4-HPPA as potent scavengers. Their reactivity toward free radicals was predicted to decrease as follows: hydroxyl >> alkoxyls > phenoxyl ≈ peroxyls >> superoxide. Shown free radical scavenging potency of 3-HPAA and 4-HPPA along with their high μM concentration produced by microbial colon degradation of polyphenols could enable at least in situ inactivation of free radicals. Docking analysis with structural forms of 3-HPAA and 4-HPPA indicates dianionic ligands as potent inhibitors of COX-2, an inducible enzyme involved in colon carcinogenesis. Obtained results suggest that suppressing levels of free radicals and COX-2 could be achieved by 3-HPAA and 4-HPPA indicating that these compounds may contribute to reduced risk of colon cancer development.     

In vitro cytotoxicity against K562 tumor cell line,antibacterial, antioxidant,antifungal and catalytic activities of biosynthesized silver nanoparticles using Sophora pachycarpa extract

In the present study, we demonstrate the green synthesis of silver nanoparticles using Sophora pachycarpa extract (S. pachycarpa; SPE) as capping, reducing, and stabilizing agents. The biosynthesized silver nanoparticles (SPE-AgNPs) were tested for catalytic, antibacterial, antifungal, antioxidant, and anti-cancer activities. The affecting parameters (the concentration of silver nitrate, the temperature of the reaction, and time of reaction) on the synthesis process were optimized. The biosynthesized SPE-AgNPs were studied by X-Ray diffraction (XRD), transmission electron microscopy (TEM), field emission scanning electron microscopy (FESEM), dynamic light scattering (DLS), energy-dispersive X-ray spectroscopy (EDS) and Fourier-transform infrared spectroscopy (FT-IR). The FESEM and TEM results revealed spherical and oval-like morphology with sizes ranging from 30 to 40 nm. Photocatalytic performance experiments of SPE-AgNPs were determined by the rapid degradation of the eriochrome black T (EBT) and methylene blue (MB) under sunlight and UV irradiations. The results showed that SPE-AgNPs degraded more than 90% and 80% of both dyes under UV and sunlight irradiations, respectively. In addition, the SPE-AgNPs exhibited good antibacterial and antifungal properties against S. aureus, S. epidermidis, P. aeruginosa, E. coli, K. pneumoniae, E. faecalis, and C. albicans with MIC values of 6.25, 6.25, 0.78, 0.39, 0.78, 1.56 and 0.78 µg/ml. The green synthesized SPE-AgNPs were found to inhibit the activity of DPPH free radicals efficiently. Eventually, the SPE-AgNPs exhibited significant in vitro cytotoxicity against K562 tumor cell line (IC50 = 19.5 µg/ml). All these studies indicated that AgNPs synthesized using S. pachycarpa extract have applications in the environmental and biomedical fields.     

Enantiomeric separation of a melatonin agonist Ramelteon using amylose-based chiral stationary phase

A new simple isocratic chiral liquid chromatographic method was developed for the enantiomeric purity of Ramelteon[(S)-N-[2-(1,6,7,8-tetrahydro-2H-indeno[5,4-b]furan-8-yl) ethyl]-propionamide], a melatonin agonist in bulk drugs. The chromatographic separation was achieved on Chiralpak AD-H, 250 mm × 4.6 mm, 5 μm column using a mobile phase system consisting of n-hexane, ethanol and methanesulfonic acid in the ratio of 900:100:0.1 (v/v/v). The mobile phase was pumped on the column at the flow rate of 1 mL min^?1. Addition of methane sulfonic acid in the mobile phase enhanced chromatographic efficiency and resolution between the enantiomers. The resolution between the enantiomers was found to be more than four. The developed method was subsequently validated and proved to be accurate and precise. The experimentally established limit of detection and quantification of (R)-enantiomer were found to be 25.5 and 77.2 ng ml^?1, respectively, for 20 μl injection volumes. The percentage recovery of (R)-enantiomer was ranged from 98.5 to 101.9 in bulk drug samples of Ramelteon. The stability of Ramelteon sample in analytical solution was checked for about 48 h at room temperature and was found to be stable for about 48 h. The proposed method was found to be suitable and accurate for the quantitative determination of (R)-enantiomer in drug substance.     

The effect of silica–alumina catalysts on degradation of polyolefins by a continuous flow reactor

Catalytic degradation of polyolefins was performed in a continuous flow reactor that allows the study of the degradation processes at steady state, characterized by constant values of reaction parameters and properties of the products. The continuous flow reactor was operated at atmospheric pressure and at feed rate of 0–1.5 kg h^?1 polyolefins over two silica–alumina catalysts having different SiO₂/Al₂O₃ mole ratio. Polyethylene (PE), polypropylene (PP) and polystyrene (PS) were degraded at 420, 380 and 360 °C respectively. The cracking effect of silica–alumina was proved by the increased amount of gaseous products and by the decreased molecular weight of liquid products. The differences in surface area and in concentration and acidic strength of active centers of the two catalysts affected the distribution of degradation products. Molar rate of degradation was increased in the presence of catalysts, however the mass rate of degradation was decreased leading to higher values of the calculated activation energies. These interesting results might open new perspectives in understanding the macroscopic mechanism for catalytic degradation of polyolefins.     

The remediation of wastewater containing 4-chlorophenol using integrated photocatalytic and biological treatment

In this work, the performance of integrated photocatalytic and biological treatment was studied for the degradation of 4-chlorophenol (MCP) present in wastewaters. Photocatalysis was used as a pre-treatment to biological degradation. Pollutant removal efficiency was quantified using MCP removal and total organic carbon (TOC) removal. Both photocatalytic as well as biological treatments were carried out in batch reactors, using TiO₂ as the photocatalyst. The inoculum for biological experiments was obtained from paper mill effluent treatment plant and was developed through a process of selection and acclimatization. Effect of TiO₂ concentration on the photocatalytic degradation of MCP was studied along with the effect of the duration of photochemical oxidation and glucose concentrations (0 g/L, 1 g/L and 2 g/L) on the biodegradation of MCP. Integrated biological and photochemical degradation was found to be more effective in treating MCP, especially at higher concentrations (400 mg/L). An initial MCP concentration of 400 mg/L required 96 h for complete mineralization when treated with the process combination, whereas the treatment went on up to 264 h when biodegradation alone was employed.     

Oxidative thermal degradation of LDPE and the determination of some thermodynamic quantities

The pyrolysis of polyolefin wastes is one of the possible ways to obtain chemical feedstocks. In this work, the thermal degradation of low density polyethylene, (LDPE), which is a major product within plastics, was investigated in a semi-batch reactor system. First-order rate kinetics approach was chosen and reaction rate coefficients, k, and some thermodynamic quantities determined such as activation energy, reaction enthalpy, free activation enthalpy, and entropy of degradation of LDPE for different air flow rates. We found that the maximum value of some thermodynamic quantities, such as reaction rate coefficient is 0.0243 min⁻¹ at 600 mL min⁻¹ air flow rate and the free activation enthalpy (ΔG^≠) is 148.66 kJ mol⁻¹ at 450 mL min⁻¹ air flow rate and the reaction enthalpy (ΔH^≠) is 57.65 J mol⁻¹ at 623 K temperature conditions. Moreover, we found that the oxidative degradation of LDPE is not spontaneous and has lower energy necessary (for degradation) than non-oxidative degradation processes.