共查询到20条相似文献,搜索用时 78 毫秒
1.
L L Ng 《Journal of the Association of Official Analytical Chemists》1988,71(3):534-538
A reverse-phase liquid chromatographic method for determination of dexamethasone acetate and of cortisone acetate was subjected to an interlaboratory study by 8 collaborators for each steroid acetate. Bulk drug substance, suspensions, and tablets were assayed. Bulk drug or dosage form is dissolved in an acetonitrile-buffer mixture and analyzed by an external standard method. The steroid acetate is resolved from extraneous components by reverse-phase chromatography and detected at 254 nm. The sample solutions are stable for at least 72 h. For dexamethasone acetate, coefficients of variation were 0.9 and less than or equal to 3.1% for the bulk drug substance and the suspensions, respectively. For cortisone acetate, coefficients of variation were 0.7% for bulk material, less than or equal to 2.0% for suspensions, and less than or equal to 2.5% for tablets. All dosage forms were commercial formulations. The 2 methods have been adopted official first action. 相似文献
2.
E A Bunch 《Journal of the Association of Official Analytical Chemists》1987,70(6):967-973
A normal phase liquid chromatographic method for the determination of dexamethasone in bulk drugs and elixirs was collaboratively studied by 6 laboratories. The method uses a silica column, water-modified acetic acid-methanol-methylene chloride mobile phase, cortisone internal standard, and photometric detection at 254 nm. Collaborators were supplied blind duplicate samples of 3 bulk drugs, 2 commercial elixirs, and 1 authentic elixir. Dexamethasone elixir dosage level is 0.5 mg/5 mL. Mean recovery of dexamethasone from the authentic elixir formulated to contain 0.471 mg/5 mL was 94.5%. (Authentic elixirs were found to stabilize about 6% below the theoretical concentration.) Mean recovery for the bulk drugs was between 97.1 and 100.1%. Mean coefficients of variation for bulk drug and elixir samples were less than 0.8% and 3.6%, respectively. Identification tests for dexamethasone by thin-layer chromatography, infrared spectroscopy, and relative LC retention times, as well as the gas chromatographic determination of alcohol in the elixirs were also collaboratively studied. Mean recovery of alcohol from the synthetic elixir was 98.6%. The mean coefficient of variation for alcohol for all samples analyzed was less than 1.4%. The LC method for dexamethasone in drug substance and elixirs, the identification tests, and the GC method for alcohol in dexamethasone elixirs have been adopted official first action. 相似文献
3.
A A Fatmi G V Williams E A Hickson 《Journal of the Association of Official Analytical Chemists》1988,71(3):528-530
A reverse-phase liquid chromatographic method is described for the assay of medroxyprogesterone acetate in tablets. An octadecylsilane (C18) column with a mobile phase of methanol-0.01M dibasic ammonium phosphate (80 + 20 v/v, pH 7.2 +/- 0.1) and photometric detection at 254 nm separates medroxyprogesterone acetate from excipients. Detector responses were linear to concentrations of medroxyprogesterone acetate over the range 50-150 micrograms/mL (r = 0.999). Mean recovery of medroxyprogesterone acetate added to tablet excipients was 100.8%. Mean assay results were 101.3% (n = 3). The assay results are comparable to those obtained by the compendial liquid chromatographic method. 相似文献
4.
E Smith 《Journal of the Association of Official Analytical Chemists》1979,62(4):812-817
To determine desoxycorticosterone acetate in oil injections, reverse phase partition chromatography on silanized, purified siliceous earth was used to separate the corticosteroid ester from the bulk of the oil vehicle. The latter was retained on the column while the steroid and the sterol and triterpenoid fractions of the oil were eluted. An internal standard was added to this eluate, which was then subjected to reverse phase high performance liquid chromatography (HPLC). The desoxycorticosterone acetate was quantitatively separated in the HPLC procedure from any free desoxycorticosterone, preservatives, and minor components of the oil. The suitability of the HPLC procedure was verified with a number of C18 packing materials, both pellicular and microparticular. The desoxycorticosterone acetate was adequately resolved from the internal standard, progesterone, with most C18 packing materials evaluated. The proposed procedure provides a suitable stability-indicating assay for desoxycorticosterone acetate in oil injections. 相似文献
5.
R D Thompson 《Journal of the Association of Official Analytical Chemists》1985,68(5):1051-1055
A liquid chromatographic (LC) method for the determination of colchicine in pharmaceutical dosage forms and the bulk drug was evaluated in an interlaboratory study which included 13 participating laboratories. The method involves extraction (or dissolution) of the active ingredient with methanol-water (1 + 1), followed by filtration of the extract and reverse phase LC using an octylsilane bonded phase column and UV detection at 254 nm. The mobile phase consists of a methanol-phosphate buffer mixture (pH = 5.5). Three commercial tablet formulations (0.5-0.6 mg colchicine/tablet), 1 synthetic injectable preparation (0.510 mg colchicine/mL), and 1 bulk drug sample were assayed in duplicate by the proposed method. The reproducibility and repeatability standard deviations based on nonpooled results for each sample ranged from 0.0062 mg/mL to 0.0147 mg/tablet and from 0.0037 mg/mL to 0.0127 mg/tablet, respectively; the corresponding coefficients of variation ranged from 1.21 to 2.54% and from 0.73 to 2.19%, respectively. The mean recovery from the synthetic injectable formulation was 100.0%. The method has been adopted official first action. 相似文献
6.
M C Alembik I W Wainer 《Journal of the Association of Official Analytical Chemists》1988,71(3):530-533
A rapid, accurate method for separating and determining the enantiomeric composition of amphetamine bulk drug and commercial preparations was developed and subjected to collaborative study. Amide derivatives of the amphetamine enantiomers are formed by using achiral 2-naphthoyl chloride. The resulting enantiomeric amides are then chromatographed on a commercially available chiral stationary phase with hexane-isopropyl alcohol-acetonitrile (97 + 3 + 0.5) mobile phase, with detection at 254 nm. Seven collaborators received bulk drug and commercial samples of amphetamine. The collaborators and authors determined the mean percent l- and d-amphetamine from 2 injections of each sample. The method can detect the presence of as little as 0.5% of the l-enantiomer in d-amphetamine, with reproducibility between laboratories of +/- 71.3%. The method has been adopted official first action for determination of the enantiomeric composition of amphetamine bulk drug and preparations. 相似文献
7.
采用不同浓度的乙酸和丙酸在中高温下进行厌氧发酵批次试验,采用修正的Gompertz模型和产甲烷的一级动力学模型分析,研究酸浓度和温度对发酵产气动力学的影响。研究表明,当乙酸和丙酸浓度较低时降解较快,高浓度酸抑制产气。乙酸在中温条件下降解较快,质量浓度为5 000 mg/L时中温反应有最大产甲烷速率101 mL/d;质量浓度为10 000 mg/L时高温条件下有最大产甲烷速率77 mL/d,随酸浓度增加,最大产甲烷速率减小,高温反应器对酸的耐受度较高。丙酸在高温条件下更易降解,浓度为4 000 mg/L时,中高温反应均有最大产气速率:78 mL/d(中温)和96 mL/d(高温)。另外,高浓度乙酸和丙酸厌氧降解产气具有滞后性,且随酸浓度的增加滞后期延长,降解过程受到抑制,一级动力学常数减小。温度对厌氧降解的影响大于酸浓度对厌氧降解的影响。 相似文献
8.
Results from the first study in Hong Kong, Southern China, to investigate the concentrations of organic acids in bulk deposition, aerosol and gas phase samples are presented. 57 daily bulk deposition samples were collected in central Kowloonand analyzed by ion chromatography, from May 1999 to May 2000. The volume-weighted (vw) mean concentrations for formate, acetate, propanoate and oxalate were 6.1, 4.5, 0.4 and 1.4 μeq dm-3, respectively, with vw mean pH being 4.65.The maximum acidity contributions by formic and acetic acidsfor bulk deposition samples collected on a daily basis, withpH < 5.0, were 17 and 14%, respectively. The concentrationsof these acids were significantly correlated with each other, butnot with pH. Higher organic acid concentrations were foundin the dry, winter season, and for the synoptic weather systemtypes: approaching cyclone and cold front. Oxalate levels weregenerally higher in bulk deposition samples for north/northeasterly air masses, higher surface windspeeds, and low rainfall amounts. Formic and acetic acids were present at higher concentrations in the gas phase (mean concentrations at two sites were in the range from 3.2 to 6.5 μg m-3, with formate usually < acetate), than in aerosols (mean concentration of formate, acetate or oxalate ≤2.2 μg m-3). Higher levels of organic acids both in aerosols and in the gas phase were found at a busy roadside site than at a residential site. Deposition fluxes for formic and acetic acidsare reported. 相似文献
9.
K L Egli 《Journal of the Association of Official Analytical Chemists》1985,68(4):803-806
A liquid chromatographic method has been developed that determines the amount of sulfasalazine in tablets and bulk powder in the presence of residual synthesis by-products and excipients. The method was tested on crude product containing large amounts of impurities. A C-18 reverse phase column with water-acetonitrile-acetic acid mobile phase was found to effectively separate the drug on the column. Six different commercial samples of 500 mg tablets were assayed. The results varied from 92.6 to 101.8% of the declared amount. Spectrophotometric determinations, which do not discriminate between the drug and impurities, gave 95.4-101.8% of declared. One commercial sample of bulk powder was assayed. 相似文献
10.
P S Jaglan B L Cox T S Arnold M F Kubicek D J Stuart T J Gilbertson 《Journal of the Association of Official Analytical Chemists》1990,73(1):26-30
A liquid chromatographic (LC) method has been developed for the determination of the desfuroylceftiofur metabolite of ceftiofur as a residue in the plasma of animals. Plasma sample in 0.1M pH 8.7 phosphate buffer containing dithioerythritol is incubated under nitrogen for 15 min at 50 degrees C. The sample is centrifuged, charged to a C18 cartridge, and washed with 0.1M ammonium acetate. The desfuroylceftiofur residue on the cartridge is derivatized by adding 0.1M ammonium acetate containing iodoacetamide and letting the cartridge stand in the dark for 30 min. The cartridge is then drained and rinsed, and the desfuroylceftiofur acetamide is eluted with methanol. The mixture is evaporated to dryness, dissolved in pH 10.6 sodium hydroxide, and charged to a SAX cartridge. The derivative is eluted with 2% acetic acid, reduced in volume, and dissolved in mobile phase for liquid chromatography. The LC system includes a C8 column and guard cartridge with UV detection at 254 nm. The gradient mobile phase (flow rate 1 mL/min) is 0.01M pH 5 ammonium acetate programmed to 29% methanol-water (60 + 40) in 25 min. Recoveries were 90-100% with a sensitivity of 0.1 ppm or less. The procedure has been applied to the plasma of cattle, rats, horses, pigs, and dogs. 相似文献
11.
J F Brower 《Journal of the Association of Official Analytical Chemists》1984,67(4):674-676
A normal phase liquid chromatographic (LC) method for the determination of prednisolone in tablets and bulk drugs was studied by 7 analysts. An LC system, consisting of a methanol-water-ethylene dichloride-acetic acid mobile phase and a silica column, was used to analyze bulk drugs, individual tablets, and composite samples. Analysts were supplied with 16 samples, including simulated formulations, composites of commercial tablets, intact tablets, and bulk drug substances. Results agreed with those obtained by the author. The coefficients of variation of the analysts' results ranged from 1.34% for bulk drugs to 2.14% for tablet composites. The LC method is suggested as an alternative to the official AOAC and USP XX blue tetrazolium colorimetric methods. 相似文献
12.
A procedure is described for the quantitation of Zoalene (3,5-dinitro-o-toluamide) and its 2 major monoamino metabolites in chicken tissues. The method includes blender extraction of tissue with chloroformethyl acetate (1 + 1), adsorption of the drug and metabolites on neutral alumina, and subsequent elution of the residues with pH 3.5 formate buffer-methanol (6.5 + 3.5). Recovered residues were separated on a 5 micron C18 column with the alumina eluting solvent as the LC mobile phase. The parent drug and metabolites were detected and quantitated with an electrochemical detector in the reductive mode with a minimum level of reliable measurement of 0.1 ppm. Overall mean recoveries greater than 85% were obtained with Zoalene and its 2 monoamino metabolites in breast, thigh, and liver tissues fortified with 0.25-2.00 ppm. The results on tissues from chickens fed a diet containing 0.0125% Zoalene are presented. 相似文献
13.
R A Rude J T Peeler N G Risty 《Journal of the Association of Official Analytical Chemists》1987,70(6):1000-1002
Ethyl acetate and diethyl ether were compared for their ability to recover Ascaris spp. and Trichuris spp. eggs from seeded milorganite, liquid sludge, and cabbage. Concentrations of 10, 100, and 1000 eggs/10 g test sample were prepared for 20 replicates of each product. The use of diethyl ether yielded fewer eggs/10 g than did ethyl acetate in 5 of 6 sets of data. For Ascaris spp., recovery from cabbage was 10 times higher with ethyl acetate at the higher concentration than with diethyl ether. For Trichuris spp., recovery from liquid sludge was slightly higher with diethyl ether for all egg concentrations. The other results ranged from 0 to 23% difference in recovery for the 2 agents. Depending on the parasites in question and the products to be screened, the substitution of ethyl acetate for diethyl ether may be significant. 相似文献
14.
P M Lacroix D Moir E G Lovering 《Journal of the Association of Official Analytical Chemists》1990,73(4):521-525
A liquid chromatographic method for the assay of pindolol and related compounds in the bulk drug has been developed. The method resolves 6 known and several unknown impurities from the drug and each other by using a nitrile column, an acetonitrile-sodium acetate buffer (35 + 65), and a UV detector set at 219 nm. Minimum quantifiable amounts of impurities are 0.02% or less relative to the drug. Ten lots of pindolol raw material were evaluated for purity and drug content. Total levels of impurities in these samples, quantitated against pindolol, ranged from about 0.03 to 0.24%. Assay results were within the range of 98.5 to 101.5%. 相似文献
15.
Milk immunoglobulin G (IgG), separated with protein G affinity chromatography, and IgG in colostral whey were encapsulated by 0.5% (w/v) of Tween 80, sucrose stearate, or soy protein, which were used as secondary emulsifiers in the water in oil in water type multiple emulsion. The residual contents of separated IgG and IgG in colostral whey, ranging from 58.7 to 49.7% and from 13.2 to 21.3%, respectively, in the inner water phase (water phase surrounded by oil phase) with emulsifiers were determined by ELISA. However, the emulsion stability decreased after 24 h, and the residual IgG content in the inner water phase was lowered. Encapsulation of IgG in the multiple emulsion increased the stability of separated IgG against acid (pH 2.0) and alkali (pH 12.0) by 21-56% and 33-62%, respectively, depending on the emulsifier used. Moreover, multiple emulsion also provided a remarkable protective effect on separated IgG stability against proteases. The residual contents of separated IgG in multiple emulsion, using Tween 80 as secondary emulsifier, incubated for 2 h with pepsin (pH 2.0) and trypsin and chymotrypsin (pH 7.6) (enzyme/substrate = 1/20) were 35.4, 72.5, and 82.3%, whereas those of separated IgG in enzyme solution were only 7.2, 33. 1, and 35.2%, respectively. However, the separated IgG loss during the preparation of multiple emulsion was almost 41-50%. 相似文献
16.
Simple analytical method for organophosphorus pesticide determination in unpolished rice, using removal of fats by zinc acetate 总被引:1,自引:0,他引:1
K Adachi N Ohokuni T Mitsuhashi 《Journal of the Association of Official Analytical Chemists》1984,67(4):798-800
A rapid and simple method is developed for the determination of organophosphorus pesticides in unpolished rice. The new method incorporated acetonitrile-water (1 + 1) extraction, removal of fats by zinc acetate, and further cleanup on an activated charcoal chromatographic column. The higher fatty acids in the extract react rapidly with zinc acetate to form insoluble zinc carboxylates, which precipitate. Additional interferences were cleaned up on an activated charcoal chromatographic column, and organophosphorus pesticides adsorbed on the activated charcoal were eluted with acetone-hexane. Dimethoate is not retained on the activated charcoal and must be extracted with dichloromethane from the first acetonitrile-water eluate. Pesticides are measured by flame photometric gas chromatography. Recoveries from 50 g unpolished rice samples fortified with 5-50 micrograms diazinon, 6-30 micrograms parathion, 8-40 micrograms fenitrothion and IBP, 10-50 micrograms dimethoate and fenthoate, 20-100 micrograms malathion, or 40-200 micrograms EPN ranged from 75.7 to 95.8%. 相似文献
17.
《Communications in Soil Science and Plant Analysis》2012,43(3-4):485-501
Abstract Studies were conducted to ascertain the suitability of mineral wool (MW), either alone or in combination with sphagnum peat moss, as a substrate for potted greenhouse plants. Two types of hydrophyllic mineral wools, cleaned mineral wool (CMW) and uncleaned mineral wool (UMW), were used. Unamended CMW had a low bulk density, excellent water holding capacity, good aeration, but a high pH. Once peat moss was added to the CMW, bulk density remained low, water holding capacity remained good, and the pH dropped to a more suitable level. Unamended UMW had a high bulk density, good water holding capacity, poor aeration, and a high pH. Once peat moss was added to UMW, bulk density decreased, water holding capacity remained good, aeration increased, and the pH decreased to a more optimal level. CMW and UMW, were used unamended, as well as amended with 25%, 50%, and 75% peat moss. Two bedding plants, Impatiens walleriana ’Dazzler Violet’ and Begonia semperflorens ’Whiskey’ were grown for six and nine weeks respectively, and Euphorbia pulcherrima ’Glory’ was grown for 20 weeks, in nine different substrates. Plants grown in unamended CMW and UMW were generally smaller in size and lower in fresh weight than plants grown in 50% MW/50% peat moss. The plants grown in MW with either 25% or 75% peat moss were similar in size and weight to plants grown in 50% MW/50% peat moss. Plant tissue analysis showed that generally plants were receiving adequate nutrition. 相似文献
18.
G A Perfetti F L Joe G W Diachenko 《Journal of the Association of Official Analytical Chemists》1989,72(6):903-906
A liquid chromatographic (LC) method is described for the determination of sulfite in grapes and certain grape products. Sulfite is extracted from grapes with aqueous formaldehyde solution buffered at pH 5; free sulfite is converted to hydroxymethylsulfonate (HMS), which is extremely stable at pH 3-7. Subsequent heating to 80 degrees C for 30 min converts reversibly bound forms of sulfite to HMS. The extract is then analyzed by reverse-phase ion-pairing liquid chromatography, using a C18 column and a mobile phase of aqueous 0.005 M tetrabutylammonium ion in 0.05 M acetate, pH 4.7, and a flow rate of 1 mL/min. Aqueous KOH is added to the eluate to convert HMS to free sulfite, which is then treated with 5,5'-dithiobis[2-nitrobenzoic acid]. This reaction produces the 3-carboxy-4-nitrothiophenolate anion, which is determined by measurement of electronic absorption at 450 nm. For grapes spiked with HMS at 5-20 ppm (as SO2), recoveries ranged from 92 to 112%, with a coefficient of variation of 4.6%. The method was also used to determine sulfite in various grape products. Results were comparable to those obtained by the AOAC official Monier-Williams method. 相似文献
19.
W P Cochrane M Lanouette 《Journal of the Association of Official Analytical Chemists》1979,62(1):100-106
An ion-suppression reverse phase high pressure liquid chromatographic method is described for determining naphthaleneacetic acid (NAA) residues in apples. Samples are extracted with acidic chloroform, filtered through pre-acidified Hy-Flo Supercel, and cleaned up by acid-base partitioning. The extract can be successfully chromatographed on either a muLiChrosorb NH2 or muBondapak C18 column and quantitated by using a variable wavelength ultraviolet detector set at 220 nm. The mobile phase is acetonitrile-water (20 + 80) buffered to pH 3.5 (MULiChrosorb column) or pH 5.2 (MUBondapak column) and flowing at 1.0--2.0 ml/min. Recoveries ranged from 86 to 98%. The minimum detectable amount was 0.5 ng, which easily permitted the quantitation of 0.01 ppm NAA in 50 g sample. A fluorometric detector was 4 times as sensitive, using an excitation wavelength of 220 mm and monitoring the emission at 340 nm. For this detector, the minimum detectable amount was 0.12 ng NAA. 相似文献
20.
通过比较不同的提取溶剂和使用量,就水体中毒死蜱和TCP残留提取的效果及不同的流动相组成和比例对毒死蜱和TCP测定的影响,建立了水体中毒死蜱及TCP的HPLC残留分析方法。结果表明,水体中毒死蜱和TCP最佳提取溶剂为乙酸乙酯,提取次数为2次,用量分别为50和30mL。色谱条件为:流动相为甲醇:水=90:10或乙腈:水=90:10,流速1mL·min^-1;紫外检测波长300nm。当流动相为甲醇:水=90:10时,毒死蜱和TCP的保留时间分别为6.4和3.6min;当流动相为乙腈:水=90:10时,其保留时间分别为5.6和2.5min。毒死蜱和TCP的检出限分别为0.5和0.15ng。当毒死蜱和TCP在水中的添加浓度为0.01~5mg·L^-1时,标准添加回收率分别为91.4%-105.1%和90.6%~105.4%,变异系数分别为0.99%~4.12%和0.29%~9.33%。水样中毒死蜱和TCP的最小检出浓度分别为2和0.6ng·mL^-1。 相似文献