Development of a capillary electrophoretic method for determination of ketorolac enantiomers in human plasma using cationic β-cyclodextrin derivative as a chiral selector

A novel approach for the separation of ketorolac enantiomers by capillary electrophoresis is presented. A cationic β-cyclodextrin derivative based on imidazole was synthesized and used as a chiral selector in the background electrolyte. The influence of pH and ionic strength of background electrolyte, as well as cationic β-cyclodextrin derivative concentration on the resolution of ketorolac enantiomers, was investigated. The highest value of the resolution for ketorolac enantiomers was 1.46 when the background electrolyte consisted of 25 mM NaH₂PO₄ (pH 6.4) with 1 mM 1-butyl-3-β-cyclodextrinimidazolium tosylate. Additionally, the possibilities of cationic derivatives for the separation of ketoprofen enantiomers were shown (peak resolution 1.06). The two-step preconcentration mode was developed to reduce the limit of detection of individual enantiomers. The proposed approach was successfully applied to determine ketorolac enantiomers in tablet “Ketorol express” and human plasma. The calibration range of ketorolac enantiomers for plasma samples was 0.25–2.50 μg/ml with coefficients of determination ≥ 0.99. The relative standard deviation both of the peak area and migration time was less than 15%, as well as the accuracy ranged from 90.1% to 110.2% for both analytes. The limits of detection were 44 and 55 ng/ml for R- and S-ketorolac. The quantity of ketorolac in plasma was verified with high-performance liquid chromatography.     

Development and validation of a chiral HPLC method for rapid screening of allylic alcohol asymmetric epoxidation processes

A simple and rapid HPLC method has been developed using a polysaccharide chiral stationary phase (Chiralpak AD-H) for the resolution of glycidyl tosylate enantiomers. These compounds were obtained by asymmetric epoxidation of allyl alcohol with chiral titanium-tartrate complexes as catalyst after in situ derivatization of the intermediate glycidols. Separations were achieved using two types of mobile phase: a normal-phase (n-hexane), and a polar-phase (methanol or acetonitrile). The influence of the type and concentration of organic modifier in the mobile phase (ethanol or 2-propanol), the flow rate and the column temperature was investigated. In normal-phase mode, the optimized conditions were: n-hexane/ethanol 70/30 (v/v) at a flow rate of 1.2 mL min⁻¹ and 40 °C. In polar-phase mode, the optimized conditions were: methanol at a flow rate of 0.8 mL min⁻¹ and 20 °C. In both cases, analysis time was ≤11 min and the chiral resolution was ≥2. Nevertheless, due to the better Rs obtained in normal-phase mode, only this method was validated to avoid peaks overlapping in real samples. This method was found to be linear in the 5-300 μg mL⁻¹ range (R² > 0.999) with an LOD of 1.5 μg mL⁻¹ for both glycidyl tosylate enantiomers. Repeatability and intermediate precision at three different concentrations levels were below 0.5 and 7.2% R.S.D. for retention time and area, respectively. This method was applied successfully for the determination of glycidyl tosylate enantiomers after in situ derivatization of glycidols obtained in allylic alcohol asymmetric epoxidation processes with chiral titanium-tartrate complexes as catalysts.     

Enantiomeric Enrichments via the Self‐Disproportionation of Enantiomers (SDE) by Achiral,Gravity‐Driven Column Chromatography: a Case Study Using N‐(1‐Phenylethyl)acetamide for Optimizing the Enantiomerically Pure Yield and Magnitude of the SDE

This work explores the self‐disproportionation of enantiomers (SDE) via achiral, gravity‐driven column chromatography as typically used in laboratory settings for the purpose of enantiomeric enrichment using N‐(1‐phenylethyl)acetamide (PEA) as a case study. The major finding of this work is the very large magnitude of the SDE for PEA across a variety of conditions and broad range of starting ee values, thereby facilitating a simple, reliable, and predictable means of obtaining enantiomerically pure samples. For example, starting with a sample of PEA of ee as low as 28%, a single column run yielded an enantiomerically pure sample (>99.9% ee) from the first fractions and a significantly enantiomerically depleted sample (<17% ee) from the final fractions. An assessment of SDE via achiral, gravity‐driven column chromatography was also rendered with regard to the differing objectives that workers might target – a large magnitude of the SDE, obtaining an optimum sample of desired ee, or preparative‐scale separation of the excess enantiomer. Overall, it can be considered that the SDE phenomenon via achiral, gravity‐driven column chromatography – readily applicable in the usual laboratory settings – is a simple and convenient method for enantiomeric enrichment with a high degree of proficiency. Advantages of SDE via achiral, gravity‐driven column chromatography over conventional fractional recrystallization for the enantiomeric enrichment of amides/amines, and applicable also to many other classes of compounds as well, are discussed.     

Isotope Effects during Metabolism of (+)- and (−)- Trans Tramadol Isotopomers by Human Liver Microsomes

Abstract

As for the unlabelled (±)-1(e)-(m-methoxyphenyl)-2(e)-(dimethylaminomethyl)cyclohexane 1(a)-ol, tramadol, (T), pronounced stereochemical effects were observed for the isotopomers with regard to the extent of formation of O- and N-demethylated metabolites. The pharmacological active O-demethylated metabolite M1 was formed from the unlabelled as well as from the labelled (+)-tramadols about 6 times less than from the corresponding (?)-T. In contrast, the N-demethylated metabolite M2 was formed from the (+)-tramadols about 1.5 times more than from the corresponding (?)-T. These steric effects were modulated by the smaller apparent isotope effects for the isotopomers. Isotope effects were expressed as k_H/k_D (calculated from concentrations) and as ^DV, ^DV/K and ^HK_m/^DK_m (from Eadie-Hofstee plots).     

Intermittent simulated moving bed chromatography: 3. Separation of Tröger's base enantiomers under nonlinear conditions

One of the modified simulated moving bed (SMB) processes, the intermittent SMB (I-SMB) process, has been recently analyzed theoretically [1] and its superior performance compared to the conventional SMB process has been demonstrated at a rather low total feed concentration through experiments and simulations [2]. This work shows that the I-SMB process outperforms the conventional SMB process also at high feed concentration where the species are clearly subject to a nonlinear adsorption isotherm. In the case of the separation of the Tröger's base's enantiomers in ethanol on ChiralPak AD, the two processes operated in a six-column 1-2-2-1 configuration (one column in sections 1 and 4 and two columns in sections 2 and 3) and in a four-column 1-1-1-1 configuration (one column in each section) are compared at high feed concentration through both experiments and simulations. Even under nonlinear conditions the four column I-SMB process can successfully separate the two enantiomers achieving purity levels as high as the two six column processes and exhibiting better productivity.     

Interaction of Thyroxine with 7 Hydroxycoumarin: A Fluorescence Quenching Study

The interaction between thyroxine hormone and 7 hydroxycoumarin (7HC) was investigated using fluorescence quenching method. The experimental results showed that thyroxine could quench the fluorescence of 7HC by forming the 7HC–thyroxine complex with static quenching. The apparent binding constants (K) between 7HC and thyroxine were determined to be 1.51 × 10⁴ (297 K) and 9.06 × 10³ (310 K). The binding sites (n) 0.98 ± 0.1. The thermodynamic parameters showed that the interaction between 7HC and thyroxine was driven mainly by hydrogen bonding interactions and van der Waals force. Calibration for thyroxine, based on quenching titration data, was linear in the concentration range 2.0 × 10⁻⁸ to 3.0 × 10⁻⁷ mol/l. The relative standard deviation was 2.58% for 2.0 × 10⁻⁷ mol/l thyroxine (n = 4) and the 3σ limit of detection was 3.42 × 10⁻⁸ mol/l in cationic surfactant CTAB medium.     

D-，L-和DL-奥硝唑随温度变化的太赫兹光谱

利用太赫兹时域光谱 （terahertz time domain spectroscopy,THz-TDS） 技术,在6 K到298 K之间,测量了D-,L-和DL-奥硝唑随温度变化的太赫兹（THz）光谱.实验结果表明,在0.3到2.5 THz波段,在常温时D-和L-奥硝唑的吸收峰几乎相同,但与DL-奥硝唑的吸收峰存在差异,到低温时这种差异变得更加明显,为鉴别奥硝唑旋光异构体与其消旋体提供了新的方法;低温时观察到了在常温时很难分辨的吸收峰,为振动模式指认提供更多的信息;随着温度的升高,吸收峰中心频率朝着低频的方向单调偏移,通过对实验数据的拟合,发现振动模式随温度变化符合Bose-Einstein统计规律.最后对奥硝唑旋光异构体及其消旋体分子进行量子化学计算,并模拟得到0.2—2.5 THz的低频振动光谱,根据光谱实验结果,从分子水平上对其特征吸收信号进行了理论分析. 关键词： 振动光谱 奥硝唑 对映异构体 THz时域光谱技术     

Fully automated high-performance liquid chromatographic separation of DL-amino acids derivatized witho-phthaldialdehyde together withN-isobutyryl-cysteine. Application to food samples

Summary A method is presented that enables the fully automated precolumn derivatization of mixtures of DL-amino acids (DL-AA) witho-phthaldialdehyde together withN-isobutyryl-L(orD)-cysteine. HPLC on a 250 mm×4 mm i.d. column packed with Shandon Hypersil ODS, 5 μm, and a linear gradient formed from 23 mM sodium acetate (pH 6.0) and methanol/acetonitrile (600 ml+50 ml) separates completely an AA standard composed of 17 pairs of DL-AA (including Asn and Gln), Gly and the internal standard L-homo-Arg, within 75 min at a flow rate at 1 ml/min. Applications are shown of the determination of free D-AA isolated from an orange juice concentrate and from soy sauce, and the detection of D-AA in a gelatine total hydrolysate. In the case of these foodstuffs fluorescence detection (excitation at 230 nm, emission at 445 nm) allows the routine detection of 5–10 pmol per AA; and approx. 0.2–1% D-AA, in an excess of L-AA, are quantifiable. Presented in part at the “International Symposium on Separation of Peptides, Proteins and Polynucleotides”, October 29–31, 1990, Wiesbaden (abstract 620), ANAKON '91, April 22–24, Baden-Baden (abstract C 5), and at the “15th International Symposium on Column Liquid Chromatography”, June 3–7, 1991, Basel (abstract P26/2).