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使用液相色谱 - 质谱联用技术对(RS)-非索非那定进行对映体拆分,并将其作为非对映体酰胺和酸酐衍生物进行增强检测。

Enantioseparation of (RS)-fexofenadine and enhanced detection as the diastereomeric amide and anhydride derivatives using liquid chromatography-mass spectrometry.

作者信息

Malik Poonam, Bhushan Ravi

机构信息

Department of Chemistry, Indian Institute of Technology Roorkee, India.

出版信息

Biomed Chromatogr. 2018 Jul;32(7):e4217. doi: 10.1002/bmc.4217. Epub 2018 Apr 15.

Abstract

Enantioselective analysis of (RS)-fexofenadine was carried out by achiral HPLC via a derivatization approach using N-hydroxy-benzotriazolyl-(S)-naproxen ester (synthesized for this purpose) and three chirally pure amines as chiral derivatizing reagents. There occurred formation of amide and anhydride types of diastereomeric derivatives. These were separated and isolated by HPLC (analytical and preparative). The structures and configurations were verified via recording full-scan product ion mass spectra using LC-MS, HNMR spectra, Chem3D Pro 12.0 software and the software Gaussian 09 Rev.A.02 program and hybrid density functional B3LYP with 6-31G basis set supplemented with polarimetry. Experimental conditions for synthesis and separations were optimized and the elution order was established. Analytical separation was performed on a C analytical column with different ratios of MeCN-TEAP buffer and MeOH-TEAP buffer (v/v) adjusted to pH 7.5 as mobile phase at a flow rate of 0.7 mL min . Detection was performed via UV absorbance at 225 nm. The method was validated in accordance with International Conference on Harmonization guidelines. The detection limits were 6.25 and 7.87 ng mL for first and second eluting diastereomeric derivatives, respectively.

摘要

通过使用N-羟基苯并三唑基-(S)-萘普生酯(为此目的合成)和三种手性纯胺作为手性衍生试剂的衍生化方法,采用非手性高效液相色谱法对手性(RS)-非索非那定进行对映体选择性分析。生成了酰胺和酸酐类型的非对映体衍生物。通过高效液相色谱法(分析型和制备型)对这些衍生物进行分离和纯化。通过使用液相色谱-质谱联用仪记录全扫描产物离子质谱、核磁共振氢谱、Chem3D Pro 12.0软件以及Gaussian 09 Rev.A.02程序和采用6-31G基组并辅以旋光测定法的混合密度泛函B3LYP对结构和构型进行验证。优化了合成和分离的实验条件并确定了洗脱顺序。在C分析柱上进行分析分离,以不同比例的乙腈-四乙铵缓冲液和甲醇-四乙铵缓冲液(v/v)调节至pH 7.5作为流动相,流速为0.7 mL/min。通过在225 nm处的紫外吸光度进行检测。该方法根据国际协调会议指南进行了验证。对于第一个和第二个洗脱的非对映体衍生物,检测限分别为6.25和7.87 ng/mL。

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