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首页> 外文期刊>Journal of Pharmaceutical and Biomedical Analysis: An International Journal on All Drug-Related Topics in Pharmaceutical, Biomedical and Clinical Analysis >LC-UV/MS methods for the analysis of prochelator-Boronyl salicylaldehyde isonicotinoyl hydrazone (BSIH) and its active chelator salicylaldehyde isonicotinoyl hydrazone (SIH)
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LC-UV/MS methods for the analysis of prochelator-Boronyl salicylaldehyde isonicotinoyl hydrazone (BSIH) and its active chelator salicylaldehyde isonicotinoyl hydrazone (SIH)

机译:LC-UV / MS方法分析肉豆蔻酮-硼基水杨醛异烟酰yl(BSIH)及其活性螯合剂水杨醛异烟酰(SIH)

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摘要

Salicylaldehyde isonicotinoyl hydrazone (SIH) is an intracellular iron chelator with well documented potential to protect against oxidative injury both in vitro and in vivo. However, it suffers from short biological half-life caused by fast hydrolysis of the hydrazone bond. Recently, a concept of boronate prochelators has been introduced as a strategy that might overcome these limitations. This study presents two complementary analytical methods for detecting the prochelator-boronyl salicylaldehyde isonicotinoyl hydrazone-BSIH along with its active metal-binding chelator SIH in different solution matrices and concentration ranges. An LC-UV method for determination of BSIH and SIH in buffer and cell culture medium was validated over concentrations of 7-115 and 4-115 mu M, respectively, and applied to BSIH activation experiments in vitro. An LC-MS assay was validated for quantification of BSIH and SIH in plasma over the concentration range of 0.06-23 and 0.24-23 mu M, respectively, and applied to stability studies in plasma in vitro as well as analysis of plasma taken after i.v. administration of BSIH to rats. A Zorbax-RP bonus column and mobile phases containing either phosphate buffer with EDTA or ammonium formate and methanol/acetonitrile mixture provided suitable conditions for the LC-UV and LC-MS analysis, respectively. Samples were diluted or precipitated with methanol prior to analysis. These separative analytical techniques establish the first validated protocols to investigate BSIH activation by hydrogen peroxide in multiple matrices, directly compare the stabilities of the prochelator and its chelator in plasma, and provide the first basic pharmacokinetic data of this prochelator. Experiments reveal that BSIH is stable in all media tested and is partially converted to SIH by H2O2. The observed integrity of BSIH in plasma samples from the in vivo study suggests that the concept of prochelation might be a promising strategy for further development of aroylhydrazone cytoprotective agents. (C) 2014 Elsevier B.V. All rights reserved.
机译:水杨醛异烟酰yl(SIH)是一种细胞内铁螯合剂,在体外和体内均具有防止氧化损伤的潜力。然而,它由于by键的快速水解而具有较短的生物学半衰期。最近,已经引入了硼酸螯合剂的概念作为可以克服这些限制的策略。这项研究提出了两种互补的分析方法,用于在不同溶液基质和浓度范围内检测链烷烃-硼酰基水杨醛异烟酰ino-BSIH及其活性金属结合螯合剂SIH。用于缓冲液和细胞培养基中BSIH和SIH测定的LC-UV方法分别在7-115和4-115μM的浓度下得到验证,并应用于体外BSIH活化实验。验证了LC-MS分析可分别定量测定浓度范围为0.06-23和0.24-23μM的血浆中BSIH和SIH,并将其应用于体外血浆稳定性研究以及静脉注射后血浆分析。给大鼠服用BSIH。 Zorbax-RP色谱柱和含有EDTA磷酸盐缓冲液或甲酸铵和甲醇/乙腈混合物的流动相分别为LC-UV和LC-MS分析提供了合适的条件。在分析之前,将样品用甲醇稀释或沉淀。这些分离的分析技术建立了首个经过验证的方案,以研究过氧化氢在多种基质中对BSIH的活化作用,直接比较了螯合剂及其螯合剂在血浆中的稳定性,并提供了该络合剂的第一批基本药代动力学数据。实验表明,BSIH在所有测试介质中均稳定,并被H2O2部分转化为SIH。从体内研究中观察到的血浆样品中BSIH的完整性表明,螯合的概念可能是进一步开发酰yl细胞保护剂的有前途的策略。 (C)2014 Elsevier B.V.保留所有权利。

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