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生物样品中手性有机磷酸酯梭曼的测定。

Assay of the chiral organophosphate, soman, in biological samples.

作者信息

de Jong L P, Bijleveld E C, van Dijk C, Benschop H P

出版信息

Int J Environ Anal Chem. 1987;29(3):179-97. doi: 10.1080/03067318708079835.

Abstract

The anticholinesterase, soman, (CH3)3CC(H)CH3O(CH3)P(O)F, consists of four stereoisomers assigned as C(+/-)P(+/-)-soman in which C stands for chirality in the pinacolyl moiety and P for chirality at phosphorus. The four stereoisomers are separated by gas chromatography on an optically active Chirasil-Val column, synthesized and coated in house, or on a Chirasil-Val column identical with the commercially available column when combined with a Carbowax 20M column. This method in combination with an assay based on acetylcholinesterase inhibition shows that the two isomers which do not have anticholinesterase activity, i.e. C(+/-)P(+/-)-soman, are rapidly degraded in rat blood due to hydrolysis by phosphorylphosphatases. Epimeric soman isomers, e.g. C(+/-)P(-)-soman, can be separately assayed on a Carbowax or a CPSil 8 column, using 2H-labeled soman isomers as internal standards. 2H-labeled soman stereoisomers serve as internal standards in GC-assay of all four stereoisomers on Chirasil-Val. For work-up of the four stereoisomers from rat blood the sample is first stabilized by acidification to pH 4.2 at 0 degree C to suppress hydrolysis by phosphorylphosphatases, addition of aluminum ions for complexation of fluoride ions to prevent regeneration of C(+/-)P(-)-soman by free fluoride ions from soman-inhibited carboxylesterase, and addition of (CH3)3CCH2O(CH3)P(O)F to occupy covalent binding sites for C(+/-)P(-)-soman, before extraction with a Sep-Pak C18 cartridge and elution with ethyl acetate. Using a splitless or on-column injection technique and alkali flame ionization detection, the minimum detectable concentration is 30 pg/3-ml blood sample.

摘要

抗胆碱酯酶索曼,(CH3)3CC(H)CH3O(CH3)P(O)F,由四种立体异构体组成,被指定为C(+/-)P(+/-)-索曼,其中C代表频那醇基部分的手性,P代表磷原子处的手性。这四种立体异构体可通过气相色谱法在自制的涂有光学活性Chirasil-Val固定液的柱上,或在与市售柱相同的Chirasil-Val柱上并结合Carbowax 20M柱进行分离。该方法与基于乙酰胆碱酯酶抑制的测定法相结合表明,两种没有抗胆碱酯酶活性的异构体,即C(+/-)P(+/-)-索曼,在大鼠血液中因磷酰磷酸酶的水解作用而迅速降解。差向异构的索曼异构体,如C(+/-)P(-)-索曼,可使用2H标记的索曼异构体作为内标,在Carbowax或CPSil 8柱上分别进行测定。2H标记的索曼立体异构体在Chirasil-Val柱上用于所有四种立体异构体的气相色谱测定的内标。对于从大鼠血液中处理这四种立体异构体,样品首先在0℃酸化至pH 4.2以抑制磷酰磷酸酶的水解作用,加入铝离子以络合氟离子,防止被索曼抑制的羧酸酯酶释放的游离氟离子使C(+/-)P(-)-索曼再生,并加入(CH3)3CCH2O(CH3)P(O)F占据C(+/-)P(-)-索曼的共价结合位点,然后用Sep-Pak C18柱进行萃取并用乙酸乙酯洗脱。使用不分流进样或柱上进样技术以及碱火焰离子化检测,最低可检测浓度为30 pg/3-ml血样。

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