Simultaneous determination of eight estrogens and their metabolites in serum using liquid chromatography with electrochemical detection

Piwowarska, Jadwiga; Radowicki, Stanisław; Pachecka, J

doi:10.1016/j.talanta.2009.11.069

Cited by 28 publications

(16 citation statements)

References 22 publications

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“…This site may have its conformation altered by the presence or absence of substrate at the active site, such that the affinity for (Westhoff et al, 2010). b In pregnant women (Piwowarska et al, 2010). c For patients given a 150-mg dose twice a day for 7 days (Brunton et al, 2006).…”

Section: Discussionmentioning

confidence: 99%

Inhibition of Human Liver Aldehyde Oxidase: Implications for Potential Drug-Drug Interactions

Barr

Jones

2011

Drug Metab Dispos

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ABSTRACT:During the course of our research efforts to understand the kinetics of human aldehyde oxidase as a xenobiotic-clearing enzyme, we investigated the effect of eight different inhibitors on the oxidation of the probe substrate phthalazine. Saturation kinetic parameters for phthalazine oxidation in human liver cytosol were found to be the following:Inhibitory potency of the inhibitors tested ranged from 0.1 to 5 M. Of the eight different inhibitor compounds tested, seven were observed to inhibit through a mixed mode and one through a strictly competitive mode. A ratio of the K ii and K is values was used to assess the relative competitiveness of each inhibitor. For the mixed inhibitors, the mode of inhibition varied from mostly uncompetitive to predominantly competitive (K ii /K is values ranging from 0.1 to 15). The implications for potential drug-drug interactions and inhibition mechanism are discussed. We found two inhibitors, clozapine and chlorpromazine, that have a moderate predicted risk of drug-drug interactions based on the K i value relative to the inhibitor concentration in human plasma, having a calculated [I]/K i value of 0.4 and 0.8, respectively.

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Section: Discussionmentioning

confidence: 99%

Inhibition of Human Liver Aldehyde Oxidase: Implications for Potential Drug-Drug Interactions

Barr

Jones

2011

Drug Metab Dispos

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“…For analysis of blood levels of 17b-estradiol by HPLC (Fernandez et al, 1993;Piwowarska et al, 2010), blood was treated with 10M NaOH (0.5 mL by mL of blood) and then shaken for 5 minutes. The mixture was then extracted with 5 mL of diethyl ether by rotomixing for 10 minutes.…”

Section: Hplc and Determination Of Blood Levels Of Estrogenmentioning

confidence: 99%

Critical period for dopaminergic neuroprotection by hormonal replacement in menopausal rats

Rodríguez‐Pérez

Borrajo

Valenzuela

et al. 2015

Neurobiology of Aging

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“…The selected target analyte to evaluate the suitability of the hybrid nanomaterial-based biosensor was estriol ((16α,17β)-estra-1,3,5(10)-triene-3,16,17-triol), a phenolic estrogen hormone widely used in the treatment of urogenital diseases in menopausal women. This drug, classified as endocrine disrupting compound [18,19], is commonly eliminated in the urine of patients and is not completely degraded during the treatment of sewage becoming a potential environmental risk [20]. The determination of estriol in human and environmental samples has been mainly performed by gas and liquid chromatography [19,[21][22][23] and spectrophotometric techniques [24][25][26], but these analytical procedures require exhaustive pre-treatment of samples prior to analysis.…”

Section: Introductionmentioning

confidence: 99%

“…This drug, classified as endocrine disrupting compound [18,19], is commonly eliminated in the urine of patients and is not completely degraded during the treatment of sewage becoming a potential environmental risk [20]. The determination of estriol in human and environmental samples has been mainly performed by gas and liquid chromatography [19,[21][22][23] and spectrophotometric techniques [24][25][26], but these analytical procedures require exhaustive pre-treatment of samples prior to analysis. Several authors have proposed electroanalytical techniques as reliable alternatives for estriol detection [18,20,27], and succesful results have been achieved by using proper combination of new advanced materials and highly selective bioreceptor on the transducer interfase.…”

Section: Introductionmentioning

confidence: 99%

Reduced graphene oxide-Sb2O5 hybrid nanomaterial for the design of a laccase-based amperometric biosensor for estriol

Cincotto

Canevari

Machado

et al. 2015

Electrochimica Acta

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Reduced graphene oxide-Sb2O5 hybrid nanomaterial for the design of a laccase-based amperometric biosensor for estriol, Electrochimica Acta http://dx. AbstractA novel reduced graphene oxide/Sb2O5 hybrid nanomaterial was prepared by a one-pot reaction process. The nanomaterial was characterized by different spectroscopic, microscopic and electrochemical techniques, demonstrating that the graphene sheets were doped with a Sb2O5 thin film. A glassy carbon electrode coated with the hybrid material was further employed as support for the covalent immobilization of laccase to develop an electrochemical biosensor for estriol. The enzyme biosensor showed high sensitivity (275 mA/M) and fast analytical response (4 s) for the hormone, with a limit of detection of 11 nM in the range of 25 nM to 1.03 µM. The biosensor showed high selectivity for the analytical detection of estriol.

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Simultaneous determination of eight estrogens and their metabolites in serum using liquid chromatography with electrochemical detection

Cited by 28 publications

References 22 publications

Inhibition of Human Liver Aldehyde Oxidase: Implications for Potential Drug-Drug Interactions

Inhibition of Human Liver Aldehyde Oxidase: Implications for Potential Drug-Drug Interactions

Critical period for dopaminergic neuroprotection by hormonal replacement in menopausal rats

Reduced graphene oxide-Sb2O5 hybrid nanomaterial for the design of a laccase-based amperometric biosensor for estriol

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