E. N. Semenistaya scite author profile

Growth hormone releasing peptides (GHRPs) stimulate secretion of endogenous growth hormone and are listed on the World Anti-Doping Agency (WADA) Prohibited List. To develop an effective method for GHRPs anti-doping control we have investigated metabolites of GHRP-1, GHRP-2, GHRP-6, Hexarelin, and Ipamorelin in urine after nasal administration. Each compound was administrated to one volunteer. Samples were collected for 2 days after administration, processed by solid-phase extraction on weak cation exchange cartridges and analyzed by means of nano-liquid chromatography - high resolution mass spectrometry. Six metabolites of GHRP-1 were identified. GHRP-1 in the parent form was not detected. GHRP-1 (2-4) free acid was detected in urine up to 27 h. GHRP-2, GHRP-2 free acid and GHRP-2 (1-3) free acid were detected in urine up to 47 h after administration. GHRP-6 was mostly excreted unchanged and detected in urine 23 h after administration, its metabolites were detectable for 12 h only. Hexarelin and Ipamorelin metabolized intensively and were excreted as a set of parent compounds with metabolites. Hexarelin (1-3) free acid and Ipamorelin (1-4) free acid were detected in urine samples after complete withdrawal of parent substances. GHRPs and their most prominent metabolites were included into routine ultra-pressure liquid chromatography-tandem mass spectrometry procedure. The method was fully validated, calibration curves of targeted analytes were obtained and excretion curves of GHRPs and their metabolites were plotted. Our results confirm that the detection window after GHRPs administration depends on individual metabolism, drug preparation form and the way of administration.

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Comparison of various in vitro model systems of the metabolism of synthetic doping peptides: Proteolytic enzymes, human blood serum, liver and kidney microsomes and liver S9 fraction

Zvereva¹,

Semenistaya²,

Krotov³

et al. 2016

Journal of Proteomics

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Solid‐phase extraction of small biologically active peptides on cartridges and microelution 96‐well plates from human urine

Semenistaya¹,

Zvereva²,

Krotov³

et al. 2015

Drug Testing and Analysis

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Currently liquid chromatography - mass spectrometry (LC-MS) analysis after solid-phase extraction (SPE) on weak cation-exchange cartridges is a method of choice for anti-doping analysis of small bioactive peptides such as growth hormone releasing peptides (GHRPs), desmoporessin, LHRH, and TB-500 short fragment. Dilution of urine samples with phosphate buffer for pH adjustment and SPE on weak cation exchange microelution plates was tested as a means to increase throughput of this analysis. Dilution using 200 mM phosphate buffer provides good buffering capacity without affecting the peptides recoveries. SPE on microelution plates was performed on Waters Positive Pressure-96 Processor with subsequent evaporation of eluates in nitrogen flow. Though the use of smaller sample volume decreases the pre-concentration factor and increases the limits of detection of 5 out of 17 detected peptides, the recovery, linearity, and reproducibility of the microelution extraction were comparable with cartridge SPE. The effectiveness of protocols was confirmed by analysis of urine samples containing ipamorelin, and GHRP-6 and its metabolites. SPE after urine sample dilution with buffer can be used for faster sample preparation. The use of microelution plates decreases consumption of solvents and allows processing of up to 96 samples simultaneously. Cartridge SPE with manual рН adjustment remains the best option for confirmation. Copyright © 2015 John Wiley & Sons, Ltd.

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Determination of biologically active phenols and polyphenols in various objects by chromatographic techniques

Kochetova¹,

Semenistaya²,

Ларионов³

et al. 2007

Russ. Chem. Rev.

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Living polymerization of 4-methyl-2-pentyne and 1-trimethylsilyl-1-propyne initiated by NbCl5-Ph4Sn catalyst

et al. 2008

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Determination of Biologically Active Phenols and Polyphenols in Various Objects by Chromatographic Techniques

et al. 2007

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Determination of exemestane and 17-hydroxyexemestane by high-performance liquid chromatography coupled with tandem mass spectrometry and high-resolution mass spectrometry

et al. 2010

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Characterization of the composition and antioxidant activity of plant extracts by HPLC with UV and amperometric detection

Semenistaya

Ларионов

2008

Pharm Chem J

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High-performance liquid chromatography with UV and amperometric detection has been used to analyze qualitatively and quantitatively phenolic extracts of several plants used in the production of drugs, food, and cosmetics. Phenolic compounds in aqueous alcohol, alcohol, and propyleneglycol (PPG) extracts were identified as groups using a previously constructed database of the spectra and retention times of 74 phenolic compounds. The antioxidant activity (AA) of the extracts was measured as the sum of peaks on the chromatograms after the amperometric detector. The AA of the alcohol extracts correlated with the flavonoid content. Extracts obtained using supercritical PPG had the maximum AA. 539 0091-150X/08/4209-0539

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E. N. Semenistaya

Determination of growth hormone releasing peptides metabolites in human urine after nasal administration of GHRP‐1, GHRP‐2, GHRP‐6, Hexarelin, and Ipamorelin

Comparison of various in vitro model systems of the metabolism of synthetic doping peptides: Proteolytic enzymes, human blood serum, liver and kidney microsomes and liver S9 fraction

Solid‐phase extraction of small biologically active peptides on cartridges and microelution 96‐well plates from human urine

Determination of biologically active phenols and polyphenols in various objects by chromatographic techniques

Living polymerization of 4-methyl-2-pentyne and 1-trimethylsilyl-1-propyne initiated by NbCl5-Ph4Sn catalyst

Determination of Biologically Active Phenols and Polyphenols in Various Objects by Chromatographic Techniques

Determination of exemestane and 17-hydroxyexemestane by high-performance liquid chromatography coupled with tandem mass spectrometry and high-resolution mass spectrometry

Characterization of the composition and antioxidant activity of plant extracts by HPLC with UV and amperometric detection

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