Identification of recombinant human EPO variants in greyhound plasma and urine by ELISA, LC‐MS/MS and western blotting: a comparative study

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CJC‐1295 is a peptide‐based drug that stimulates the production of growth hormone (GH) from the pituitary gland. It incorporates a functional maleimido group at the C‐terminus that allows it to covalently bind plasma proteins such as serum albumin. These CJC‐1295‐protein conjugates have a much greater half‐life compared to the unconjugated peptide and are capable of stimulating GH production for more than six days in humans after a single administration. Conjugated CJC‐1295 is difficult to detect in blood by mass spectrometry due to its low abundance, high molecular weight, and conjugation to a range of different protein substrates. Previously we described a screening procedure for the detection of CJC‐1295 in equine plasma using an immuno‐PCR assay. Here we demonstrate the confirmation of CJC‐1295 in equine plasma by LC−MS/MS after immuno‐affinity capture and tryptic digestion. Using this method, CJC‐1295 was identified down to concentrations as low as 180 pg/mL in 1 mL of equine plasma.

Section: Discussionmentioning

confidence: 99%

Section: Plasma Samplesmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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A method for confirming CJC‐1295 abuse in equine plasma samples by LC–MS/MS

Timms

Ganio

Steel

2019

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“…SDS polyacrylamide gel electrophoresis (SDS‐PAGE) and western blotting were performed as described in Timms et al RD4 and RD6 monoclonal antibodies were diluted 1 in 1000 for use. Donkey F (ab’) polyclonal secondary antibody to mouse IgG (HRP conjugated) was used at 1 in 20 000.…”

Section: Experimental Methodsmentioning

confidence: 99%

An immuno polymerase chain reaction screen for the detection of CJC‐1295 and other growth‐hormone‐releasing hormone analogs in equine plasma

Timms

Ganio

Forbes

et al. 2018

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CJC‐1295 is a 30 amino acid peptide‐based drug that stimulates the release of growth hormone (GH) from the pituitary gland. It is unique among performance‐enhancing peptides due to the presence of a reactive maleimidopropionic acid group that covalently links the peptide to free thiols on the surface of plasma proteins. Once conjugated, CJC‐1295 remains active in the bloodstream for significantly longer than non‐conjugated peptide‐based drugs that are rapidly excreted. Conjugation of CJC‐1295 to plasma proteins prevents its detection by top‐down mass‐spectrometry‐based peptide screening protocols as it effectively becomes a macromolecular protein with an undefined molecular weight. Using a pair of monoclonal antibodies raised against the CJC‐1295 peptide, we present an immuno‐polymerase chain reaction (I‐PCR) assay that is capable of detecting the CJC‐1295‐protein conjugate at concentrations down to 0.8 pg/mL. Detection of endogenous equine GHRH necessitated a screening threshold for CJC‐1295 in equine plasma of 50 pg/mL. The effectiveness of the assay for controlling the illicit use of CJC‐1295 was confirmed in equine blood samples after administration in thoroughbred race horses.

“…The detection of rHuEPO usually involves immunoaffinity capture and electrophoretic‐based detection in human and animal subjects or immunoaffinity capture and mass spectrometry (MS) in nonhuman species through the detection of rHuEPO‐specific peptides . Because these peptides are used to discriminate any suspicious sample from real administration cases, analytical methods crucially need both high sensitivity and extensive specificity.…”

Section: Introductionmentioning

confidence: 99%

Screening and confirmatory analysis of recombinant human erythropoietin for racing camels' doping control

Delcourt¹,

Garcia²,

Chabot³

et al. 2020

Recombinant human erythropoietin (rHuEPO) belongs to the therapeutic class of erythropoiesis stimulating agents (ESAs) due to its implication in the creation pathway of red blood cells and thus enhancement of oxygenation. Because of this bioactivity, rHuEPO has been considered as a major doping agent in sports competitions for decades. Over the years, doping control laboratories designed several analytical strategies applied to human and animal samples to highlight any misuse. Even though multiple analytical approaches have been reported, none has yet been dedicated to racing camels. Here, we describe an analytical strategy to test camel plasma samples at screening using an ELISA assay and a targeted nano‐liquid chromatography–high‐resolution tandem mass spectrometry for confirmatory analysis. The method was validated and has been successfully applied to post‐race samples, allowing the detection of a positive case of rHuEPO administration.