Detecting EPO in Microvolumetric Capillary Serum Shipped at Ambient Temperature for Antidoping Testing.

Drug Test Anal

Sports Medicine Research and Testing Laboratory, Salt Lake City, Utah, USA.

Published: November 2024

AI Article Synopsis

  • Erythropoietin receptor agonist (ERA) testing for antidoping can be performed using both blood and urine samples, with recent studies indicating that microvolumetric capillary serum samples collected using the Tasso+ device are just as effective as traditional methods.
  • Blood samples, which are more stable than urine samples, can be sent to laboratories for ERA analysis without the need for cold shipping conditions, allowing for easier collection in the field.
  • A study conducted with the Ultimate Fighting Championship confirmed the reliability of ERA testing in blood samples shipped at ambient temperatures, with 100% detectability of endogenous EPO, thereby suggesting a more cost-effective approach to antidoping practices.

Article Abstract

Erythropoietin receptor agonist (ERA) testing for antidoping can be achieved in both urine and blood samples. Recent published work showed the comparability between the two matrices and focused on detectability in microvolumetric capillary serum samples collected using the Tasso+ device. Currently, in the antidoping field, blood samples are required to be shipped under cold, temperature-controlled conditions. However, due to the suggested greater stability of EPO in blood compared to urine, it is believed that blood samples should be viable for ERA analysis if shipped under the ambient, not cold temperature-controlled conditions to which urine samples are subjected. In this collaborative study with the Ultimate Fighting Championship, microvolumetric capillary serum samples were collected in the field and shipped under ambient conditions to the laboratory for ERA analysis. Resulting data showed that endogenous EPO was detectable in 100% of these samples, showing no loss in detectability despite shipping under non-controlled conditions. Further, ERA analyses were conducted in the laboratory on additional in-house collected samples and post-EPO administration samples subjected to various storage and shipping conditions, also showing reliable endogenous and recombinant EPO detectability in all samples except those experiencing extreme temperature (50°C) conditions. Taken together, these data highlight the stability of EPO in blood samples and show that ERA blood samples can be collected in the field and shipped without costly temperature-controlled shipping methods and without a loss in detectability.

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Source
http://dx.doi.org/10.1002/dta.3831DOI Listing

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