Melatonin and Caffeine Supplementation Used, Respectively, as Protective and Stimulating Agents in the Cryopreservation of Human Sperm Improves Survival, Viability, and Motility after Thawing compared to Traditional TEST-Yolk Buffer

Author:

Pariz Juliana R.1234,Ranéa Caroline12,Monteiro Rosa A. C.1,Evenson Donald P.5,Drevet Joël R.6ORCID,Hallak Jorge1234ORCID

Affiliation:

1. Androscience, Science and Innovation Center in Andrology and High-Complex Clinical and Andrology Laboratory, São Paulo 04534011, Brazil

2. Division of Urology, Department of Surgery, Hospital das Clinicas, University of Sao Paulo Medical School, São Paulo 05403-000, Brazil

3. Department of Pathology, Reproductive Toxicology Unit, University of São Paulo Medical School, São Paulo 01246-903, Brazil

4. Institute for Advanced Studies, University of Sao Paulo, São Paulo 05508-060, Brazil

5. SCSA Diagnostics, Brookings 57006, USA

6. Université Clermont Auvergne, GReD Laboratory, Faculty of Medicine, Clermont-Ferrand 63001, France

Abstract

Cryopreservation processes can damage spermatozoa and impair structural and functional cell characteristics. Plasma, nuclear membranes, and cellular organelles can suffer from the freeze and thaw process. This study evaluates the protective and stimulant effect of melatonin and caffeine supplementation on the functional characteristics of human spermatozoa before and after freezing. Thirty seminal samples from normozoospermic men aged 19–45 years old collected between October 2012 and May 2017 were included. Semen samples were supplemented with either 2 mM melatonin (MEL) prior to cryopreservation, 2 mM caffeine (CAF) in postthaw, or CAF and MEL (CM) in precryopreservation and postthaw, respectively. Kinetics and seminal parameters, mitochondrial activity, DNA fragmentation, and reactive oxygen species (ROS) levels were analyzed before and after cryopreservation. A significant reduction in sperm concentration, total and progressive motility, sperm kinetics, and mitochondrial activity, as well as a significant increase in DNA fragmentation and ROS production in postthaw samples compared to fresh samples, was identified. After administration of a caffeine and/or melatonin supplement, there was a significant increase in progressive motility in the CAF (p=0.005) and CM (p=0.048) groups, as well as mitochondrial activity in the CM group (p<0.05). Cryopreservation has negative effects on overall sperm quality and increases ROS production. A combination of caffeine and melatonin in prefreeze and postthaw sperm samples has proven to be a very effective and simple way to improve semen quality. This will be particularly useful for initial low-quality semen samples, those which suffer the most from the freezing/thawing process.

Funder

Androscience, Science and Innovation Center in Andrology and High-Complex Clinical and Andrology Laboratory

Publisher

Hindawi Limited

Subject

Cell Biology,Ageing,General Medicine,Biochemistry

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