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Título : L-carnitine supplementation in conventional slow and ultra-rapid freezing media improves motility, membrane integrity, and fertilizing ability of dog epididymal sperm
Autor: Ramon Lopez, Angel Eduardo
Fernandez Collahuazo, Jessica Paola
Samaniego Campoverde, Jorge Xavier
Duma Pauta, Jose Mauricio
Mendez Alvarez, Maria Silvana
Soria Parra, Manuel Elias
Galarza Alvarez, Luis Rodrigo
Galarza Lucero, Diego Andres
Correspondencia: Galarza Lucero, Diego Andres, andres.galarza@ucuenca.edu.ec
Palabras clave : Dog sperm
Epididymis
L-carnitine
Conventional freezing
Ultra-rapid freezing
Área de conocimiento FRASCATI amplio: 4. Ciencias Agrícolas
Área de conocimiento FRASCATI detallado: 4.3.1 Ciencias veterinarias
Área de conocimiento FRASCATI específico: 4.3 Medicina Veterinaria
Área de conocimiento UNESCO amplio: 08 - Agricultura, Silvicultura, Pesca y Veterinaria
ÁArea de conocimiento UNESCO detallado: 0841 - Veterinaria
Área de conocimiento UNESCO específico: 084 - Veterinaria
Fecha de publicación : 2024
Fecha de fin de embargo: 31-dic-2050
Volumen: Volumen 270
Fuente: Animal Reproduction Science
metadata.dc.identifier.doi: 10.1016/j.anireprosci.2024.107580
Tipo: ARTÍCULO
Abstract: 
This study aimed to assess the impact of L-carnitine (LC) supplementation in conventional-slow (CS) and ultra-rapid (UR) freezing media on post-thaw quality and fertilizing ability of dog epididymal spermatozoa. Sperm samples were collected from 60 epididymides obtained from 30 adult orchiectomized dogs via retrograde flushing. Twenty pooled sperm samples were then created (3 epididymal samples/pool). Four treatments were established according to the freezing method (CS and UR) and LC supplementation (5 and 0 mM [control, Co]): CS-LC5, CS-Co, URLC5, and UR-Co. The CS freezing involved exposing 0.25 mL straw to liquid nitrogen vapors (LN2), while UR freezing submerged 30-μL drops of sperm samples directly into LN2. Sperm kinematics, membrane integrity, and fertilizing ability (by heterologous in vitro fertilization using bovine oocytes) were evaluated for all treatments. Post-thaw results revealed that the CS freezing treatments resulted in significantly higher values (P < 0.05) of curvilinear and average-path velocities, and beat-cross frequency compared to the UR freezing treatments, regardless of LC supplementation. The CS-LC5 and UR-LC5 treatments cryoprotected the sperm by increasing (P < 0.05) the percentage of ‘live-sperm/intact-acrosome’ compared to their controls treatments CS-Co and UR-Co. Regarding fertilizing ability, the CS-LC5 treatment yielded a higher percentage (P < 0.05) of pronuclei formation compared to both UR treatments. The UR-LC5 treatment, however, obtained greater percentage (P < 0.05) than their control UR-Co. In conclusion, supplementation with L-carnitine in conventional-slow and ultra-rapid freezing improved sperm motility, plasma, and acrosome membranes integrity and fertilizing ability of dog epididymal spermatozoa
URI : https://doi.org/10.1016/j.anireprosci.2024.107580
URI Fuente: https://www.journals.elsevier.com/animal-reproduction-science
ISSN : 0378-4320
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