Semen quality, lipid peroxidation, and seminal plasma antioxidant status in horses with different intensities of physical exercise

Härtlová, Helena; Rajmon, Radko; Krontorádová, Iva; Mamica, Jiří; Zita, Lukáš; Klabanová, P.; Černocký, Antonín

doi:10.2754/avb201382010031

Cited by 6 publications

(3 citation statements)

References 18 publications

(11 reference statements)

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“…These effects decrease fertilization capability up to 50% of spermatozoa during cryopreservation (Celeghini et al 2008) and reduce subsequent spermatozoa viability and the ability to fertilize an oocyte (Defoin et al 2008). The success of spermatozoa cryopreservation depends on many factors, including individuality (Härtlová et al 2013), the interaction between cryoprotectants and the extender type (Špaleková et al 2014;Stádník et al 2015), the length of cooling and equilibration period (Andrabi 2007), and the speed of freezing or thawing (Clulow et al 2008).…”

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confidence: 99%

The effect of the freezing curve type on bull spermatozoa motility after thawing

et al. 2015

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The objective of this work was to determine the effect of selected freezing curves on spermatozoa survivability after thawing, defined by its motility. The ejaculates of nine selected sires of the same age, breed, and frequency of collecting, bred under the same breeding conditions including handling, stabling, feeding system and feeding ratio composition, were repeatedly collected and evaluated. Sperm samples of each sire were diluted using only one extender and divided into four parts. Selected four freezing curves -the standard, commercially recommended threephase curve; a two-phase curve; a slow three-phase curve; and a fast three-phase curve, differing in the course of temperature vs time, were applied. The percentage rate of progressive motile spermatozoa above head was determined immediately after thawing, and after 30, 60, 90, and 120 min of the thermodynamic test (TDT). Moreover, average spermatozoa motility (AMOT) and spermatozoa motility decrease (MODE) throughout the entire TDT were evaluated. Insemination doses frozen using the simpler two-phase curve demonstrated the highest motility values (+2.97% to +10.37%; P < 0.05-0.01) immediately after thawing and during the entire TDT. Concurrently, the highest AMOT (+4.37% to +8.82%; P < 0.01) was determined. The highest spermatozoa motility values were detected after thawing doses frozen by the two-phase freezing curve in eight out of nine sires. Simultaneously, a significant effect of sire individuality was clearly confirmed. Inter-sire differences of spermatozoa motility during TDT as well as AMOT and MODE were significant (P < 0.01). The findings describing both factors of interaction indicate the necessity of individual cryopreservation of the ejaculate to increase its fertilization capability after thawing.

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confidence: 99%

The effect of the freezing curve type on bull spermatozoa motility after thawing

et al. 2015

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“…El plasma seminal equino posee actividades considerables de superóxido dismutasa (SOD) y de glutatión-peroxidasa (GPx) (4,5). Igualmente, la catalasa (CAT) se encuentra en grandes cantidades en el semen de los equinos, a excepción de la primera fracción del eyaculado, conocida como fluido preespermático, el cual se origina como secreción de las glándulas bulbouretrales (6).…”

Section: Introductionunclassified

Efecto del isoespintanol y el timol en la actividad antioxidante de semen equino diluido con fines de congelación

Betancur¹,

Rojano²

2017

Rev. Med. Vet.

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Una amplia variedad de antioxidantes evaluados en la congelación de semen equino no ha arrojado resultados satisfactorios en el mantenimiento de su calidad y fertilidad. El isoespintanol y el timol son moléculas de origen natural con una alta actividad antioxidante, lo que las hace potencialmente útiles para reducir el estrés oxidativo del semen durante la criopreservación. Este estudio tuvo como objetivo evaluar el efecto del isoespintanol y el timol en la actividad antioxidante total y enzimática de semen equino diluido con fines de congelación. El semen de cinco caballos criollos colombianos se diluyó en un medio de congelación, se dividió en tres alícuotas que se asignaron aleatoriamente a los tratamientos isoespintanol (40 μM), timol (50 μM) o control (sin antioxidante). Se evaluó la capacidad antioxidante total (TAC) por los ensayos ORAC y FRAP. La actividad de catalasa (CAT), superóxido dismutasa (SOD) y glutatión peroxidasa (GPx) se evaluaron mediante pruebas enzimáticas. La evaluación estadística se realizó mediante modelos mixtos, análisis de correlación y comparación de medias por la prueba de Tukey. Las actividades de SOD y GPx fueron menores para el isoespintanol (6,7 ± 2,2 U/ ml y 0,16 ± 0,02 U/ml), comparadas con el timol (6,9 ± 2,2 U/ml y 0,20 ± 0,02 U/ml) y el control (7,2 ± 2,2 U/ml y 0,22 ± 0,02 U/ml) (p < 0,05). No hubo diferencias para la TAC o la CAT del semen (p > 0,05). El isoespintanol reduce la actividad de SOD y GPx en el semen equino diluido con fines de congelación.

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“…breed, variation between individuals, age of sire (Thara and Nair 2007;Beran et al 2012;Härtlová et al 2013), environmental conditions (Balić et al 2012), and frequency of collecting the ejaculate (Karoui et al 2011). Collection of the ejaculate and its subsequent processing present further potential risk factors for declined sperm quality.…”

Section: Reproduction Bull Sperm Extender Ldl Cholesterol Sperm Smentioning

confidence: 99%

Influence of selected factors on bovine spermatozoa cold shock resistance

et al. 2015

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The objectives of this study were to determine the effects of sire, extender, and addition of Low Density Lipoprotein (LDL) to extenders used on the percentage rate of spermatozoa survival after cold shock. Two groups of extenders were compared: without LDL addition (control variants) and LDL enriched (experimental variants). Three extenders were used: AndroMed ® extenders, and 6-10% LDL addition into the Triladyl ® extender. In total, 12 samples of fresh semen were collected from 4 bulls during a period of 8 weeks. Bovine spermatozoa cold shock resistance (1 ± 1 °C, 10 min) was evaluated by the percentage rate of live sperm using eosin-nigrosine staining immediately and after heat incubation (37 ± 1 °C, 120 min). The results showed the effect of sire as important and individual differences between selected sires in their sperm resistance against cold shock were confirmed. AndroMed ® and Bioxcell ® were found to be providing better protection of bull semen to cold shock compared to Triladyl ® due to lower decline of live sperm proportion. Our results detected a positive effect of LDL addition on sperm resistance against cold shock, especially on lower decrease of live sperm percentage rate after 120 min of the heat test (P < 0.05). Further studies are needed to assess the optimal concentration of LDL in various kinds of extenders as well to state ideal time and temperature conditions for ensuring LDL reaction with sperm. , bull sperm, extender, LDL cholesterol, sperm survival, cold shock, eosin-nigrosine staining Reproduction

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Semen quality, lipid peroxidation, and seminal plasma antioxidant status in horses with different intensities of physical exercise

Cited by 6 publications

References 18 publications

The effect of the freezing curve type on bull spermatozoa motility after thawing

The effect of the freezing curve type on bull spermatozoa motility after thawing

Efecto del isoespintanol y el timol en la actividad antioxidante de semen equino diluido con fines de congelación

Influence of selected factors on bovine spermatozoa cold shock resistance

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