Use of galactose to vitrify ram semen in straws

Matias, Márcio Calixto; Cézar, Allan Rodolf Ribeiro; Marques, Juliana Carla Cavalcanti; Silva, Fernanda Karla Ataide da; Sandes, Vitória Nayreli Freire Gonçalves; Câmara, Diogo Ribeiro

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Veterinary Medicine • Ciênc. anim. bras. 22 • 2021 • https://doi.org/10.1590/1809-6891v22e-67525 copy

Use of galactose to vitrify ram semen in straws

Authorship SCIMAGO INSTITUTIONS RANKINGS

Abstract

Sperm vitrification is a technique with great potential for cryopreservation of genetic material, with superior effectiveness compared to conventional methods in some species. However, few studies have shown its efficiency with ejaculated sperm of rams and the use of galactose as an extracellular cryoprotectant during vitrification. This study aimed to evaluate the effect of galactose (0.01 M), with or without glycerol addition (3% and 7%) in a commercial extender (Steridyl^® - control) for ram sperm cryopreservation in straws, comparing the classic freezing method and vitrification. Ejaculates from six breeding soundness Dorper rams were collected with an artificial vagina, aliquoted, individually diluted (100 × 10⁶ sperm/mL) on extenders tested, loaded into 0.25 mL straws, and subjected to a classic freezing method or vitrification. Sperm kinematics, morphology, morphometry, viability, and physical and functional integrity of the sperm membrane were evaluated. The classic freezing method resulted in higher total and progressive motility than vitrification, as no motility was detected in vitrified samples after rewarming (p<0.05). The addition of galactose or glycerol to the commercial medium did not benefit both vitrification and the classic freezing method.

Keywords:
Semen biotechnology; Ultra-rapid freezing; Cryoprotectants; Reproduction

Sperm parameters	Extenders
	1		2		3		4
	Classic	Vitrification	Classic	Vitrification	Classic	Vitrification	Classical method	Vitrification
TM (%)	22.7±4.5^a	0*	19.1±5.4^a	0*	20.8±7.7^a	0*	2.2±0.9^b	0*
PM (%)	13.4±4.3^ab	0*	14.8±3.9^ab	0*	18.1±5.5^a	0*	1.7±1.7^b	0
Viability (%)	20.6±2.0^a	0*	17.3±2.4^a	0*	8.7±1.9^b	0*	1.9±0.6^b	0.2±0.2*
PMI (%)	34.5±4.7^a	0*	27.2±4.0^a	0.2±0.2*	20.9±3.3^a	0*	3.7±1.6^b	0*
Hypoosmotic (%)	38.5±4.4	3.2±1.3*	35.9±3.9	8.8±1.7*	32.6±3.1	7.4±2.6*	41.4±5.4	8.6±2.0*
Area (µm²)	316.0±8.2	298.6±10.6	315.0±4.2	307.2±8.2	307.5±8.1	297.8±7.5	319.1±1.7	293.3±11.3*
Perimeter (µm)	76.3±1.8	79.6±1.6	76.4±1.2	80.3±1.0*	75.8±1.5	78.1±0.9	76.5±1.2	79.4±2.0
Length (µm)	27.2±0.4	27.2±0.4	27.3±0.2	27.5±0.3	27.0±0.3	27.1±0.2	27.4±0.1	27.1±0.4
Width (µm)	15.3±0.2	14.8±0.2	15.3±0.2	15.1±0.2	15.1±0.3	14.8±0.1	15.4±0.1	14.8±0.3*

Sperm parameters	Extenders
	1		2		3		4
	Classic	Vitrification	Classic	Vitrification	Classic	Vitrification	Classic	Vitrification
Minor defects (%)	9.0±4.4	2.7±1.8	6.2±2.6	4.8±2.5	4.2±2.1	3.9±2.1	9.7±7.1	5.9±3.8
Major defects (%)	8.8±2.5	18.0±4.4	7.8±1.5	20.8±3.2*	12.0±3.6	21.9±2.6*	9.5±2.1	19.5±3.4*
Total defects (%)	17.8±5.9	20.8±4.4	14.1±3.3	25.7±3.3	16.2±5.1	25.8±2.0	19.2±7.3	25.4±2.8
Proximal droplet (%)	1.5±0.3	0.1±0.1*	1.1±0.2	0	1.8±0.9	0	1.7±0.6	0*
Tail coiled around the head (%)	0	0.1±0.1*	0	0	0.2±0.2	0	0	0
Strong coiled or bent tail (%)	5.9±2.4	17.1±4.4*	5.9±1.4	20.8±3.3*	8.0±3.1	21.7±2.6*	6.9±2.3	19.2±3.6*
Bent tail with distal droplet (%)	0.2±0.2	0	0.2±0.2	0	0.5±0.1	0*	0.2±0.2	0
Coiled or bent tail (%)	3.2±1.7	0.4±0.2	2.5±0.6	0.2±0.2*	0.9±0.4	0.6±0.3	2.2±1.0	0.8±0.4

Universidade Federal de Goiás Universidade Federal de Goiás, Escola de Veterinária e Zootecnia, Campus II, Caixa Postal 131, CEP: 74001-970, Tel.: (55 62) 3521-1568, Fax: (55 62) 3521-1566 - Goiânia - GO - Brazil
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[1] *Correspondent: diogo@vicosa.ufal.br