Effect of α‐tocopherol in the vitrification medium on the viability, lipid peroxidation, expression of key developmental, apoptotic and stress‐related genes in ovine secondary follicles

Author:

Kaushik Kalpana12ORCID,Krishna Kavya1,Johnson P.1,Gupta P. S. P.1ORCID,Nandi S.1,Mondal S.1ORCID,Suganthi R. U.1,Nikhil Kumar Tej J.1

Affiliation:

1. ICAR‐National Institute of Animal Nutrition and Physiology Bengaluru India

2. Department of Biotechnology Jain University Bengaluru India

Abstract

AbstractThe present study aimed to evaluate the effect of α‐tocopherol on viability, lipid peroxidation and the expression of apoptosis, stress and development‐related genes in the vitrified sheep secondary follicles. Ovarian secondary follicles (200–300 μm) were isolated and distributed separately to the vitrification treatment and supplemented with 5 mM, 10 mM, 20 mM and 30 mM of α‐tocopherol (while the control fresh group was without vitrification and supplementation of α‐tocopherol). After a week, the follicles were thawed and evaluated for follicular viability by trypan blue dye exclusion method, lipid peroxidation and gene expression studies. The results showed that the vitrification with 10 and 20 mM of α‐tocopherol positively affected (p < .05) the viability of vitrified follicles in comparison with vitrified ones without α‐tocopherol but the higher concentration of α‐tocopherol, i.e., 30 mM negatively affected the viability (p < .05) in comparison with the 10 and 20 mM of α‐tocopherol groups. The malondialdehyde (MDA) levels were significantly (p < .05) higher in the vitrified without α‐tocopherol group in comparison to the vitrified with 20 mM of α‐tocopherol group. The expression of apoptotic‐related gene, BCL2L1 was significantly higher in 10 mM α‐tocopherol group compared to the control fresh and CASPASE 3, 9 expressions were significantly higher in the vitrified group when compared to the vitrified with 10 mM α‐tocopherol group. Expressions of BAX, BAD, BAK, BMP‐15 and GDF‐9 showed no significant difference among the groups. The mRNA expression of SOD1 was significantly higher in the vitrified without α‐tocopherol group when compared to other groups. We conclude that the supplementation of 10 and 20 mM α‐tocopherol in vitrification solution was the efficient vitrification procedure for the vitrification of ovine secondary follicles.

Funder

Department of Biotechnology, Government of West Bengal

Publisher

Wiley

Subject

Endocrinology,Animal Science and Zoology,Biotechnology

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