Morphological evaluation of adult domestic cat testicular biopsy after vitrification

Julyne Vivian Guimarães de Carvalho; Airton Renan Bastos Soares; Inara Tayná Alves Evangelista; Danuza Leite Leão; Regiane Rodrigues Dos Santos; Sheyla Farhayldes Souza Domingues

doi:10.1017/S096719942400008X

Morphological evaluation of adult domestic cat testicular biopsy after vitrification

Zygote. 2024 May 13:1-8. doi: 10.1017/S096719942400008X. Online ahead of print.

Authors

Julyne Vivian Guimarães de Carvalho^{1

2}, Airton Renan Bastos Soares¹, Inara Tayná Alves Evangelista¹, Danuza Leite Leão¹, Regiane Rodrigues Dos Santos¹, Sheyla Farhayldes Souza Domingues^{1

2}

Affiliations

¹ Laboratory of Wild Animal Biotechnology and Medicine, Faculty of Veterinary Medicine, Federal University of Pará, Castanhal, Pará, Brazil.
² Postgraduate Programme in Animal Health and Production in the Amazon, Federal Rural University of Amazonia, Belém, Pará, Brazil.

PMID: 38738346
DOI: 10.1017/S096719942400008X

Abstract

Testicular biopsies (9 mm³) from domestic cats (n = 10) submitted to orchiectomy were submitted to equilibrium vitrification in the presence of ethylene glycol (EG) alone or combined with dimethylsulfoxide (DMSO) as intracellular cryoprotectants, and sucrose or trehalose as extracellular cryoprotectants. The samples were vitrified with 40% EG or 20% EG + 20% DMSO, plus 0.1 M or 0.5 M of sucrose or trehalose. The study was divided into Step 1 and Step 2. In Step 1, intratubular cells (spermatogonia, spermatids, spermatocytes, and Sertoli cells) were quantified and classified as intact or degenerated (pyknotic and/or vacuolated cells). Cryodamage of seminiferous cords was determined by spermatogonia and Sertoli cell scoring of nuclei alterations, tubular basement membrane detachment, epithelium shrinkage, and tubular measures (total area, epithelium area, larger and smaller diameter, and height of the epithelium). In Step 2, Hoechst 33342 stain and propidium iodide (PI) fluorescent stain were used to assess the cell viability of the four best experimental groups in Step 1. The effect of treatments on all analyses was accessed using analysis of variance (ANOVA), and Fisher's post hoc test at P < 0.05 significance was considered. In Step 1, the mean percentage of spermatogonia and Sertoli cells morphological integrity did not show a difference when using both sugars at different concentrations, but their morphology was more affected when DMSO was used. EG use associated with 0.1 M of sucrose or trehalose positively affected spermatocyte and spermatid morphology, respectively. The larger diameter and epithelium height of seminiferous tubules were increased using DMSO plus 0.5 M sucrose and DMSO plus 0.1 M trehalose. The changes in spermatogonial/Sertoli nucleoli visualization were best scored in the EG groups, while the nuclei condensation was lower with sucrose. The basement membrane was satisfactorily preserved with 0.1 M sucrose. In Step 2, the percentage of cell viability was higher when EG plus 0.1 M sucrose was used. Therefore, DMSO's negative effect on the vitrification of testicular biopsies of adult domestic cats was evident. The EG plus 0.1 M of sucrose or trehalose associations are the most suitable CPAs to preserve the testicular histology structure of adult domestic cats in vitrification.

Keywords: Cryopreservation; Cryoprotectants; Domestic cat; Testicular tissue; Vitrification.