Vitrification of feline ovarian tissue: Comparison of protocols based on equilibration time and temperature

Isa Mohammed Alkali; Martina Colombo; Teresina De Iorio; Aleksandra Piotrowska; Olga Rodak; Michał Jerzy Kulus; Wojciech Niżański; Piotr Dziegiel; Gaia Cecilia Luvoni

doi:10.1016/j.theriogenology.2024.05.023

Vitrification of feline ovarian tissue: Comparison of protocols based on equilibration time and temperature

Theriogenology. 2024 Aug:224:163-173. doi: 10.1016/j.theriogenology.2024.05.023. Epub 2024 May 18.

Authors

Isa Mohammed Alkali¹, Martina Colombo², Teresina De Iorio³, Aleksandra Piotrowska⁴, Olga Rodak⁵, Michał Jerzy Kulus⁶, Wojciech Niżański⁷, Piotr Dziegiel⁸, Gaia Cecilia Luvoni⁹

Affiliations

¹ Dipartimento di Medicina Veterinaria e Scienze Animali, Università degli Studi di Milano, via dell'Università, 6, 26900, Lodi, Italy; Department of Theriogenology, University of Maiduguri, Maiduguri, Nigeria. Electronic address: isa.mohammed@unimi.it.
² Dipartimento di Medicina Veterinaria e Scienze Animali, Università degli Studi di Milano, via dell'Università, 6, 26900, Lodi, Italy. Electronic address: martina.colombo@unimi.it.
³ Dipartimento di Medicina Veterinaria e Scienze Animali, Università degli Studi di Milano, via dell'Università, 6, 26900, Lodi, Italy; Consiglio per la Ricerca in Agricoltura e l'Analisi dell'Economia Agraria (CREA), Research Center "Zootechny and Aquaculture", Via Salaria, 31, 00015, Monterotondo, RM, Italy. Electronic address: teresina.deiorio@unimi.it.
⁴ Department of Histology and Embryology, Wrocław Medical University, ul. Chalubinskiego 6a, 50-368, Wrocław, Poland. Electronic address: aleksandra.piotrowska@umw.edu.pl.
⁵ Department of Histology and Embryology, Wrocław Medical University, ul. Chalubinskiego 6a, 50-368, Wrocław, Poland. Electronic address: olga.rodak@student.umw.edu.pl.
⁶ Division of Ultrastructural Research, Wroclaw Medical University, 50-368, Wrocław, Poland. Electronic address: mkulus@gmail.com.
⁷ Department of Reproduction and Clinic for Farm Animals, Wrocław University of Environmental and Life Sciences, Grunwaldzki Square 49, 50-366, Wrocław, Poland. Electronic address: wojciech.nizanski@upwr.edu.pl.
⁸ Department of Histology and Embryology, Wrocław Medical University, ul. Chalubinskiego 6a, 50-368, Wrocław, Poland. Electronic address: piotr.dziegiel@umw.edu.pl.
⁹ Dipartimento di Medicina Veterinaria e Scienze Animali, Università degli Studi di Milano, via dell'Università, 6, 26900, Lodi, Italy. Electronic address: cecilia.luvoni@unimi.it.

PMID: 38776704
DOI: 10.1016/j.theriogenology.2024.05.023

Abstract

Global contraction of biodiversity pushed most members of Felidae into threatened or endangered list except the domestic cat (Felis catus) thence preferred as the best model for conservation studies. One of the emerging conservation strategies is vitrification of ovarian tissue which is field-friendly but not yet standardized. Thus, our main goal was to establish a suitable vitrification protocol for feline ovarian tissue in field condition. Feline ovarian tissue fragments were punched with biopsy punch (1.5 mm diameter) and divided into 4 groups. Group 1 was fresh control (Fr), while the other three were exposed to 3 vitrification protocols (VIT_CT, VIT_RT1 and VIT_RT2). VIT_CT involved two step equilibrations in solutions containing dimethyl sulfoxide (DMSO) and ethylene glycol (EG) for 10 min each at 4 °C. VIT_RT1 involved three step equilibration in solutions containing DMSO, EG, polyvinylpyrrolidone and sucrose for 14 min in total at room temperature, while in VIT_RT2 all conditions remained the same as in VIT_RT1 except equilibration timing which was reduced by half. After vitrification and warming, fragments were morphologically evaluated and then cultured for six days. Subsequently, follicular morphology, cellular proliferation (expression of Ki-67, MCM-7) and apoptosis (expression of caspase-3) were evaluated, and data obtained were analysed using generalised linear mixed model and chi square tests. Proportions of intact follicles were higher in Fr (P = 0.0001) and VIT_RT2 (P = 0.0383) in comparison to the other protocols both post warming and after the six-day culture. Generally, most follicles remained at primordial state which was confirmed by the low expression of Ki-67, MCM-7 markers. In conclusion, VIT_RT2 protocol, which has lower equilibration time at room temperature has proven superior thus recommended for vitrification of feline ovarian tissue.

Keywords: Conservation of biodiversity; Cryoprotectant; Field conditions; Ovarian fragments; Room temperature; Ultrastructure.

Publication types

Comparative Study

MeSH terms

Animals
Cats
Cryopreservation* / methods
Cryopreservation* / veterinary
Female
Ovary*
Temperature
Vitrification*