Influence of Cryopreservation Solution on the In Vitro Culture of Skin Tissues Derived from Collared Peccary (Pecari tajacu Linnaeus, 1758)

Alana A Borges; Gabriela P O Lira; Lucas E Nascimento; Luiza B Queiroz Neta; Maria V O Santos; Moacir F Oliveira; Alexandre R Silva; Alexsandra F Pereira

doi:10.1089/bio.2017.0090

Influence of Cryopreservation Solution on the In Vitro Culture of Skin Tissues Derived from Collared Peccary (Pecari tajacu Linnaeus, 1758)

Biopreserv Biobank. 2018 Apr;16(2):77-81. doi: 10.1089/bio.2017.0090. Epub 2017 Dec 7.

Authors

Alana A Borges¹, Gabriela P O Lira¹, Lucas E Nascimento¹, Luiza B Queiroz Neta¹, Maria V O Santos¹, Moacir F Oliveira², Alexandre R Silva³, Alexsandra F Pereira¹

Affiliations

¹ 1 Laboratory of Animal Biotechnology, Federal Rural University of Semi-Arid , Mossoró, Brazil .
² 2 Laboratory of Applied Animal Morphophysiology, Federal Rural University of Semi-Arid , Mossoró, Brazil .
³ 3 Laboratory of Animal Germplasm Conservation, Federal Rural University of Semi-Arid , Mossoró, Brazil .

Abstract

Skin vitrification is a promising and alternative tool for the conservation of biodiversity, especially for wild mammals, such as collared peccaries. Several factors can affect the success of this procedure, such as the cryoprotectant solution used. Therefore, this study was carried out to compare the efficiency of various vitrification solutions for recovery of viable cells after in vitro culture of cryopreserved skin tissues derived from the collared peccary, aiming to study the application in biobanking, where cellular use is not immediately required. Then, Dulbecco's modified Eagle's medium (DMEM) composed of 2.2 g/L sodium bicarbonate and 10% fetal bovine serum (FBS) was supplemented with 3.0 M ethylene glycol (EG) or 3.0 M dimethyl sulfoxide (DMSO) or 1.5 M EG plus 1.5 M DMSO with or without sucrose (SUC; 0.25 M) to produce six solutions for solid-surface vitrification. After warming, skin tissues were cultured in vitro and recovered cells were analyzed for morphology, adhesion, subconfluence, and proliferative activity for developing the growth curve and determining the population doubling time (PDT), and viability by Trypan Blue. The vitrification did not alter the ability of the tissues to adhere to the culture dish, as well as the day of all explants with cell growth, subconfluence samples, subconfluence total time, and PDT (p > 0.05). Moreover, independent of the cryoprotectant solution used, the vitrification altered the day of all attached explants (p < 0.05). Nevertheless, for viability after the first passage, only the EG-SUC (86.9%) and DMSO-SUC (91.4%) groups maintained viable cell recovery similar to the nonvitrified group (96.3%, p > 0.05). Additionally, for viability after the third passage, only the EG-SUC group maintained the cell quality (88.3%), when compared with the nonvitrified (97.8%, p > 0.05). In conclusion, DMEM with 10% FBS, 3.0 M EG, and 0.25 M sucrose was the most efficient solution for vitrifying collared peccary skin tissues, leading to the in vitro culture of viable cells.

Keywords: cryobanking; cryoprotectants; somatic tissues; wild mammals.

MeSH terms

Animals
Artiodactyla
Cryopreservation / methods*
Cryoprotective Agents* / chemistry
Cryoprotective Agents* / pharmacology
Skin* / cytology
Skin* / metabolism
Tissue Banks*
Tissue Culture Techniques / methods*

Substances

Cryoprotective Agents