Cryopreservation and Culture of Testicular Tissues: An Essential Tool for Biodiversity Preservation

Silva, Alexandre Rodrigues; Pereira, Alexsandra Fernandes; Comizzoli, Pierre

doi:10.1089/bio.2020.0010

Cited by 20 publications

(23 citation statements)

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“…We hypothesize that more cells had time to revive over 24 h of culture and eventually were present in higher proportions than in the refrigerated/fresh tissue shipped overnight to our laboratory. This is a phenomenon that has been already reported in gonadal tissues in many species (from ungulates to carnivores) following vitrification and warming [ 3 , 18 ].…”

Section: Discussionmentioning

confidence: 65%

“…Our next step is to decipher and quantify DNA repair mechanisms in tissues through staining of proliferating cell nuclear antigen (PCNA) or RAD51 protein [ 16 ] and detection of heat shock proteins [ 17 ]. Similarly, testicular cell viability improved after culture like in other species, which is considered a good sign of functional reanimations [ 3 ]. Interestingly, viability after vitrification and culture was even better than in fresh tissues.…”

Section: Discussionmentioning

confidence: 99%

“…Therefore, it is critical to collect or rescue and store genetic materials from all individuals for later use. As seen in other rare and endangered species, long-term preservation of ovarian and testicular tissues from individuals sterilized for medical reasons or dying unexpectedly offers additional options to study and propagate genetically valuable animals over multiple generations [ 3 ]. Cryopreservation of testicular tissues is now conducted in humans, laboratory models, domestic species, and some wildlife [ 3 , 4 , 5 ].…”

Section: Introductionmentioning

confidence: 99%

“…Among the multiple preservation protocols that are available for testicular tissues, vitrification or ultra-rapid freezing is the most convenient approach that has already provided encouraging results for carnivore tissues regarding the maintenance of histomorphometry [ 3 , 6 ]. While cryoprotectants, exposure conditions, tissue biopsy size, or freezing rates play critical roles in tissue survival [ 3 ], warming is an essential step that is often overlooked. Proper warming can prevent devitrification/ice recrystallization and ensure optimal reanimation in preserved tissues.…”

Section: Introductionmentioning

confidence: 99%

“…Interestingly, spermatozoa from frozen-thawed testicular tissues are viable in the cat model (based on the birth of healthy offspring after transfer of embryos produced by sperm injection) [ 9 ]. However, testicular tissues contain a large number of germ cells at early stages (in seminiferous tubules) that have the potential to develop into mature sperm cells after in vitro culture or xenografting as seen in other species, including the domestic ferret [ 3 , 10 ]. Spermatogenesis requires adequate germ cell support that may be compromised during freezing/warming as seen in humans [ 5 ] or in the cat model [ 6 ].…”

Section: Introductionmentioning

confidence: 99%

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Long-Term Preservation of Testicular Tissue Integrity and Viability Using Vitrification in the Endangered Black-Footed Ferret (Mustela nigripes)

Lima

Silva

Marinari

et al. 2020

Animals

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Systematic cryo-banking of semen and testicular tissues is critical to preserve the genetic value of recently deceased or neutered black-footed ferrets (BFFs). Specifically, recovering or producing mature sperm cells from vitrified-warmed issues offers additional options in assisted reproduction. This could, in turn, enhance the genetic management of this rare and endangered species over multiple generations. The objective of the study was to evaluate structural properties, DNA fragmentation, cell viability, and germ cell composition in vitrified testicular tissues from BFFs directly after warming or after warming plus a short in vitro culture period. Tissue biopsies from five adult BFFs were either kept fresh or vitrified with a standard protocol (using dimethylsulphoxide (DMSO) and glycerol) and warmed at 50 °C for 5 s. Some of the warmed samples were then cultured in vitro for 24 h. Fresh, warmed, and warmed/cultured tissues were analyzed using different indicators: histology of seminiferous tubules, intact Sertoli cells (vimentin labeling), DNA integrity, cell viability, germ cell composition (Oct4 and Boule labeling). Percentages of intact seminiferous tubules decreased after vitrification/warming and returned to the level of fresh samples after culture. While percentages of cells labeled with vimentin, with intact DNA integrity, or proportions of viable cells were affected by vitrification/warming, they all reached similar or better levels than the fresh tissue after culture. Proportions of cells labeled with Boule antibodies also improved during in vitro culture post-warming. We demonstrated for the first time that BFF testes subjected to vitrification, rapid warming, and short in vitro culture were viable and maintained the ability to resume germ cell progression. Cryopreserved testicular tissues could potentially contribute to new strategies to enhance BFF assisted reproduction as well as conservation efforts.

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Section: Discussionmentioning

confidence: 65%