Effect of chelating and antioxidant agents on morphology and DNA methylation in freeze‐drying rabbit (<i>Oryctolagus cuniculus</i>) spermatozoa

Mercati, Francesca; Domingo, Paula; Pasquariello, Rolando; Dall'Aglio, Cecilia; Michele, Alessandro Di; Forti, Katia; Cocci, Paolo; Boiti, Cristiano; Gil, Lidia; Zerani, Massimo; Maranesi, Margherita

doi:10.1111/rda.13577

Cited by 8 publications

(6 citation statements)

References 48 publications

(61 reference statements)

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“…The process includes freezing samples followed by primary drying through sublimation of ice at freezing temperature under vacuum and secondary drying through desorption by slowly elevating temperature under vacuum (Weng 2021). Protectants and supplements used in this procedures include trehalose (Martins et al 2007, Sánchez-Partida et al 2008, Ito et al 2019, Shahmoradi et al 2021, buffers like EGTA (Liu et al 2004, Martins et al 2007, Ringleb et al 2013 or EDTA (Mercati et al 2020), fetal bovine serum (Choi et al 2011), or media/ buffer only (Keskintepe et al 2002, Kwon et al 2004). Sperm cells from many species have been preserved using that method (Patrick et al 2017a, Saragusty et al 2020.…”

Section: Dehydration Methods and Storage Options For Germplasmsmentioning

confidence: 99%

Long-term preservation of germ cells and gonadal tissues at ambient temperatures

Comizzoli

Lee

2022

Reproduction and Fertility

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Objective: To present an overview of different approaches and recent advances for long-term preservation of germ cells and gonadal tissues at ambient temperatures. Methods: Review of the existing literature. Results: Preserving viable spermatozoa, eggs, embryos, and gonadal tissues for the long term is critical in human fertility treatment and for the management of animal populations (livestock, biomedical models, and wild species). The need and number of banked germplasms are growing very fast in all disciplines, but current storage options at freezing temperatures are often constraining and not always sustainable. Recent research indicates that structures and functions of gametes or gonadal tissues can be preserved for the long-term using different strategies based on dehydration and storage at supra-zero temperatures. However, more studies are needed in rehydration and reanimation of germplasms (including proper molecular and cellular evaluations). Conclusions: While a lot of research is still warranted to optimize drying and rehydration conditions for each sample type and each species, alternative preservation methods will change the paradigm in fertility preservation and biobanking. It will transform the way we maintain and manage precious biomaterials for the long term.

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Section: Dehydration Methods and Storage Options For Germplasmsmentioning

confidence: 99%

Long-term preservation of germ cells and gonadal tissues at ambient temperatures

Comizzoli

Lee

2022

Reproduction and Fertility

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“…Membrane-permeable trehalose would, in theory, allow better control of its uptake (and removal) by changing concentrations and, even more, by longer exposure to trehalose gradients. Surprisingly, a recent report claimed that trehalose lacks any DNA protection activity (Ito et al 2019); given that this report comes from an authoritative group, alternative compounds with antioxidant activity, like rosmarinic acid or melatonin, should be explored, as suggested by Mercati et al (2020). However, in our opinion, natural xeroprotectants found in tardigrades, midges or other anhydrobiotic organisms should guide our choices.…”

Section: Future Directions: Spermatozoamentioning

confidence: 97%

Dry storage of mammalian spermatozoa and cells: state-of-the-art and possible future directions

Loi

Anzalone

Palazzese

et al. 2021

Reprod. Fertil. Dev.

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This review provides a snapshot of the current state-of-the-art of drying cells and spermatozoa. The major successes and pitfalls of the most relevant literature are described separately for spermatozoa and cells. Overall, the data published so far indicate that we are closer to success in spermatozoa, whereas the situation is far more complex with cells. Critical for success is the presence of xeroprotectants inside the spermatozoa and, even more so, inside cells to protect subcellular compartments, primarily DNA. We highlight workable strategies to endow gametes and cells with the right combination of xeroprotectants, mostly sugars, and late embryogenesis abundant (LEA) or similar ‘intrinsically disordered’ proteins to help them withstand reversible desiccation. We focus on the biological aspects of water stress, and in particular cellular and DNA damage, but also touch on other still unexplored issues, such as the choice of both dehydration and rehydration methods or approaches, because, in our view, they play a primary role in reducing desiccation damage. We conclude by highlighting the need to exhaustively explore desiccation strategies other than lyophilisation, such as air drying, spin drying or spray drying, ideally with new prototypes, other than the food and pharmaceutical drying strategies currently used, tailored for the unique needs of cells and spermatozoa.

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“…Assessments of epigenetic patterns and gene expression after dehydration have also been performed (Table 1 and Figure 1). Global DNA methylation (5‐methylcytosine) level appears not to be affected by lyophilization in rabbit sperm (Mercati et al, 2020). The proportion of cat germinal vesicles with tri‐methylation of histone H3K4me3 (detected by immunostaining) after microwave drying is lower as observed during cryopreservation (P. C. Lee & Comizzoli, 2019).…”

Section: Damages and Stresses On Biological Structures And Functions ...mentioning

confidence: 99%

“…Supplementation of drying medium with chelators like EDTA/ EGTA ensures long-term stability of mouse or hamster sperm DNA integrity during drying and storage, as well as successful embryo development after sperm injection (Kaneko & Nakagata, 2006;Muneto & Horiuchi, 2011). During the lyophilization of rabbit sperm, adding antioxidants (rosmarinic acid or melatonin) to a medium already containing a chelating agent like EDTA does not improve morphology or DNA methylation level (Mercati et al, 2020). However, desferal (an iron chelator) provides a synergistic effect with intracellular sugar (trehalose or sucrose) to improve the membrane integrity of bovine sperm during air drying (Sitaula et al, 2009).…”

Section: Fundamental Roles Of Trehalose and Chelatorsmentioning

confidence: 99%

Damages and stress responses in sperm cells and other germplasms during dehydration and storage at nonfreezing temperatures for fertility preservation

Comizzoli

Amelkina

Lee

2022

Molecular Reproduction Devel

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Long‐term preservation of sperm, oocytes, and gonadal tissues at ambient temperatures has the potential to lower the costs and simplify biobanking in human reproductive medicine, as well as for the management of animal populations. Over the past decades, different dehydration protocols and long‐term storage solutions at nonfreezing temperatures have been explored, mainly for mammalian sperm cells. Oocytes and gonadal tissues are more challenging to dehydrate so little to no progress have been made. Currently, the detrimental effects of the drying process itself are better characterized than the impact of long‐term storage at nonfreezing temperatures. While structural and functional properties of germ cells can be preserved after dehydration, a long list of damages and stresses in nuclei, organelles, and cytoplasmic membranes have been reported and sometimes mitigated. Characterizing those damages and better understanding the response of germ cells and tissues to the stress of dehydration is fundamental. It will contribute to the development of optimal protocols while proving the safety of alternative storage options for fertility preservation. The objective of this review is to (1) document the types of damages and stress responses, as well as their mitigation in cells dried with different techniques, and (2) propose new research directions.

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Effect of chelating and antioxidant agents on morphology and DNA methylation in freeze‐drying rabbit (Oryctolagus cuniculus) spermatozoa

Cited by 8 publications

References 48 publications

Long-term preservation of germ cells and gonadal tissues at ambient temperatures

Long-term preservation of germ cells and gonadal tissues at ambient temperatures

Dry storage of mammalian spermatozoa and cells: state-of-the-art and possible future directions

Damages and stress responses in sperm cells and other germplasms during dehydration and storage at nonfreezing temperatures for fertility preservation

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