CryoLetters Volume 43 - Issue 4
CryoLetters 43 (4), 189-199 (2022)
© CryoLetters, editor@cryoletters.org
doi.org/10.54680/fr22410110112
PERSPECTIVE: A state of the art review of isochoric cryopreservation and cryoprotectants
George-Andrei Beşchea1*+, Ştefan-Ioan Câmpean1+, Maria-Bianca Tăbăcaru1, Beatrice-Georgiana Vuţoiu1, Alexandru Şerban1 and Gabriel Năstase2
- Transilvania University of Braşov, Faculty of Civil Engineering, Department of Building Services, Braşov, Romania
- University Politehnica of Bucharest, Faculty of Mechanical Engineering and Mechatornics, Thermotechnics, engines, thermal and refrigeration equipment Department, Bucharest, Romania
Corresponding author’s E-mail: george.beschea@unitbv.ro
Abstract
There is a developing enthusiasm for discovering new methods, cryoprotectants, systems and devices for cells, tissues, and organ preservation in medicine, in sub-zero temperature conditions and a growing interest in developing more efficient and economical methods for long-term preservation of food in a frozen state. Most of the preservation protocols currently used in medicine and food preservation involve the use of atmospheric pressure, and temperatures lower than normal body temperature in medicine, or lower than room temperature in the food industry. In this state of the art review, we analyzed the results of a new preservation method that uses an isochoric system. We aimed to offer a clear overview of the potential of this new technology. Firstly, to study the origins of isochoric preservation, we searched using the WoS Database. A search with the world “isochoric” returned 488 results. A more specific search of the term “isochoric freezing” returned 94 results. From these searches, we selected the 12 most relevant articles and discuss them here in detail. We present an overall characterization and criticism of the current use and potential of this new preservation method that can be used in the medicine and food industry. The main findings indicate encouraging results for the tested biological matter, including for the preservation of food products (e.g. cherries, spinach, potatoes), biological organisms (e.g. Caenorhabditis elegans, Escherichia coli, Listeria, Salmonella typhimurium), organs (e.g. rat hearts), tissues (e.g., tilapia fish filets) or cells (e.g., mammalian cells, pancreatic cells). Accordingly, we conclude that the isochoric system holds huge potential as a new technique in the field of preservation.
Keywords: cryopreservation; cryoprotectants; historical events; isochoric systems
CryoLetters 43 (4), 200-205 (2022)
© CryoLetters, editor@cryoletters.org
doi.org/10.54680/fr22410110312
Potential application of cryogenic freezer on turbot sperm cryopreservation
İlhan Aydin1, Atife Tuba Beken2, Rafet Çağrı Öztïrk3, Hamza Polat2 and Yahya Terzi3*
- General Directorate of Agricultural Research and Policies-TAGEM, Ankara
- Central Fisheries Research Institute, Trabzon, Turkey
- Department of Fisheries Technology Engineering, Faculty of Marine Sciences, Karadeniz Technical University, Trabzon, Turkey
*Corresponding author’s E-mail: yhyterzi@gmail.com
Abstract
Background
Cryopreservation is a common practice to preserve fish sperm for prolonged periods.
Objective
To examine the effect of different freezing protocols on sperm characteristics, fertilization, and hatching rate of turbot.
Materials and methods
Milt was obtained from ten 8-year-old turbot (54.3 ± 1.7 cm in length and 3,106 ± 283 g in weight) at the peak of spawning season. Six batches of milts with >90% motility was pooled and diluted to 1:3 by adding dimethyl sulfoxide (DMSO, 10%) as cryoprotectant. Then straws filled with semen were subjected to three freezing protocols (cooling rates). Sperm characteristics were assessed using sperm class analyzer before and after cryopreservation. Cryopreserved and fresh sperm were used for artificial fertilization to assess fertilization and hatching rates.
Results
Cryopreservation protocol has significantly deleterious effects on total motility, progressive motility, curvilinear velocity, straight line velocity, average path velocity, linearity index, straightness index, oscillation index, and amplitude of lateral head displacement of sperm. However, the beat frequency of cryopreserved sperm was found to be similar to control sperm. The fertilization rate of sperm subjected to three freezing protocols were similar, varying between 65.3 % and 75.6 %, and the hatching rates varied from 51.2% to 70.7%.
Conclusion
The results show the potential application of cryopreservation in fish hatcheries.
Keywords: cryopreservation; sperm motility; sperm quality; turbot
CryoLetters 43 (4), 206-221 (2022)
© CryoLetters, editor@cryoletters.org
doi.org/10.54680/fr22410110512
Proteomic profile of vitrified in vitro-produced bovine embryos (Bos taurus indicus)
Joane Isis Travassos Vieira1*, José Carlos Ferreira-Silva1, Fabiana Aparecida Cavalcante Silva2, Elton Pedro Nunes Pena3, Lucas Carvalho Freitas3, Maiana Silva Chaves1, João Gabriel Viana Grázia1, Lucas Carvalho Pereira1, Renan Henrique dos Santos Fagundes1, Tercilio Calsa Junior3, José Pompeu dos Santos Filho1, Vicente José Figueiredo Freitas4 and Marcos Antonio Lemos Oliveira1
- Laboratory of Reproductive Biotechniques, Department of Veterinary Medicine, Federal Rural University of Pernambuco, Brazil
- Laboratory of Phytosanitary diagnosis, Northeast Strategic Technologies Center (CETENE), Brazil
- Laboratory of Plant Genomics and Proteomics, Department of Genetics, Federal University of Pernambuco, Brazil
- Laboratory of Physiology and Control of Reproduction, Department of Veterinary Medicine, Ceará State University, Brazil
*Corresponding author’s E-mail: ferreirasilva.jc@gmail.com
Abstract
Background
The proteomic profile of cryopreserved in vitro produced bovine embryos is little known but can provide insights on the successful application of cryo procedures in support of animal breeding.
Objective
To identify embryonic proteins and biomarkers related to improved cryotolerance of vitrified in vitro produced bovine embryos.
Materials and methods
Proteins were isolated from embryo pools (n = 25 embryos per replicate) and analyzed using the nanoLC - MS/MS system. Further, the UniProtKB database (Uniprot — http://www.uniprot.org/) was used for protein identification. Proteins were classified based on their molecular mass, isoelectric point, and enzymatic activity. Post-translational modification predictions and functional gene ontology analysis were performed as well. Finally, a protein-protein interaction network was created to shed light on the embryo interactome.
Results
Based on the MS/MS approach, 66 proteins were identified from vitrified Bos taurus embryos. The retrieved proteins were presumably annotated, which allowed a description of the qualitative and functional aspects of the embryo proteome after the vitrification process.
Conclusion
These findings allowed us to conclude that in vitro-produced vitrified embryos expressed proteins that underlie biological processes related to reproduction, stress and lipid metabolic process, which are essential to maintain embryo viability.
Keywords: blastocyst; cryopreservation; LC/MS/MS; proteome; reproduction
CryoLetters 43 (4), 222-226 (2022)
© CryoLetters, editor@cryoletters.org
doi.org/10.54680/fr22410110712
Use of biological and synthetic polymers for human spermatozoa cryopreservation
Maryna Petrushko1,2 and Taisiia Yurchuk1*
- Institute for Problems of Cryobiology and Cryomedicine (IPC&C) of the National Academy of Sciences of Ukraine, 23, Pereyaslavska Str., Kharkiv 61016, Ukraine
- ART-Clinic of Reproductive Medicine, 38B, Gagarina av., Kharkiv 61000, Ukraine
*Corresponding author’s E-mail: taisiya.yur@gmail.com
Abstract
Background
Spermatozoa cryopreservation is an integral part of the assisted reproductive technologies for treatment of infertility. It is also used to preserve the reproductive potential of men. However, using a standard freezing method with glycerol leads to a decrease in morphological and functional characteristics of spermatozoa in the case of oligoasthenoteratozoospermia (OAT). Therefore, it is relevant to develop effective methods of cryopreservation for such sperm. The use of various biopolymers can stabilize the membrane and bind excess water, which forms ice crystals in the medium that causes cell damage when temperature decreases.
Objective
To study the effectiveness of using cryoprotectant mixtures based on biological and synthetic polymers [serum albumin, polyvinylpyrrolidone (PVP) and insulin] for the cryopreservation of human spermatozoa with OAT.
Materials and methods
Human spermatozoa with OAT were cryopreserved using different cryoprotectant media containing 10% glycerol or 10% PVP, 20% albumin and 1 μg/mL human insulin. The viability, motility and mitochondrial membrane potential of spermatozoa were assessed after rewarming.
Results
A cryoprotectant solution containing 10% PVP, 20% human serum albumin and 1 μg/mL insulin enabled a similar level (%) of viable gametes compared with the standard method using glycerol, while the number of motile cells was significantly lower (p < 0.008). The membrane mitochondrial potential did not differ significantly from fresh sperm.
Conclusion
The data obtained in this study show the effectiveness of a biopolymer mixture containing PVP, serum albumin and insulin for the cryopreservation of human OAT spermatozoa.
Keywords: cryopreservation; insulin; oligoasthenoteratozoospermia; polyvinylpyrrolidone; serum albumin; spermatozoa
CryoLetters 43 (4), 227-236 (2022)
© CryoLetters, editor@cryoletters.org
doi.org/10.54680/fr22410110212
Time dependent impact of reactive oxidants on seminal attributes, mitochondrial membrane potential, lipid peroxidation and capacitation-like changes of Karan-Fries (KF) bulls during cryopreservation
Nitish. A. Kulkarni1*, A. K. Roy1, Sujata Pandita1, C. G. Shashank1 and H. S. Chethan2
- Animal Physiology Division, ICAR-National Dairy Research Institute, Karnal, Haryana, 132001, India
- Animal Reproduction Gynaecology and Obstetrics Division, ICAR-NDRI, Karnal, India
*Corresponding author’s E-mail: kulkarni.nitish97@gmail.com
Abstract
Background
Cryopreservation of semen is a valuable technique; however, it is also known to be detrimental to the structure of spermatozoa and fertility due to cryo-injury and subsequent generation of reactive oxidants.
Objective
To determine the time-dependent impact of reactive oxidants on seminal attributes, mitochondrial membrane potential (MMP), lipid peroxidation status (LPO) and early capacitation like changes.
Methods
Semen samples were collected by artificial vagina technique from six Karan-Fries (KF) bulls and subsequently examined at 0 h (before cryopreservation) and at 24 hours, 15 days and 2-months of storage for various seminal attributes, MMP (Δψm), and early capacitation-like changes. Simultaneously, LPO (TBARS) was determined in fresh and post-thaw seminal plasma.
Results
A sharp decrease (P<0.01) in semen quality was observed only after 24 h of cryopreservation except for viability and acrosomal integrity. Sperm viability and acrosome integrity reduced significantly up to 2 months of cryopreservation. The lipid peroxidation status was found to be lower in fresh seminal plasma (2.63±0.22 vs. 3.51±0.34 units/mL) as compared to post-thaw. Furthermore, the active Δψm of fresh semen showed a significant (P<0.01) decrease after 24 hours (77.92±0.387 vs. 54.52±0.28%) of cryopreservation, while there was a non-significant decrease in active MMP after 15 d and 2-months (53.68±0.138 and 52.76±0.16%). Moreover, significant (P<0.01) early capacitation-like changes were found in post-thaw spermatozoa (25.72±0.12 vs. 9.1±0.19%) as compared to fresh ejaculate.
Conclusion
Spermatozoa incur the majority of damages during the early phase of cryopreservation, however the damage associated by different stressors cannot be neglected.
Keywords: capacitation; cryopreservation; KF bulls; mitochondrial membrane potential; reactive oxygen species
CryoLetters 43 (4), 237-245 (2022)
© CryoLetters, editor@cryoletters.org
doi.org/10.54680/fr22410110412
The adaptation to freezing tolerance of hydrated lettuce seeds: effects of regional climate and of seed characteristics
Yingying Han1, Ganesh K Jaganathan1, Jingwen Zhou1, Shiwei Wei2 and Baolin Liu1*
- Institute of Biothermal Science and Technology, School of Health Science and Engineering, University of Shanghai for Science and Technology, 516 Jungong Road, Shanghai, China
- Shanghai Agrobiological Gene Center, 2901 Beidi Road, Shanghai, China
*Corresponding author’s E-mail: blliuk@163.com
Abstract
Background
With global warming, soil seed banks at high altitudes face dual challenges, excessive water absorption and thinner snow cover that increase underground temperature. A better understanding of freezing tolerance of hydrated seeds provides insights for conservation in natural soil seed banks.
Objective
To understand the adaptation mechanisms of seed freezing tolerance under various climates, in relation to cooling rate and seed size.
Materials and methods
Twelve ecotypes of lettuce (Lactuca sativa) seeds were collected from different geographical locations around the world. Seeds were fully hydrated and tested for their freezing tolerance using programmed cooling methods.
Results
The size of seeds from different climate regions varied, and was correlated with the freezing tolerance of the hydrated seeds (P<0.05). Larger seeds showed poorer freezing tolerance. The local climates of maternal plants were also well correlated to seed freezing tolerance (P<0.05), especially under slow cooling conditions. The seeds collected in regions with high spring rainfall exhibited greater freezing tolerance.
Conclusion
Freezing tolerance of hydrated seeds is affected by the climate of maternal plants and by seed size. Our data revealed the existence of an adaptation mechanism of freezing tolerance among various ecotypes of lettuce seeds.
Keywords: climate; freezing tolerance; hydrated seeds; Lactuca sativa; seed size
CryoLetters 43 (4), 246-254 (2022)
© CryoLetters, editor@cryoletters.org
doi.org/10.54680/fr22410110612
Extenders and cryosolutions for grumatã (Prochilodus vimboides) sperm preservation
Alexmiliano V. Oliveira1*, Eduardo A. T. Lanna2, Naiara C. Motta3, Guilherme Souza4, Genaina A. Souza5, Jerusa M. Oliveira6, Thiago A. Freato7 and Felipe M. Santos6
- Agricultural Research Company of Minas Gerais, EPAMIG, Viçosa, MG, Brazil
- Department of Animal Science, Federal University of Viçosa, MG, Brazil
- Department of Animal Science, Federal University of Lavras, Lavras, MG, Brazil
- Non-governmental Organization, Piabanha Project, Itaocara, RJ, Brazil
- Department of Forest Engineering, Federal University of Viçosa, MG, Brazil
- Department of Animal Biology, Federal University of Viçosa, MG, Brazil
- Meteorological and Climate Research Center Applied to Agriculture, State University of Campinas, Campinas, SP, Brazil
*Corresponding author’s E-mail: alexmiliano@epamig.br
Abstract
Background
Prochilodus vimboides populations are being reduced in rivers due to changes in their habitat, overfishing, urbanization, and pollution.
Objective
To evaluate the effect of sperm extender solutions for short-term storage and cryosolutions for freezing sperm of Prochilodus vimboides.
Materials and methods
For short-term storage, the sperm was diluted in 0.9% NaCl, 1.2% NaCl, 5% glucose, 5% BTS®, or 6% MIII®. Sperm motility was evaluated after 0, 24, 48, and 72 h of short-term storage at 4-6°C. For cryopreservation, sperm samples were diluted in the same extenders and factorially combined with three cryoprotectants (dimethylsulfoxide, methyl glycol, and ethylene glycol). After thawing, sperm motility and oxidative stress parameters were evaluated.
Results
Dilution of samples in BTS® preserved sperm motility >40% for up to 48 h. Samples cryopreserved in 5% glucose and methylglycol presented higher sperm motility, lower catalase, and lipid peroxidation activities.
Conclusion
Prochilodus vimboides sperm can be cooled for up to 48 h in an extender solution of 5% BTS® and cryopreserved in 5% glucose and methyl glycol.
Keywords: characiformes; cryopreservation; oxidative stress; short-term storage