Your search keyword '"cryoprotective agents"' showing total 261 results

1. In Vitro and In Vivo Evaluation of the Fertilization Capacity of Frozen/Thawed Rooster Spermatozoa Supplemented with Different Concentrations of Trehalose.

Author

Petričáková, Kristýna, Janošíková, Martina, Ptáček, Martin, Savvulidi, Filipp Georgijevič, and Zita, Lukáš

Subjects

*FERTILIZATION in vitro, *GENE flow, *TREHALOSE, *ARTIFICIAL insemination, *GERMPLASM, *FROZEN semen, *SPERMATOZOA, *CRYOPROTECTIVE agents

Abstract

Simple Summary: The Czech Golden Spotted Hen is the only original Czech hen breed included in the National Genetic Reserve Program. The objective of this program is to preserve the genetic resources of native breeds in the Czech Republic through reproductive biotechnologies, such as artificial insemination or the cryopreservation of sperm. The objective of the present study was to investigate the impact of varying concentrations of the non-penetrating cryoprotectant trehalose on sperm fertilization capacity. This was achieved by assessing sperm functional and kinematic parameters, as well as fertility rates. The established methodology was used to optimize the cryopreservation procedure for the National Program of Genetic Reserves of the Czech Golden Spotted Hen breed. The objective of this study was to evaluate the impact of the supplementation of varying concentrations of the impermeable disaccharide trehalose on the in vitro and in vivo fertilization capacity of cryopreserved rooster spermatozoa in the original Czech Golden Spotted Hen breed. The control trehalose concentration was 0 mM, while TRE50 (50 mM), TRE100 (100 mM), and TRE200 (200 mM) were used as experimental trehalose concentrations. The kinematic and functional parameters of frozen/thawed spermatozoa were evaluated in vitro using mobile computer-assisted sperm analysis and a flow cytometer. The addition of 100 mM trehalose demonstrated the most favorable results for total (34.17%) and progressive (3.57%) motility after thawing. A statistically significant difference was found for these kinetic parameters compared to the other monitored concentrations. This experimental group was also found to have a significantly higher percentage of spermatozoa without plasma membrane or acrosome damage (33.37%) compared to the TRE50 group (30.74%; p < 0.05) and the TRE200 group (29.05%; p < 0.05). In vivo, artificial insemination was performed to verify fertilization ability. Hens (n = 40) were artificially inseminated twice (10 hens/treatment) with a 3-day interval between inseminations. In conclusion, the addition of 100 mM trehalose significantly improved total and progressive motility after thawing and preserved plasma membrane and acrosome integrity (p < 0.05). The fertilization rate of eggs fertilized with semen frozen with the addition of 100 mM trehalose was not significantly different from the other concentrations tested or the control group but was numerically higher (23.21% vs. 15.20% of fertilized eggs in this group). [ABSTRACT FROM AUTHOR]

Published

2024

2. Orthobiologic Products: Preservation Options for Orthopedic Research and Clinical Applications.

Author

Fang, William H. and Vangsness Jr., C. Thomas

Subjects

*MESENCHYMAL stem cells, *BIOLOGICAL products, *PROGENITOR cells, *EXTRACELLULAR vesicles, *CRYOPROTECTIVE agents

Abstract

The biological products used in orthopedics include musculoskeletal allografts—such as bones, tendons, ligaments, and cartilage—as well as biological therapies. Musculoskeletal allografts support the body's healing process by utilizing preserved and sterilized donor tissue. These allografts are becoming increasingly common in surgical practice, allowing patients to avoid more invasive procedures and the risks associated with donor site morbidity. Bone grafting is one of the most frequently used procedures in orthopedics and traumatology. Biologic approaches aim to improve clinical outcomes by enhancing the body's natural healing capacity and reducing inflammation. They serve as an alternative to surgical interventions. While preliminary results from animal studies and small-scale clinical trials have been promising, the field of biologics still lacks robust clinical evidence supporting their efficacy. Biological therapies include PRP (platelet-rich plasma), mesenchymal stem cells (MSCs)/stromal cells/progenitor cells, bone marrow stem/stromal cells (BMSCs), adipose stem/stromal cells/progenitor cells (ASCs), cord blood (CB), and extracellular vesicles (EVs), including exosomes. The proper preservation and storage of these cellular therapies are essential for future use. Preservation techniques include cryopreservation, vitrification, lyophilization, and the use of cryoprotective agents (CPAs). The most commonly used CPA is DMSO (dimethyl sulfoxide). The highest success rates and post-thaw viability have been achieved by preserving PRP with a rate-controlled freezer using 6% DMSO and storing other cellular treatments using a rate-controlled freezer with 5% or 10% DMSO as the CPA. Extracellular vesicles (EVs) have shown the best results when lyophilized with 50 mM or 4% trehalose to prevent aggregation and stored at room temperature. [ABSTRACT FROM AUTHOR]

Published

2024

3. Permeability and Toxicity of Cryoprotective Agents in Silkworm Embryos: Impact on Cryopreservation.

Author

Urbán-Duarte, David, Tomita, Shuichiro, Sakai, Hiroki, Sezutsu, Hideki, Álvarez-Gallardo, Horacio, Kainoh, Yooichi, Furukawa, Seiichi, and Uchino, Keiro

Subjects

*CRYOPROTECTIVE agents, *SILKWORMS, *PROPYLENE glycols, *DIMETHYL sulfoxide, *VITRIFICATION

Abstract

The permeation of cryoprotectants into insect embryos is critical for successful cryopreservation. However, the permeability of silkworm embryos to cryoprotectants and the effects of cryopreservation remain poorly studied. In this study, we evaluated the permeability and toxicity of four cryoprotective agents (CPAs) as well as the vitrification effect on the viability of silkworm embryos. Among the four CPAs, propylene glycol (PG) showed the best permeability. Ethylene glycol (EG) and PG were the least toxic CPAs, but glycerol (GLY) and dimethyl sulfoxide (DMSO) were more toxic. Moreover, we examined several factors including the kind and the concentration of CPAs, exposure time, embryonic stage, and silkworm strains. Embryos at the earlier phases of stage 25 were more tolerant to vitrification using EG. We found that over 21% of embryos treated with EG at the early 2 phase of stage 25: 163 h after egg laying (AEL) developed and progressed to serosa ingestion after vitrification and rewarming. The result was the same in other strains as well. Our results are valuable for the development of new cryopreservation protocols of silkworm embryos. [ABSTRACT FROM AUTHOR]

Published

2024

4. Evaluation of Cryopreservation of Bovine Ovarian Tissue by Analysis of Reactive Species of Oxygen, Toxicity, Morphometry, and Morphology.

Author

Bizarro-Silva, Camila, Bergamo, Larissa Zamparone, Costa, Camila Bortoliero, González, Suellen Miguez, Yokomizo, Deborah Nakayama, Rossaneis, Ana Carolina, Verri Junior, Waldiceu Aparecido, Sudano, Mateus José, Andrade, Evelyn Rabelo, Alfieri, Amauri Alcindo, and Seneda, Marcelo Marcondes

Subjects

OVARIAN transplantation, REACTIVE oxygen species, OVARIES, TRANSPLANTATION of organs, tissues, etc., REPRODUCTIVE technology, OVARIAN follicle, CRYOPROTECTIVE agents

Abstract

Simple Summary: There is a growing demand for the development of optimal protocols for ovarian tissue cryopreservation in different animal models to enable the maintenance of cell morphology. Therefore, it is crucial to understand the effects of conservation on ovarian cell proliferation and apoptosis to improve follicular development after in vitro culture and/or ovarian tissue transplantation. This study compared the effects of three concentrations (1, 1.5, and 3 M) of dimethyl sulfoxide (DMSO) during vitrification to identify optimal conditions for preserving bovine preantral follicles and to contribute to the improvement of the technique and its future application in assisted reproduction procedures. Following vitrification, cryopreserved ovarian fragments exhibited similar percentages of intact follicles, with only the 3 M DMSO concentration differing from the control. Upon analyzing the free radical production, the 3 M concentration exhibited higher oxidative stress levels than lower DMSO concentrations. Exposure to 3 M DMSO for 30 min led to a higher rate of follicular degeneration. After in vitro cultivation of the vitrified fragments, the 1 M DMSO concentration showed higher percentages of morphologically intact follicles than the other concentrations. Accordingly, bovine preantral follicles could be cryopreserved in situ with greater efficiency in 1 M DMSO. Ovarian tissue cryopreservation has been widely investigated for preserving female fertility. In the present study, we aimed to compare the effects of three concentrations (1, 1.5, and 3 M) of dimethylsulfoxide (DMSO) on the vitrification of ovarian tissue. The ovarian cortex was divided into control and vitrified groups: (i) 1 M-DMSO, (ii) 1.5 M-DMSO, and (iii) 3 M-DMSO. Follicles from all fragments were analyzed for DMSO-induced deleterious effects, morphological and morphometric aspects, and concentration of reactive oxygen species. Additionally, the fragments were cultured to assess the integrity and return of follicular development post-vitrification. All DMSO concentrations resulted in a higher percentage of degenerated preantral follicles than before the cryopreservation process. After vitrification, the cryopreserved ovarian fragments showed similar percentages of intact follicles; however, the 3 M DMSO concentration differed from the control. Analyzing free radical production, we found that the 3 M DMSO concentration had higher levels of oxidative stress than the lower DMSO. After in vitro cultivation of the vitrified/warmed fragments, the 1 M DMSO concentration exhibited higher percentages of morphologically intact follicles than the other concentrations. Therefore, we suggest that bovine preantral follicles can be cryopreserved in situ with greater efficiency in 1 M DMSO. [ABSTRACT FROM AUTHOR]

Published

2024

5. Current State and Challenges of Tissue and Organ Cryopreservation in Biobanking.

Author

Khaydukova, Irina V., Ivannikova, Valeria M., Zhidkov, Dmitry A., Belikov, Nikita V., Peshkova, Maria A., Timashev, Peter S., Tsiganov, Dmitry I., and Pushkarev, Aleksandr V.

Subjects

*BIOMATERIALS, *ICE crystals, *TISSUES, *REGENERATIVE medicine, *REPRODUCTIVE health, *CRYOPROTECTIVE agents

Abstract

Recent years have witnessed significant advancements in the cryopreservation of various tissues and cells, yet several challenges persist. This review evaluates the current state of cryopreservation, focusing on contemporary methods, notable achievements, and ongoing difficulties. Techniques such as slow freezing and vitrification have enabled the successful preservation of diverse biological materials, including embryos and ovarian tissue, marking substantial progress in reproductive medicine and regenerative therapies. These achievements highlight improved post-thaw survival and functionality of cryopreserved samples. However, there are remaining challenges such as ice crystal formation, which can lead to cell damage, and the cryopreservation of larger, more complex tissues and organs. This review also explores the role of cryoprotectants and the importance of optimizing both cooling and warming rates to enhance preservation outcomes. Future research priorities include developing new cryoprotective agents, elucidating the mechanisms of cryoinjury, and refining protocols for preserving complex tissues and organs. This comprehensive overview underscores the transformative potential of cryopreservation in biomedicine, while emphasizing the necessity for ongoing innovation to address existing challenges. [ABSTRACT FROM AUTHOR]

Published

2024

6. Hormone-Driven Temperature Optimization for Elevated Reproduction in Goldfish (Carassius auratus) under Laboratory Conditions.

Author

Taheri-Khas, Zeynab, Gharzi, Ahmad, Vaissi, Somaye, Heshmatzad, Pouria, and Kalhori, Zahra

Subjects

*FERTILIZATION in vitro, *TEMPERATURE control, *FISH larvae, *FISH farming, *GOLDFISH, *FROZEN semen, *CRYOPROTECTIVE agents, *SPERMATOZOA

Abstract

Simple Summary: This study investigated the use of hormones and temperature control to improve breeding success. Injecting Ovaprim significantly increased egg and sperm production. However, temperature played a critical role. A medium temperature (around 22 °C) produced the best results, with more eggs, faster egg release, and healthier sperm. Both low and high temperatures negatively impacted sperm quality and larval fish survival. Using extender E4 (15% DMSO) for cryopreservation improved fertilization rates. Overall, the study highlights the importance of precise hormone control and temperature management for successful goldfish reproduction, benefiting for fish farming. This study investigates the efficacy of hormone-induced artificial reproduction in goldfish (Carassius auratus) under controlled temperatures. Ovaprim injections significantly enhanced ovulation and sperm production compared to controls. Medium temperature (22 °C) produced the highest ovulation rates, fastest ovulation timing, and optimal sperm quality (motility and morphology) compared to high (28 °C) and low (16 °C) temperature groups. The low-temperature group exhibited reduced sperm motility duration and higher rates of sperm and larvae damage. The sperm volume of the high-temperature group was higher, but their post-injection survival rates were lower. Furthermore, the lowest spawning rate and low egg quality were noted in the high temperature. Cryopreservation using extender E4 (15% DMSO) exhibited superior post-thaw sperm motility and achieved higher fertilization rates. Fertilization rates, embryo development, and larval survival were all highest at the medium temperature. Larvae hatched from fresh sperm at medium temperature exhibited faster growth and fewer deformities. These findings suggest that hormone stimulation coupled with a medium temperature regimen is critical for successful artificial reproduction in goldfish. Cryopreservation with extender E4 holds promise for sperm banking; however, further optimization is necessary to improve fertilization success with thawed sperm. Future research could explore the influence of temperature on sperm physiology and refine cryopreservation protocols to enhance fertilization rates. [ABSTRACT FROM AUTHOR]

Published

2024

7. Addition of Cryoprotectant DMSO Reduces Damage to Spermatozoa of Yellow Catfish (Pelteobagrus fulvidraco) during Cryopreservation: Ultrastructural Damage, Oxidative Damage and DNA Damage.

Author

Zhang, Yuxin, Liu, Dongqing, Wang, Qinghua, Ruan, Qingxin, Hua, Sijie, Zhang, Weiwei, Yang, Sen, and Meng, Zining

Subjects

*FLATHEAD catfish, *GERMPLASM conservation, *SPERM motility, *GERMPLASM, *ELECTRON microscopes, *FROZEN semen, *CRYOPROTECTIVE agents

Abstract

Simple Summary: Spermatozoa cryopreservation technology has been widely used to preserve high-quality male spermatozoa and has to some extent solved the problem of spermatozoa supply in yellow catfish (Pelteobagrus fulvidraco). However, cryopreservation can still cause cellular damage and affect spermatozoa viability and fertility. Therefore, it is necessary to study cryo-injury, which is beneficial for further optimizing the spermatozoa cryopreservation protocol. In this experiment, we investigated the effects of adding or not adding 10% DMSO on spermatozoa motility, ultrastructural damage, oxidative damage, and DNA damage of thawed yellow catfish. Using 10% DMSO as a cryoprotectant can improve spermatozoa motility (75.64 ± 1.12), significantly alleviate injuries to organelles and membrane structures, improve SOD (7.99 × 104 ± 5.24 nmol/mgprot) and T-AOC (3.7 × 105 ± 0.06 nmol/mgprot) enzyme activity, reduce MDA (1.09 ± 0.45 nmol/mgprot) enzyme activity, and mitigate the degree of oxidative damage. It also greatly reduces the DNA fragmentation rate (59 ± 1.56%). The research results provide data support for the optimization of the cryopreservation protocol for the spermatozoa of yellow catfish, which is beneficial for the preservation of the germplasm resources of yellow catfish and the effective utilization of resources during large-scale production. Spermatozoa cryopreservation protocols have been established for yellow catfish (Pelteobagrus fulvidraco), but cryopreservation can still cause cellular damage and affect spermatozoa viability and fertility. Therefore, the aim of this paper was to evaluate the effects of adding or not adding cryoprotectants during low-temperature storage on the ultrastructural damage, oxidative damage, and DNA damage of thawed yellow catfish spermatozoa. The mixed semen of three male yellow catfish was divided into a fresh spermatozoa group, a frozen spermatozoa group (DMSO+) with a cryoprotectant (10% DMSO), and a frozen spermatozoa group without a cryoprotectant (DMSO−). Ultrastructural of the spermatozoa after thawing were observed under an electron microscope and the spermatozoa were assayed for SOD, MDA, and T-AOC enzyme activities, as well as for DNA integrity. In terms of movement parameters, compared with DMSO−, the addition of DMSO has significantly improved sperm motility, curve line velocity (VCL), and straight line velocity (VSL). The ultrastructural results showed that although thawed spermatozoa exhibited increased damage than fresh spermatozoa, 10% DMSO effectively reduced the damage to the plasma membrane, mitochondria, and flagellum of spermatozoa by cryopreservation, and most of the spermatozoa were preserved with intact structure. The results of oxidative damage showed that compared with frozen spermatozoa, 10% DMSO significantly increased the activities of SOD and T-AOC enzymes and clearly reduced the activity of the MDA enzyme. The antioxidant capacity of spermatozoa was improved, lipid peroxidation was reduced, and the oxidative damage caused by cryopreservation was mitigated. The DNA integrity of spermatozoa showed that 10% DMSO clearly reduced the DNA fragmentation rate. In conclusion, 10% DMSO can effectively reduce the ultrastructural damage, oxidative damage, and DNA damage of yellow catfish spermatozoa during cryopreservation; it can also further optimize the cryopreservation protocol for yellow catfish spermatozoa. Meanwhile, it also provides a theoretical basis for the future optimization of the cryopreservation protocols. [ABSTRACT FROM AUTHOR]

Published

2024

8. Exploring the Potential Effects of Cryopreservation on the Biological Characteristics and Cardiomyogenic Differentiation of Rat Adipose-Derived Mesenchymal Stem Cells.

Author

Farag, Ahmed, Ngeun, Sai Koung, Kaneda, Masahiro, Aboubakr, Mohamed, Elhaieg, Asmaa, Hendawy, Hanan, and Tanaka, Ryou

Subjects

*MESENCHYMAL stem cell differentiation, *TROPONIN I, *MESENCHYMAL stem cells, *CRYOPRESERVATION of cells, *GENE expression, *CRYOPROTECTIVE agents

Abstract

Cryopreservation is essential for the broad clinical application of mesenchymal stem cells (MSCs), yet its impact on their cellular characteristics and cardiomyogenic differentiation potential remains a critical concern in translational medicine. This study aimed to evaluate the effects of cryopreservation on the biological properties and cardiomyogenic capacity of rat adipose-derived MSCs (AD-MSCs). We examined their cellular morphology, surface marker expression (CD29, CD90, CD45), trilineage differentiation potential (adipogenic, osteogenic, chondrogenic), and gene expression profiles for the pluripotency marker REX1 and immunomodulatory markers TGFβ1 and IL-6. After inducing cardiomyocyte differentiation, we assessed cardiac-specific gene expressions (Troponin I, MEF2c, GSK-3β) using quantitative RT-qPCR, along with live/dead cell staining and immunofluorescence for cardiac-specific proteins (Troponin T, α-actinin, Myosin Heavy Chain). Cryopreserved AD-MSCs preserved their morphology, surface markers, and differentiation potential, but exhibited a reduced expression of REX1, TGFβ1, and IL-6. Additionally, cryopreservation diminished cardiomyogenic differentiation, as indicated by the lower levels of Troponin I, MEF2c, and GSK-3β seen compared to non-cryopreserved cells. Despite this, high cell viability (>90%) and maintained cardiac protein expression were observed post-cryopreservation. These findings highlight the necessity of optimizing cryopreservation protocols to ensure the full therapeutic potential of AD-MSCs, particularly in applications related to cardiac regenerative medicine. [ABSTRACT FROM AUTHOR]

Published

2024

9. Effects of Cryoprotectant Concentration and Exposure Time during Vitrification of Immature Pre-Pubertal Lamb Cumulus–Oocyte Complexes on Nuclear and Cytoplasmic Maturation.

Author

Temerario, Letizia, Martino, Nicola Antonio, Bennink, Monika, de Wit, Agnes, Hiemstra, Sipke Joost, Dell'Aquila, Maria Elena, and Lamy, Julie

Subjects

*OVUM, *SHEEP breeds, *ETHYLENE glycol, *REACTIVE oxygen species, *SHEEP breeding, *CRYOPROTECTIVE agents

Abstract

Simple Summary: In the last years, many domesticated and wild animal species, as well as local and transboundary breeds, have been threatened with genetic depletion and extinction. The application of conservation strategies to sheep breeds is necessary to safeguard the productive characteristics but also the historical and cultural value that they exert on their territory and inhabitants. Despite many advances that have been made in gamete cryopreservation, in vitro embryo production (IVEP) and juvenile in vitro production (JIVET), the efficiency of these technologies is still low, and the application is restricted in the ovine species. In the present study, a high concentration-rapid exposure (HC-RE) and a low concentration-slow exposure (LC-SE) vitrification protocol, using dimethyl sulfoxide (DMSO) and ethylene glycol (EG) as permeating cryoprotectants (CPAs), were applied to pre-pubertal lamb immature cumulus–oocyte complexes (COCs) and evaluated on nuclear and cytoplasmic parameters after in vitro maturation (IVM). Slightly more encouraging results were observed with the LC-SE vitrification protocol, leading to the hypothesis that low CPA concentrations in association with prolonged exposure times could be more promising to pursue in order to improve pre-pubertal lamb immature COC vitrification. Oocyte vitrification allows for the storing of endangered breed female gametes. Cryoprotectant (CPA) concentration and exposure time should ensure cell protection with minimal toxicity. In the present study, a high concentration-rapid exposure (HC-RE) and a low concentration-slow exposure (LC-SE) vitrification protocol, using dimethyl sulfoxide (DMSO) and ethylene glycol (EG) as permeating CPAs, were evaluated on meiotic competence and bioenergetic-oxidative status of pre-pubertal lamb immature COCs after in vitro maturation (IVM). For each protocol, COCs vitrified through a traditional protocol and fresh ones were used as controls. Both protocols allowed COC morphology preservation after vitrification-warming (V-W) and cumulus expansion after IVM. The maturation rate (7% and 14%) was comparable to the vitrified control (13% and 21%) but not satisfactory compared to fresh ones (58% and 64%; p < 0.001). The rate of mature oocytes displaying a perinuclear/subcortical (P/S) mitochondrial distribution pattern, an index of cytoplasmic maturity, was comparable between vitrified and fresh oocytes. The LC-SE vitrification protocol did not affect quantitative bioenergetic-oxidative parameters compared to both controls whereas HC-RE protocol significantly reduced intracellular reactive oxygen species (ROS) levels, indicating cell viability loss. In conclusion, to improve pre-pubertal lamb immature COC vitrification, the combination of low CPA concentrations with prolonged exposure time could be more promising to investigate further. [ABSTRACT FROM AUTHOR]

Published

2024

10. Comparative Study on the Sperm Proteomes of Horses and Donkeys.

Author

Ren, Hong, Wen, Xin, He, Qianqian, Yi, Minna, Dugarjaviin, Manglai, and Bou, Gerelchimeg

Subjects

*PROTEIN expression, *SPERMATOZOA, *MASS spectrometry, *DONKEYS, *FERTILITY, *HORSES, *CRYOPROTECTIVE agents

Abstract

Simple Summary: This study identified the protein expression profiles of horse and donkey sperm and investigated the effect of sperm proteins on sperm viability. In short, we first assessed the viability of horse and donkey sperm, revealing higher viability in donkey sperm compared to horse sperm. Subsequently, 4D-DIA protein-sequencing technology was employed to identify 3436 proteins expressed in horse sperm and 3404 proteins expressed in donkey sperm, with 73 proteins specific to horse sperm, and 41 specific to donkey sperm. Further analysis established a correlation between sperm proteins and sperm viability. These findings are significant in elucidating the reproductive variances and evolutionary relationships between horses and donkeys. The reproductive performance of horse sperm and donkey sperm has been reported to differ. Sperm proteins play a crucial role in sperm viability and fertility. Although differences between species are known, no prior study has investigated disparities in the sperm proteome between horses and donkeys. Therefore, this study characterized and compared the sperm proteomes of horses and donkeys using 4D-DIA mass spectrometry technology. We identified 3436 proteins in horse sperm and 3404 proteins in donkey sperm. Of these, 3363 proteins were expressed in both horse and donkey sperm, with 73 proteins being specifically expressed in horse sperm, and 41 in donkey sperm. According to data analysis, donkeys exhibited a greater percentage of motility and progressive movement in straight-line sperm than horses, as well as lower percentages of static and slow sperm than horses. Joint analysis of the results from the horse and donkey sperm proteomes and their CEROS II-read parameters demonstrated a possible association between sperm proteins and their sperm viability patterns. These findings suggest that there are discrepancies in the expression levels and protein compositions of horse and donkey sperm and that certain specific proteins may be responsible for the differences in performance between these two species. [ABSTRACT FROM AUTHOR]

Published

2024

11. In Vitro Gene Conservation Status and the Quality of the Genetic Resources of Native Hungarian Sheep Breeds.

Author

Mujitaba, Malam Abulbashar, Tokár, Alexandra, Balogh, Eszter Erika, Debnár, Viktória Johanna, Javkhlan, Ariuntungalag, Vásárhelyi, Panka Boglárka, Egerszegi, István, Nagy, Szabolcs Tamás, and Kútvölgyi, Gabriella

Subjects

GERMPLASM, SHEEP breeding, SPERMATOZOA, COMMUNITY banks, SEMEN, SHEEP breeds, CRYOPROTECTIVE agents

Abstract

Simple Summary: Considering the global decline in local sheep genetic resources, we conducted the current study to assess the status and quality of Hungarian native sheep breed genetic resources stored in a small Gene Bank established between 2014 and 2017. Semen samples from 24 rams of different breeds were collected during the breeding season and out of season using an artificial vagina, cryopreserved manually. Frozen/thawed spermatozoa were evaluated for motility and kinematic parameters, viability, chromatin structure, and morphometry of the sperm nuclei. We observed breed, season, and individual ram effects on the motility, kinematics, viability, and morphometrical parameters of the post-thaw spermatozoa samples stored in the Gene Bank. The stored samples are of good quality, and the cryopreservation technique adopted for the small Gene Bank proved promising for conserving the genetic resources of the native Hungarian sheep, as it resulted in acceptable post-thaw parameters. To maintain rare and valuable genotypes, cryo-conservation of not only spermatozoa but also oocytes and embryos is needed. Therefore, we plan to implement an extended gene conservation program involving a more significant number of individuals of native Hungarian sheep breeds. Studies revealed a global loss of genetic resources for local sheep breeds. Therefore, the current study aimed to introduce and highlight the progress made on Hungary's existing gene conservation program (small Gene Bank). Furthermore, we evaluated breed (Tsigai, Cikta, and Racka), season, and individual variabilities (n = 24) of the pre-freeze and post-thaw semen stored in the Gene Bank to enhance the gene conservation of the breeds. The samples were cryopreserved manually, and post-thaw spermatozoa were analyzed for motility (CASA), viability, chromatin structure, and morphometry of the sperm nuclei. Ejaculate volume, spermatozoa concentration, subjective motility and standard motility, kinematic parameters, and spermatozoa's head area standard deviation of the post-thaw samples differed significantly among breeds (p < 0.05). Season affected ejaculate volume, total spermatozoa number/ejaculate, STR, BCF, and ALH. We observed a significant (p < 0.001; 0.05) breed and season interaction on concentration, total spermatozoa number/ejaculate, VCL, LIN, WOB, spermatozoa's head average perimeter and nucleus length (Tsigai and Cikta differed but were statistically the same as Racka). Similarly, season significantly (p < 0.05) affected the proportion of ejaculate suitable for freezing. There was a significant (p < 0.05) difference in kinematic parameters and viability among the rams across the breeds. The spermatozoa's head morphometry of the Tsigai and Cikta breeds differed significantly (p < 0.05) among the rams. There were individual and breed differences in many spermatozoa quality parameters. The stored samples are of good quality, with more than 40% having intact membranes and low abnormal chromatin condensation. [ABSTRACT FROM AUTHOR]

Published

2024

12. In Vitro Generation of Haploid Germ Cells from Human XY and XXY Immature Testes in a 3D Organoid System.

Author

Galdon, Guillermo, Zarandi, Nima Pourhabibi, Deebel, Nicholas A., Zhang, Sue, Cornett, Olivia, Lyalin, Dmitry, Pettenati, Mark J., Lue, YanHe, Wang, Christina, Swerdloff, Ronald, Shupe, Thomas D., Bishop, Colin, Stogner, Kimberly, Kogan, Stanley J., Howards, Stuart, Atala, Anthony, and Sadri-Ardekani, Hooman

Subjects

*GERM cell differentiation, *FLUORESCENCE in situ hybridization, *KLINEFELTER'S syndrome, *X chromosome, *GERM cells, *CRYOPROTECTIVE agents

Abstract

Increasing survival rates of children following cancer treatment have resulted in a significant population of adult survivors with the common side effect of infertility. Additionally, the availability of genetic testing has identified Klinefelter syndrome (classic 47,XXY) as the cause of future male infertility for a significant number of prepubertal patients. This study explores new spermatogonia stem cell (SSC)-based fertility therapies to meet the needs of these patients. Testicular cells were isolated from cryopreserved human testes tissue stored from XY and XXY prepubertal patients and propagated in a two-dimensional culture. Cells were then incorporated into a 3D human testicular organoid (HTO) system. During a 3-week culture period, HTOs maintained their structure, viability, and metabolic activity. Cell-specific PCR and flow cytometry markers identified undifferentiated spermatogonia, Sertoli, Leydig, and peritubular cells within the HTOs. Testosterone was produced by the HTOs both with and without hCG stimulation. Upregulation of postmeiotic germ cell markers was detected after 23 days in culture. Fluorescence in situ hybridization (FISH) of chromosomes X, Y, and 18 identified haploid cells in the in vitro differentiated HTOs. Thus, 3D HTOs were successfully generated from isolated immature human testicular cells from both euploid (XY) and Klinefelter (XXY) patients, supporting androgen production and germ cell differentiation in vitro. [ABSTRACT FROM AUTHOR]

Published

2024

13. Effects of Cannabinoids on Intestinal Motility, Barrier Permeability, and Therapeutic Potential in Gastrointestinal Diseases.

Author

Crowley, Kijan, Kiraga, Łukasz, Miszczuk, Edyta, Skiba, Sergiusz, Banach, Joanna, Latek, Urszula, Mendel, Marta, and Chłopecka, Magdalena

Subjects

*TRP channels, *CANNABINOIDS, *INTESTINAL barrier function, *GASTROINTESTINAL diseases, *ADENYLATE cyclase, *CRYOPROTECTIVE agents, *PERMEABILITY

Abstract

Cannabinoids and their receptors play a significant role in the regulation of gastrointestinal (GIT) peristalsis and intestinal barrier permeability. This review critically evaluates current knowledge about the mechanisms of action and biological effects of endocannabinoids and phytocannabinoids on GIT functions and the potential therapeutic applications of these compounds. The results of ex vivo and in vivo preclinical data indicate that cannabinoids can both inhibit and stimulate gut peristalsis, depending on various factors. Endocannabinoids affect peristalsis in a cannabinoid (CB) receptor-specific manner; however, there is also an important interaction between them and the transient receptor potential cation channel subfamily V member 1 (TRPV1) system. Phytocannabinoids such as Δ9-tetrahydrocannabinol (THC) and cannabidiol (CBD) impact gut motility mainly through the CB1 receptor. They were also found to improve intestinal barrier integrity, mainly through CB1 receptor stimulation but also via protein kinase A (PKA), mitogen-associated protein kinase (MAPK), and adenylyl cyclase signaling pathways, as well as by influencing the expression of tight junction (TJ) proteins. The anti-inflammatory effects of cannabinoids in GIT disorders are postulated to occur by the lowering of inflammatory factors such as myeloperoxidase (MPO) activity and regulation of cytokine levels. In conclusion, there is a prospect of utilizing cannabinoids as components of therapy for GIT disorders. [ABSTRACT FROM AUTHOR]

Published

2024

14. Cryopreservation of Potamotrygon Stingrays' Semen: Enhancing One Conservation Effort.

Author

Ramos, Sofia Dressel, Jorge-Neto, Pedro Nacib, Colbachini, Helen, Gricio, Emanuele Almeida, de Moraes Francisco, Fábio, Padilha, Fabiana Lucia André, Gutierrez, Rafael Caprioli, Requena, Letícia Alecho, Reisfeld, Laura Chrispim, Henrique, Paloma Canedo, Leite, Roberta Ferreira, and Pizzutto, Cristiane Schilbach

Subjects

*FROZEN semen, *SEMEN, *CRYOPROTECTIVE agents, *SPERMATOZOA, *REPRODUCTIVE technology, *STINGRAYS, *ANIMAL breeders, *BIOMETRIC identification

Abstract

This pioneering study aimed to evaluate the cryopreservation of semen from P. falkneri (n = 4) and P. motoro (n = 4), maintained ex situ at the Sao Paulo Aquarium, Brazil. For this purpose, the animals were physically restrained, biometric data of the disc and clasper were obtained, and semen was collected through manual massage. Total motility and progressive motility parameters were evaluated using Computer-Assisted Sperm Analysis (CASA) with IVOS II equipment and Animal Breeders II software. The semen extenders INRA 96 and OptiXcell were used to assess their efficacy in sperm cryopreservation. INRA required the addition of 5% dimethyl sulfoxide (DMSO) as a cryoprotectant. The results indicated that there was no difference in semen motility values before and after freezing with INRA + DMSO (p = 0.6226). On the other hand, samples cryopreserved with OptiXcell showed a difference in semen motility post-thaw (p = 0.0156). These findings contribute to a broader study on optimizing cryopreservation protocols to ensure long-term viability and fertility of semen, enhancing genetic diversity and supporting wild population restoration. A multidisciplinary approach integrating reproductive biology, ecology, physiology, and assisted reproduction technologies, aligned with the One Conservation concept, is essential for advancing conservation and management strategies for these threatened species. [ABSTRACT FROM AUTHOR]

Published

2024

15. Phonon Properties and Lattice Dynamics of Two- and Tri-Layered Lead Iodide Perovskites Comprising Butylammonium and Methylammonium Cations—Temperature-Dependent Raman Studies.

Author

Mączka, Mirosław, Smółka, Szymon, and Ptak, Maciej

Subjects

*PEROVSKITE, *PHONONS, *LEAD iodide, *PHASE transitions, *ELECTRON-phonon interactions, *LATTICE dynamics, *RAMAN scattering, *CRYOPROTECTIVE agents

Abstract

Hybrid lead iodide perovskites are promising photovoltaic and light-emitting materials. Extant literature data on the key optoelectronic and luminescent properties of hybrid perovskites indicate that these properties are affected by electron–phonon coupling, the dynamics of the organic cations, and the degree of lattice distortion. We report temperature-dependent Raman studies of BA2MAPb2I7 and BA2MA2Pb3I10 (BA = butylammonium; MA = methylammonium), which undergo two structural phase transitions. Raman data obtained in broad temperature (360–80 K) and wavenumber (1800–10 cm−1) ranges show that ordering of BA+ cations triggers the higher temperature phase transition, whereas freezing of MA+ dynamics occurs below 200 K, leading to the onset of the low-temperature phase transition. This ordering is associated with significant deformation of the inorganic sublattice, as evidenced by changes observed in the lattice mode region. Our results show, therefore, that Raman spectroscopy is a very valuable tool for monitoring the separate dynamics of different organic cations in perovskites, comprising "perovskitizer" and interlayer cations. [ABSTRACT FROM AUTHOR]

Published

2024

16. A New Cell Line from the Brain of Red Hybrid Tilapia (Oreochromis spp.) for Tilapia Lake Virus Propagation.

Author

Mohamad, Aslah, Khemthong, Matepiya, Trongwongsa, Pirada, Lertwanakarn, Tuchakorn, Setthawong, Piyathip, and Surachetpong, Win

Subjects

*CELL lines, *TILAPIA, *CYTOCHROME oxidase, *CRYOPROTECTIVE agents, *VIRUS diseases, *CELL culture

Abstract

Simple Summary: Simple Summary: In this study, a new cell line derived from red hybrid tilapia brain tissue, RHTiB, was established. This fibroblast-like cell line was maintained for over 50 passages with optimal growth at 25 °C in Leibovitz-15 medium with 10% fetal bovine serum at pH 7.4. Genetic and chromosomal analyses confirmed its origin from red hybrid tilapia. Additionally, immunofluorescence and RT-qPCR tests revealed successful TiLV propagation in RHTiB cell lines. The development of this novel cell line offers valuable prospects in enhancing diagnostic techniques in red hybrid tilapia. Tilapia lake virus (TiLV) presents a substantial threat to global tilapia production. Despite the development of numerous cell lines for TiLV isolation and propagation, none have been specifically derived from red hybrid tilapia (Oreochromis spp.). In this study, we successfully established a new cell line, RHTiB, from the red hybrid tilapia brain. RHTiB cells were cultured for 1.5 years through over 50 passages and demonstrated optimal growth at 25 °C in Leibovitz-15 medium supplemented with 10% fetal bovine serum at pH 7.4. Morphologically, RHTiB cells displayed a fibroblast-like appearance, and cytochrome oxidase I gene sequencing confirmed their origin from Oreochromis spp. Mycoplasma contamination testing yielded negative results. The revival rate of the cells post-cryopreservation was observed to be between 75 and 80% after 30 days. Chromosomal analysis at the 25th passage revealed a diploid count of 22 pairs (2n = 44). While no visible cytopathic effects were observed, both immunofluorescence microscopy and RT-qPCR analysis demonstrated successful TiLV propagation in the RHTiB cell line, with a maximum TiLV concentration of 107.82 ± 0.22 viral copies/400 ng cDNA after 9 days of incubation. The establishment of this species-specific cell line represents a valuable advancement in the diagnostic and isolation tools for viral diseases potentially impacting red hybrid tilapia. [ABSTRACT FROM AUTHOR]

Published

2024

17. New Approach to the Cryopreservation of GV Oocytes and Cumulus Cells through the Lens of Preserving the Intercellular Gap Junctions Based on the Bovine Model.

Author

Yurchuk, Taisiia, Likszo, Pawel, Witek, Krzysztof, Petrushko, Maryna, and Skarzynski, Dariusz J.

Subjects

*CELL junctions, *OVUM, *CRYOPROTECTIVE agents, *GENE expression, *BOS, *CRYOPRESERVATION of cells

Abstract

Differences in structural and functional properties between oocytes and cumulus cells (CCs) may cause low vitrification efficiency for cumulus–oocyte complexes (COCs). We have suggested that the disconnection of CCs and oocytes in order to further cryopreservation in various ways will positively affect the viability after thawing, while further co-culture in vitro will contribute to the restoration of lost intercellular gap junctions. This study aimed to determine the optimal method of cryopreservation of the suspension of CCs to mature GV oocytes in vitro and to determine the level of mRNA expression of the genes (GJA1, GJA4; BCL2, BAX) and gene-specific epigenetic marks (DNMT3A) after cryopreservation and in vitro maturation (IVM) in various culture systems. We have shown that the slow freezing of CCs in microstraws preserved the largest number of viable cells with intact DNA compared with the methods of vitrification and slow freezing in microdroplets. Cryopreservation caused the upregulation of the genes Cx37 and Cx43 in the oocytes to restore gap junctions between cells. In conclusion, the presence of CCs in the co-culture system during IVM of oocytes played an important role in the regulation of the expression of the intercellular proteins Cx37 and Cx43, apoptotic changes, and oocyte methylation. Slow freezing in microstraws was considered to be an optimal method for cryopreservation of CCs. [ABSTRACT FROM AUTHOR]

Published

2024

18. Granulocyte Colony Stimulating Factor-Mobilized Peripheral Blood Mononuclear Cells: An Alternative Cellular Source for Chimeric Antigen Receptor Therapy.

Author

Ballesteros-Ribelles, Antonio, Millán-López, Alejandro, Carmona-Luque, MDolores, and Herrera, Concha

Subjects

*MONONUCLEAR leukocytes, *T cells, *GRANULOCYTE-colony stimulating factor, *CHIMERIC antigen receptors, *STEM cell transplantation, *T cell receptors, *LYMPHOCYTE count, *CRYOPROTECTIVE agents

Abstract

Lymphocyte collection by apheresis for CAR-T production usually does not include blood mobilized using granulocyte colony stimulating factor (G-CSF) due to the widespread knowledge that it causes a decrease in the number and functionality of lymphocytes. However, it is used for stem cell transplant, which is a common treatment for hematological malignancies. The growing demand for CAR therapies (CAR-T and NK-CAR), both in research and clinics, makes it necessary to evaluate whether mobilized PBSC products may be potential candidates for use in such therapies. This review collects recent works that experimentally verify the role and functionality of T and NK lymphocytes and the generation of CAR-T from apheresis after G-CSF mobilization. As discussed, T cells do not vary significantly in their phenotype, the ratio of CD4+ and CD8+ remains constant, and the different sub-populations remain stable. In addition, the expansion and proliferation rates are invariant regardless of mobilization with G-CSF as well as the secretion of proinflammatory cytokines and the cytotoxic ability. Therefore, cells mobilized before apheresis are postulated as a new alternative source of T cells for adoptive therapies that will serve to alleviate high demand, increase availability, and take advantage of the substantial number of existing cryopreserved products. [ABSTRACT FROM AUTHOR]

Published

2024

19. Advancements in Understanding and Enhancing Antioxidant-Mediated Sperm Cryopreservation in Small Ruminants: Challenges and Perspectives.

Author

Berean, Daniel Ionut, Bogdan, Liviu Marian, and Cimpean, Raluca

Subjects

CRYOPROTECTIVE agents, RUMINANTS, MESSENGER RNA, REPRODUCTIVE health, SPERMATOZOA, FLOW cytometry, MASS spectrometry, RNA metabolism

Abstract

Cryopreservation poses significant challenges to the preservation of sperm integrity and function, particularly in small ruminants where cryodamage is pronounced. This review explores the molecular mechanisms underlying sperm cryodamage and strategies for improving cryopreservation outcomes, with a focus on the role of antioxidants. Cryopreservation-induced alterations in proteins and RNA transcripts critical for sperm function, including motility, capacitation, fertilization, and embryo development, are discussed. Proteomic, transcriptomic, and epigenomic advancements have provided valuable insights into these mechanisms, offering potential biomarkers for predicting sperm freezability and enhancing cryopreservation strategies. Combining technologies such as mass spectrometry and flow cytometry allows for a comprehensive understanding of molecular and cellular changes induced by the freezing–thawing process. However, challenges remain in optimizing cryoprotectant formulations and antioxidant supplementation to improve post-thaw sperm fertility. Further research is needed to explore a wider range of novel cryoprotectants, antioxidants, and proteins for cryopreservation media, as well as to validate their efficacy in enhancing sperm viability and function. Additionally, investigations into the effects of cryopreservation on RNA transcripts and epigenetic factors in small ruminant species are warranted to advance our understanding of sperm preservation. Overall, this review highlights the importance of antioxidants in mitigating cryodamage and underscores the need for continued research to refine cryopreservation protocols and improve reproductive outcomes in small ruminants. [ABSTRACT FROM AUTHOR]

Published

2024

20. Astaxanthin Added during Post-Warm Recovery Mitigated Oxidative Stress in Bovine Vitrified Oocytes and Improved Quality of Resulting Blastocysts.

Author

Dujíčková, Linda, Olexiková, Lucia, Makarevich, Alexander V., Bartková, Alexandra Rosenbaum, Němcová, Lucie, Chrenek, Peter, and Strejček, František

Subjects

OVUM, ASTAXANTHIN, OXIDATIVE stress, BLASTOCYST, FROZEN semen, CRYOPROTECTIVE agents, SPERMATOZOA

Abstract

Various antioxidants are tested to improve the viability and development of cryopreserved oocytes, due to their known positive health effects. The aim of this study was to find whether astaxanthin (AX), a xanthophyll carotenoid, could mitigate deteriorations that occurred during the vitrification/warming process in bovine oocytes. Astaxanthin (2.5 µM) was added to the maturation medium during the post-warm recovery period of vitrified oocytes for 3 h. Afterward, the oocytes were fertilized in vitro using frozen bull semen and presumptive zygotes were cultured in the B2 Menezo medium in a co-culture with BRL-1 cells at 38.5 °C and 5% CO2 until the blastocyst stage. AX addition significantly reduced ROS formation, lipid peroxidation, and lysosomal activity, while increasing mitochondrial activity in vitrified oocytes. Although the effect of AX on embryo development was not observed, it stimulated cell proliferation in the blastocysts derived from vitrified oocytes and improved their quality by upregulation or downregulation of some genes related to apoptosis (BCL2, CAS9), oxidative stress (GPX4, CDX2), and development (GJB5) compared to the vitrified group without AX. Therefore, the antioxidant properties of astaxanthin even during short exposure to bovine vitrified/warmed oocytes resulted in improved blastocyst quality comparable to those from fresh oocytes. [ABSTRACT FROM AUTHOR]

Published

2024

21. The Cryoprotective Effect of an Antifreeze Collagen Peptide Complex Obtained by Enzymatic Glycosylation on Tilapia.

Author

Liu, Shouchun, Zhang, Luyao, Li, Zhuyi, Chen, Jing, Zhang, Yinyu, Yang, Xuebo, Chen, Qiuhan, Cai, Hongying, Hong, Pengzhi, Zhu, Chunhua, and Zhong, Saiyi

Subjects

PEPTIDES, ANTIFREEZE solutions, GLYCOSYLATION, MUSCLE proteins, TILAPIA, CRYOPROTECTIVE agents, TRANSGLUTAMINASES, COLLAGEN

Abstract

Antifreeze peptides have become effective antifreeze agents for frozen products, but their low quantity of active ingredients and high cost limit large-scale application. This study used the glycosylation of fish collagen peptides with glucosamine hydrochloride catalyzed by transglutaminase to obtain a transglutaminase-catalyzed glycosylation product (TGP) and investigate its antifreeze effect on tilapia. Compared with the blank group, the freshness (pH value of 6.31, TVB-N value of 21.7 mg/100 g, whiteness of 46.28), textural properties (especially hardness and elasticity), and rheological properties of the TGP groups were significantly improved. In addition, the protein structures of the samples were investigated using UV absorption and fluorescence spectroscopy. The results showed that the tertiary structure of the TGP groups changed to form a dense polymer. Therefore, this approach can reduce the denaturation and decomposition of muscle fibers and proteins in fish meat more effectively and has a better protective effect on muscle structure and protein aggregation, improving the stability of fish meat. This study reveals an innovative method for generating antifreeze peptides by enzymatic glycosylation, and glycosylated fish collagen peptide products can be used as new and effective green antifreeze agents in frozen foods. [ABSTRACT FROM AUTHOR]

Published

2024

22. Multiscale Thermal Technologies: Exploring Hot and Cold Potentials in Biomedical Applications.

Author

Yu, Bangrui and Huang, Haishui

Subjects

*SURFACE plasmon resonance, *MATERIALS science, *TREATMENT effectiveness, *BIOLOGICAL systems, *OVARIAN transplantation, *CRYOPROTECTIVE agents

Abstract

The editorial in the journal "Bioengineering (Basel)" discusses the advancements and challenges in utilizing thermal technology in biomedical applications, particularly in cryopreservation and thermal therapy. The document highlights innovative research on cryopreservation techniques, including the use of liquid helium and natural cryoprotectants like honey. It also explores the potential of thermal technology in cancer therapy and cardiovascular interventions, emphasizing the need for further research to optimize treatments and ensure long-term biocompatibility. The integration of biology, materials science, and thermodynamics is crucial for addressing current obstacles and unlocking the full therapeutic potential of thermal engineering in clinical settings. [Extracted from the article]

Published

2024

23. Ovotestis Isolation and Cryopreservation of Nesiohelix samarangae (Oriental Snail) as a Snail Model for Conserving Other Endangered Snail Species.

Author

Jeong, Jukyeong, Lee, Seungki, and Choi, Jung Kyu

Subjects

*ENDANGERED species, *GENITALIA, *WILDLIFE conservation, *GERMPLASM, *GERM cells, *CRYOPROTECTIVE agents, *SPERMATOZOA, *FROZEN semen, *GONADS

Abstract

Simple Summary: This study aimed to develop a cryopreservation system for Nesiohelix samarangae (oriental snail)'s reproductive organ to aid in species conservation. This snail possesses simultaneous hermaphroditism, meaning it has both male and female germ cells in its reproductive organs. Its reproductive glands are divided into acini, containing various stages of sperm development. Ovotestis cryopreservation using 2% alginate encapsulation showed superior viability compared to non-encapsulated methods. This system contributes to the genetic conservation and maintenance of genetic diversity within the species. This study aimed to develop a cryopreservation system for the reproductive organs of Nesiohelix samarangae (oriental snail) to support the conservation of their species. The reproductive glands of N. samarangae are divided into numerous acini by acinar boundaries. Within each acinus, the presence of spermatogonia, spermatocytes, spermatids, and sperm were observed, indicating various stages of sperm development. The spermatocytes were irregular in shape and possessed large nuclei. Spermatids, on the other hand, were predominantly located within the lumen of the tissue and exhibited densely packed nuclei. Furthermore, sperm with tails attached were observed within the tissue. In order to preserve the oriental snail species, we utilized the vitrification method to freeze the reproductive organs. Comparing the two methods, it was observed that cryopreservation of ovotestis using 2% alginate encapsulation exhibited superior viability following thawing, surpassing the viability achieved with the non-encapsulated approach. In this study, the establishment of a cryopreservation system for the reproductive organs of the oriental snail not only contributes to the genetic conservation of the endangered snail species but also plays a role in maintaining genetic resources and diversity. [ABSTRACT FROM AUTHOR]

Published

2024

24. DMSO and Its Role in Differentiation Impact Efficacy of Human Adenovirus (HAdV) Infection in HepaRG Cells.

Author

Hofmann, Katharina, Hofmann, Samuel, Weigl, Franziska, Mai, Julia, and Schreiner, Sabrina

Subjects

*DIMETHYL sulfoxide, *ADENOVIRUSES, *EXTRACELLULAR matrix, *CRYOPROTECTIVE agents, *VIRAL replication, *CELL culture, *INFECTION

Abstract

Differentiated HepaRG cells are popular in vitro cell models for hepatotoxicity studies. Their differentiation is usually supported by the addition of dimethyl sulfoxide (DMSO), an amphipathic solvent widely used in biomedicine, for example, in potential novel therapeutic drugs and cryopreservation of oocytes. Recent studies have demonstrated drastic effects, especially on epigenetics and extracellular matrix composition, induced by DMSO, making its postulated inert character doubtful. In this work, the influence of DMSO and DMSO-mediated modulation of differentiation on human adenovirus (HAdV) infection of HepaRG cells was investigated. We observed an increase in infectivity of HepaRG cells by HAdVs in the presence of 1% DMSO. However, this effect was dependent on the type of medium used for cell cultivation, as cells in William's E medium showed significantly stronger effects compared with those cultivated in DMEM. Using different DMSO concentrations, we proved that the impact of DMSO on infectability was dose-dependent. Infection of cells with a replication-deficient HAdV type demonstrated that the mode of action of DMSO was based on viral entry rather than on viral replication. Taken together, these results highlight the strong influence of the used cell-culture medium on the performed experiments as well as the impact of DMSO on infectivity of HepaRG cells by HAdVs. As this solvent is widely used in cell culture, those effects must be considered, especially in screening of new antiviral compounds. [ABSTRACT FROM AUTHOR]

Published

2024

25. Degradation of Poly(ethylene terephthalate) Catalyzed by Nonmetallic Dibasic Ionic Liquids under UV Radiation.

Author

Zhang, Ruiqi, Zheng, Xu, Cheng, Xiujie, Xu, Junli, Li, Yi, Zhou, Qing, Xin, Jiayu, Yan, Dongxia, and Lu, Xingmei

Subjects

*ULTRAVIOLET radiation, *IONIC liquids, *ETHYLENE glycol, *ETHYLENE, *CATALYTIC activity, *POLYETHYLENE terephthalate, *RADIATION exposure, *CRYOPROTECTIVE agents

Abstract

Nonmetallic ionic liquids (ILs) exhibit unique advantages in catalyzing poly (ethylene terephthalate) (PET) glycolysis, but usually require longer reaction times. We found that exposure to UV radiation can accelerate the glycolysis reaction and significantly reduce the reaction time. In this work, we synthesized five nonmetallic dibasic ILs, and their glycolysis catalytic activity was investigated. 1,8-diazabicyclo [5,4,0] undec-7-ene imidazole ([HDBU]Im) exhibited better catalytic performance. Meanwhile, UV radiation is used as a reinforcement method to improve the PET glycolysis efficiency. Under optimal conditions (5 g PET, 20 g ethylene glycol (EG), 0.25 g [HDBU]Im, 10,000 µW·cm−2 UV radiation reacted for 90 min at 185 °C), the PET conversion and BHET yield were 100% and 88.9%, respectively. Based on the UV-visible spectrum, it was found that UV radiation can activate the C=O in PET. Hence, the incorporation of UV radiation can considerably diminish the activation energy of the reaction, shortening the reaction time of PET degradation. Finally, a possible reaction mechanism of [HDBU]Im-catalyzed PET glycolysis under UV radiation was proposed. [ABSTRACT FROM AUTHOR]

Published

2024

26. Effect of Different Drying Methods on the Quality of Oudemansiella raphanipes.

Author

Hou, Shuting, Zhang, Defang, Yu, Dongmei, Li, Hao, Xu, Yaping, Wang, Wuxia, Li, Ruiting, Feng, Cuiping, Meng, Junlong, Xu, Lijing, Cheng, Yanfen, Chang, Mingchang, and Geng, Xueran

Subjects

DRYING, FREEZE-drying, POLYSACCHARIDES, SCANNING electron microscopy, GLUCURONIC acid, CRYOPROTECTIVE agents, INFRARED radiation

Abstract

In this study, we used fresh Oudemansiella raphanipes as raw materials and pre-treated through hot air drying (HD), infrared radiation drying (ID), and vacuum freeze drying (VD) to investigate the effects of different drying methods on the rehydration rate, appearance quality, microstructure, and volatile flavor components of the dried products, as well as to determine the physicochemical properties and bioactivities of the polysaccharides in the dried O. raphanipes. The results showed that the VD O. raphanipes had the highest rehydration rate and the least shrinkage in appearance, and it better maintained the original color of the gills, but their aroma was not as strong as that of the HD samples. The scanning electron microscopy results indicate that VD maintains a good porous structure in the tissue, while HD and ID exhibit varying degrees of shrinkage and collapse. Seventy-five common volatile substances were detected in the three dried samples, mainly alkanes, alcohols, and esters. The polysaccharides (PS-H, PS-I, and PS-V) extracted from the dried samples of these three species of O. raphanipes had similar infrared spectral features, indicating that their structures are basically consistent. The highest yield was obtained for PS-V, and the polysaccharide content and glucuronic acid content of PS-I were higher than those of the remaining two polysaccharides. In addition, PS-V also showed better antioxidant activity and inhibitory activity against α-glucosidase as well as α-amylase. In conclusion, among the above three drying methods, the quality of O. raphanipes obtained by vacuum freeze drying is the best, and this experiment provides a theoretical basis for the selection of drying methods for O. raphanipes. [ABSTRACT FROM AUTHOR]

Published

2024

27. The Dynamical Properties of Three Different Variants of the Orange Carotenoid Protein: A Quasielastic Neutron Scattering Study.

Author

Hajizadeh, Mina, Golub, Maksym, Moldenhauer, Marcus, Lohstroh, Wiebke, Friedrich, Thomas, and Pieper, Jörg

Subjects

QUASI-elastic scattering, NEUTRON scattering, PROTEINS, ICE nuclei, ELASTIC scattering, CRYOPROTECTIVE agents, SMALL-angle neutron scattering

Abstract

Besides a well-adapted structure, proteins often require a specific dynamical flexibility to undergo conformational changes in order to carry out their function. The latter dynamics can be directly measured by quasielastic neutron scattering as demonstrated here for three variants of the orange carotenoid protein (OCP), which plays a pivotal role in the protection of the cyanobacterial photosynthetic apparatus against photodamage. We investigate the dynamics of the structurally compact, dark-adapted wild type of OCP (OCPwt) in comparison with that of two mutant forms. The latter two mutants differ preferentially in their structures. The orange mutant OCP-W288A is assumed to have a compact structure and to preferentially bind the pigment echinenone, while the pink mutant OCP-W288A appears to represent the more elongated structure of the red active state of OCP binding the carotenoid canthaxanthin, respectively. The study reveals three major findings: (a) the dynamics of the red active state of OCP is significantly enhanced due to a larger number of protein residues being exposed to the solvent at the surface of the protein; (b) the dynamics of all OCP forms appear to be suppressed upon the freezing of the solvent, which is most likely due to an ice-induced aggregation of the proteins; and (c) the wild type and the compact mutant exhibit different dynamics attributed to a missing H-bond between the pigment and protein, resulting a destabilization of the surrounding protein. [ABSTRACT FROM AUTHOR]

Published

2024

28. Pros and Cons of Cryopreserving Allogeneic Stem Cell Products.

Author

Valentini, Caterina Giovanna, Pellegrino, Claudio, and Teofili, Luciana

Subjects

*STEM cells, *CRYOPRESERVATION of cells, *COVID-19 pandemic, *TREATMENT effectiveness, *HEMATOPOIETIC stem cells, *FROZEN human embryos, *CRYOPROTECTIVE agents, *FROZEN semen

Abstract

The COVID-19 pandemic has precipitously changed the practice of transplanting fresh allografts. The safety measures adopted during the pandemic prompted the near-universal graft cryopreservation. However, the influence of cryopreserving allogeneic grafts on long-term transplant outcomes has emerged only in the most recent literature. In this review, the basic principles of cell cryopreservation are revised and the effects of cryopreservation on the different graft components are carefully reexamined. Finally, a literature revision on studies comparing transplant outcomes in patients receiving cryopreserved and fresh grafts is illustrated. [ABSTRACT FROM AUTHOR]

Published

2024

29. Ovarian Tissue Cryopreservation versus Other Fertility Techniques for Chemoradiation-Induced Premature Ovarian Insufficiency in Women: A Systematic Review and Future Directions.

Author

Chaudhri, Eman N., Salman, Ayman, Awartani, Khalid, Khan, Zaraq, and Hashmi, Shahrukh K.

Subjects

*PREMATURE ovarian failure, *FERTILITY, *HUMAN fertility, *FERTILITY preservation, *CRYOPROTECTIVE agents, *EMBRYO implantation, *FROZEN human embryos, *INDUCED ovulation

Abstract

Current advances in cancer therapy have increased survival, emphasizing the need for life quality improvement. Fertility loss is common post-chemotherapy. Current guidelines establish embryo and oocyte cryopreservation to address premature ovarian insufficiency (POI). Ovarian tissue cryopreservation has also recently become an acceptable option for fertility preservation, particularly as it is the only option for pre-pubertal patients. Few definitions for optimum fertility outcomes, and few systematic reviews comparing embryo, oocyte, and ovarian tissue cryopreservation as a means of fertility preservation (FP) in pre- and post-pubertal female cancer patients exist. This systematic review aims to improve understanding of gonadotoxic effects of chemoradiation therapy in cancer patients, to analyze the different fertility preservation techniques and procedures available to women with chemoradiation induced ovarian insufficiency, and to compare and recognize the benefits of each technique in restoring fertility, sexual hormone function, and quality of life. Searches were conducted electronically on PubMed, Cochrane, and EBSCOHost, including clinical trials, prospective, and retrospective studies of female cancer patients undergoing anti-cancer therapy, with predefined MeSH terminology. Data were collected, analyzed, and compared. Non-randomized clinical studies were evaluated for risk bias through the Newcastle–Ottawa Scale. In total, 23 studies were included. From there, 647 patients opted for oocyte cryopreservation, 267 for embryo cryopreservation, and 1382 for ovarian tissue cryopreservation (OTC). A total of 175, 18, and 121 live births resulted respectively from oocyte, embryo, and OTC, respectively. Studies without live births discussed other fertility markers as indicators of improvement in sexual hormone function and fertility. The gonadotoxic effects of chemotherapy call for FP intervention. Oocyte and embryo cryopreservation/implantation are well-established procedures. With changing trends and life quality consideration, OTC is a promising interventional method for pre-pubertal patients facing the prospect of fertility loss. [ABSTRACT FROM AUTHOR]

Published

2024

30. Effects of Quality Enhancement of Frozen Tuna Fillets Using Ultrasound-Assisted Salting: Physicochemical Properties, Histology, and Proteomics.

Author

He, Yuke, Zhao, Zhou, Wu, Yaogang, Lu, Zhiyuan, Zhao, Caibo, Xiao, Juan, and Guo, Zhiqiang

Subjects

FISH fillets, FROZEN meat, YELLOWFIN tuna, FROZEN fish, TUNA, PROTEOMICS, CRYOPROTECTIVE agents

Abstract

Salting pretreatment is an effective method to improve the quality of frozen fish. This study investigated the quality changes and proteomic profile differences of frozen yellowfin tuna fillets pretreated with ultrasound-assisted salting (UAS) and static salting (SS). This study was centered on three aspects: physicochemical indicators' determination, histological observation, and proteomic analysis. The results showed that UAS significantly increased yield, salt content, and water-holding capacity (WHC), decreased total volatile base nitrogen (TVBN) compared to SS (p < 0.05), and significantly increased water in the protein matrix within myofibrils. Histological observations showed that the tissue cells in the UAS group were less affected by frozen damage, with a more swollen structure and rougher surface of myofibrils observed. Furthermore, 4D label-free proteomics revealed 56 differentially abundant proteins (DAPs) in UAS vs. NT comparison, mainly structural proteins, metabolic enzymes, proteasomes, and their subunits, which are associated with metabolic pathways such as calcium signaling pathway, gap junction, actin cytoskeletal regulation, and necroptosis, which are intimately associated with quality changes in freeze-stored tuna fillets. In brief, UAS enhances the potential for the application of salting pretreatment to improve frozen meat quality, and 4D label-free proteomics provides knowledge to reveal the potential links between quality and molecular changes in processed frozen meat to optimize future UAS meat processing. [ABSTRACT FROM AUTHOR]

Published

2024

31. Novel Apoplastic Antifreeze Proteins of Deschampsia antarctica as Enhancer of Common Cell Freezing Media for Cryobanking of Genetic Resources, a Preliminary Study.

Author

Short, Stefania E., Zamorano, Mauricio, Aranzaez-Ríos, Cristian, Lee-Estevez, Manuel, Díaz, Rommy, Quiñones, John, Ulloa-Rodríguez, Patricio, Villalobos, Elías Figueroa, Bravo, León A., Graether, Steffen P., and Farías, Jorge G.

Subjects

*ANTIFREEZE proteins, *CRYOPROTECTIVE agents, *ICE crystals, *CRYSTAL morphology, *FREEZING points, *ATLANTIC salmon, *SPERMATOZOA

Abstract

Highlights: Cryopreservation generates ice recrystallization. D. antarctica apoplastic proteins show antifreeze activity. PMI of S. salar sperm can be maintained with AFPs. High MMP of sperm increases with AFPs. D. antarctica apoplastic proteins act as nonpermeable cryoprotectants. Antifreeze proteins (AFPs) are natural biomolecules found in cold-adapted organisms that lower the freezing point of water, allowing survival in icy conditions. These proteins have the potential to improve cryopreservation techniques by enhancing the quality of genetic material postthaw. Deschampsia antarctica, a freezing-tolerant plant, possesses AFPs and is a promising candidate for cryopreservation applications. In this study, we investigated the cryoprotective properties of AFPs from D. antarctica extracts on Atlantic salmon spermatozoa. Apoplastic extracts were used to determine ice recrystallization inhibition (IRI), thermal hysteresis (TH) activities and ice crystal morphology. Spermatozoa were cryopreserved using a standard cryoprotectant medium (C+) and three alternative media supplemented with apoplastic extracts. Flow cytometry was employed to measure plasma membrane integrity (PMI) and mitochondrial membrane potential (MMP) postthaw. Results showed that a low concentration of AFPs (0.05 mg/mL) provided significant IRI activity. Apoplastic extracts from D. antarctica demonstrated a cryoprotective effect on salmon spermatozoa, with PMI comparable to the standard medium. Moreover, samples treated with apoplastic extracts exhibited a higher percentage of cells with high MMP. These findings represent the first and preliminary report that suggests that AFPs derived from apoplastic extracts of D. antarctica have the potential to serve as cryoprotectants and could allow the development of novel freezing media. [ABSTRACT FROM AUTHOR]

Published

2024

32. Ultra-Fast Vitrification: Minimizing the Toxicity of Cryoprotective Agents and Osmotic Stress in Mouse Oocyte Cryopreservation.

Author

Cho, Jung-Ran, Yu, Eun-Hee, Lee, Hyun-Joo, Kim, In-Hye, Jeong, Ji-Hye, Lee, Dan-Bi, Cho, Seong-Keun, and Joo, Jong-Kil

Subjects

*CRYOPROTECTIVE agents, *VITRIFICATION, *OVUM, *SPINDLE apparatus, *EMBRYOLOGY, *OSMOTIC pressure, *ENDOPLASMIC reticulum, *CHROMOSOMES, *SLEEP spindles

Abstract

Globally, women have been adopting oocyte cryopreservation (OC) for fertility preservation for various reasons, such as inevitable gonadotoxic treatment for specific pathologic states and social preferences. While conventional vitrification (C-VIT) has improved the success rate of OC, challenges of possible toxicities of high-concentration cryoprotective agents and osmotic stress persist. To overcome these challenges, we evaluated the ultra-fast vitrification (UF-VIT) method, which reduces the equilibration solution stage exposure time compared to C-VIT by observing mouse oocyte intracellular organelles and embryonic development. Consequently, compared to fresh mouse oocytes, UF-VIT presented significant differences only in endoplasmic reticulum (ER) intensity and mitochondrial (MT) distribution. Meanwhile, C-VIT showed substantial differences in the survival rate, key ER and MT parameters, and embryonic development rate. UF-VIT exhibited considerably fewer negative effects on key MT parameters and resulted in a notably higher blastocyst formation rate than C-VIT. Meiotic spindle (spindle and chromosomes) morphology showed no significant changes between the groups during vitrification/warming (VW), suggesting that VW did not negatively affect the meiotic spindle of the oocytes. In conclusion, UF-VIT seems more effective in OC owing to efficient cytoplasmic water molecule extraction, osmotic stress reduction, and minimization of cell contraction and expansion amplitude, thus compensating for the drawbacks of C-VIT. [ABSTRACT FROM AUTHOR]

Published

2024

33. Specifics of Cryopreservation of Hydrogel Biopolymer Scaffolds with Encapsulated Mesenchymal Stem Cells.

Author

Egorikhina, Marfa N., Rubtsova, Yulia P., Linkova, Daria D., Charykova, Irina N., Farafontova, Ekaterina A., and Aleinik, Diana Ya.

Subjects

*MESENCHYMAL stem cells, *BIOPOLYMERS, *HYDROGELS, *CRYOPROTECTIVE agents, *STEM cells, *REGENERATIVE medicine, *FROZEN semen, *SPERMATOZOA analysis

Abstract

The demand for regenerative medicine products is growing rapidly in clinical practice. Unfortunately, their use has certain limitations. One of these, which significantly constrains the widespread distribution and commercialization of such materials, is their short life span. For products containing suspensions of cells, this issue can be solved by using cryopreservation. However, this approach is rarely used for multicomponent tissue-engineered products due to the complexity of selecting appropriate cryopreservation protocols and the lack of established criteria for assessing the quality of such products once defrosted. Our research is aimed at developing a cryopreservation protocol for an original hydrogel scaffold with encapsulated MSCs and developing a set of criteria for assessing the quality of their functional activity in vitro. The scaffolds were frozen using two alternative types of cryocontainers and stored at either −40 °C or −80 °C. After cryopreservation, the external state of the scaffolds was evaluated in addition to recording the cell viability, visible changes during subsequent cultivation, and any alterations in proliferative and secretory activity. These observations were compared to those of scaffolds cultivated without cryopreservation. It was shown that cryopreservation at −80 °C in an appropriate type of cryocontainer was optimal for the hydrogels/adipose-derived stem cells (ASCs) tested if it provided a smooth temperature decrease during freezing over a period of at least three hours until the target values of the cryopreservation temperature regimen were reached. It was shown that evaluating a set of indicators, including the viability, the morphology, and the proliferative and secretory activity of the cells, enables the characterization of the quality of a tissue-engineered construct after its withdrawal from cryopreservation, as well as indicating the effectiveness of the cryopreservation protocol. [ABSTRACT FROM AUTHOR]

Published

2024

34. Influences of Supplementing Selective Members of the Interleukin-6 Cytokine Family on Bovine Oocyte Competency.

Author

McKinley, Endya, Speckhart, Savannah L., Keane, Jessica A., Oliver, Mary A., Rhoads, Michelle L., Edwards, J. Lannett, Biase, Fernando H., and Ealy, Alan D.

Subjects

*LEUKEMIA inhibitory factor, *OVUM, *CYTOKINES, *CRYOPROTECTIVE agents, *INTERLEUKIN-6, *RECOMBINANT proteins, *OVARIAN follicle

Abstract

Simple Summary: In vitro-produced (IVP) bovine embryos have reduced developmental potential and post-transfer survival. One reason this may occur is because of the lack of growth, differentiation factors, and cytokines that are present within the follicle but absent within oocyte maturation culture systems. This work explored whether supplementing selective members of the interleukin-6 (IL6) cytokine family during in vitro bovine oocyte maturation affects maturation success, cumulus–oocyte complex (COC) gene expression, fertilization success, and embryo development potential. Human recombinant proteins for IL6, IL11, and leukemia inhibitory factor (LIF) were supplemented to COCs during the maturation period, then fertilization and embryo culture commenced without further cytokine supplementation. Several key outcomes were observed. Both LIF and IL11 increased one COC transcript associated with oocyte competency whereas IL6 did not produce this effect. None of the cytokines influenced fertilization success but supplementing COCs with LIF or IL11 increased the ability of these oocytes to generate blastocyst stage embryos. No effect of IL6 supplementation was detected. Collectively, this work provides evidence that supplementing LIF or IL11 during in vitro oocyte maturation complexes improves oocyte competency, but no such effects were detected when IL6 was supplemented during maturation. This work explored whether supplementing selective members of the interleukin-6 (IL6) cytokine family during in vitro bovine oocyte maturation affects maturation success, cumulus–oocyte complex (COC) gene expression, fertilization success, and embryo development potential. Human recombinant proteins for IL6, IL11, and leukemia inhibitory factor (LIF) were supplemented to COCs during the maturation period, then fertilization and embryo culture commenced without further cytokine supplementation. The first study determined that none of these cytokines influenced the rate that oocytes achieved arrest at meiosis II. The second study identified that LIF and IL11 supplementation increases AREG transcript abundance. Supplementation with IL6 supplementation did not affect AREG abundance but reduced HAS2 transcript abundance. Several other transcriptional markers of oocyte competency were not affected by any of the cytokines. The third study determined that supplementing these cytokines during maturation did not influence fertilization success, but either LIF or IL11 supplementation increased blastocyst development. No effect of IL6 supplementation on subsequent blastocyst development was detected. The fourth experiment explored whether each cytokine treatment affects the post-thaw survivability of cryopreserved IVP blastocysts. None of the cytokines supplemented during oocyte maturation produced any positive effects on post-thaw blastocyst re-expansion and hatching. In conclusion, these outcomes implicate IL11 and LIF as potentially useful supplements for improving bovine oocyte competency. [ABSTRACT FROM AUTHOR]

Published

2024

35. Comparative Transcriptomic Analyses for the Optimization of Thawing Regimes during Conventional Cryopreservation of Mature and Immature Human Testicular Tissue.

Author

Pei, Cheng, Todorov, Plamen, Cao, Mengyang, Kong, Qingduo, Isachenko, Evgenia, Rahimi, Gohar, Mallmann-Gottschalk, Nina, Uribe, Pamela, Sanchez, Raul, and Isachenko, Volodimir

Subjects

*THAWING, *CRYOPROTECTIVE agents, *FROZEN human embryos, *GENE expression, *CRYOBIOLOGY, *RNA sequencing, *PROTEIN-protein interactions

Abstract

Cryopreservation of human testicular tissue, as a key element of anticancer therapy, includes the following stages: saturation with cryoprotectants, freezing, thawing, and removal of cryoprotectants. According to the point of view existing in "classical" cryobiology, the thawing mode is the most important consideration in the entire process of cryopreservation of any type of cells, including cells of testicular tissue. The existing postulate in cryobiology states that any frozen types of cells must be thawed as quickly as possible. The technologically maximum possible thawing temperature is 100 °C, which is used in our technology for the cryopreservation of testicular tissue. However, there are other points of view on the rate of cell thawing, according to how thawing should be carried out at physiological temperatures. In fact, there are morphological and functional differences between immature (from prepubertal patients) and mature testicular tissue. Accordingly, the question of the influence of thawing temperature on both types of tissues is relevant. The purpose of this study is to explore the transcriptomic differences of cryopreserved mature and immature testicular tissue subjected to different thawing methods by RNA sequencing. Collected and frozen testicular tissue samples were divided into four groups: quickly (in boiling water at 100 °C) thawed cryopreserved mature testicular tissue (group 1), slowly (by a physiological temperature of 37 °C) thawed mature testicular tissue (group 2), quickly thawed immature testicular tissue (group 3), and slowly thawed immature testicular tissue (group 4). Transcriptomic differences were assessed using differentially expressed genes (DEG), the Kyoto Encyclopedia of Genes and Genomes (KEGG), gene ontology (GO), and protein–protein interaction (PPI) analyses. No fundamental differences in the quality of cells of mature and immature testicular tissue after cryopreservation were found. Generally, thawing of mature and immature testicular tissue was more effective at 100 °C. The greatest difference in the intensity of gene expression was observed in ribosomes of cells thawed at 100 °C in comparison with cells thawed at 37 °C. In conclusion, an elevated speed of thawing is beneficial for frozen testicular tissue. [ABSTRACT FROM AUTHOR]

Published

2024

36. Kaempferol Enhances Sperm Post-Thaw Survival by Its Cryoprotective and Antioxidant Behavior.

Author

Baňas, Štefan, Benko, Filip, Ďuračka, Michal, Lukáč, Norbert, and Tvrdá, Eva

Subjects

*FLAVONOLS, *CRYOPROTECTIVE agents, *ANTIOXIDANTS, *SPERM motility, *PROTEIN expression

Abstract

This study examined the effects of three selected doses of kaempferol (KAE; 12.5, 25 or 50 μM) on bovine sperm motility and oxidative profile directly related to cold storage. We also elucidated the effect of KAE on the expression profiles of heat shock proteins (HSPs) 70 and 90 as well as the pro-apoptotic BCL2-associated X (BAX) protein and the anti-apoptotic B-cell lymphoma 2 (Bcl-2) protein. Frozen samples supplemented with KAE were compared with a native control (fresh spermatozoa) and a cryopreserved control, frozen in the absence of KAE. Our results demonstrate that the administration of all KAE doses led to a higher degree of sperm motility (p < 0.05) when compared with the cryopreserved control. The highest levels of protection of sperm DNA (p < 0.05), lipids (p < 0.05) and proteins (p < 0.05) were detected in samples exposed to 25 μM KAE when compared with samples frozen without KAE. Administration of 25 μM KAE led to a significant increase in HSP70 and HSP90 (p < 0.05) when compared with the unsupplemented frozen control. No significant differences were observed in the expression patterns of BAX; however, a significant up-regulation of Bcl-2 protein was observed in the frozen samples enriched with 25 μM KAE when compared with the cryopreserved control (p < 0.05). In summary, we may consider KAE as an effective agent in stabilizing the sperm membranes by preventing reactive oxygen species (ROS) overproduction in the mitochondria and subsequent oxidative damage to molecules critical for a proper sperm architecture and function. These protective properties of KAE may lead to higher post-thaw sperm activity and viability. [ABSTRACT FROM AUTHOR]

Published

2023

37. Successful Cryopreservation of Spermatogonia Stem Cells of Neotropical Catfish (Rhamdia quelen) and Enriched Germ Cell Transplantation into Common Carp (Cyprinus carpio) Testes.

Author

Rosa, Ivana F., Martinez, Emanuel R. M., Digmayer, Melanie, Doretto, Lucas B., and Nóbrega, Rafael H.

Subjects

*GONADS, *CARP, *GERM cells, *STEM cells, *CELL transplantation, *FROZEN semen, *SERTOLI cells, *CRYOPROTECTIVE agents

Abstract

Cryopreservation and transplantation of spermatogonial stem cells (SSCs) offer new possibilities in the conservation of valuable genetic resources. Therefore, the present study developed a cryopreservation method for whole testicular tissue and for spermatogonial stem cells of jundia catfish (Rhamdia quelen) and developed an enriched germ cell transplantation of jundia catfish into depleted common carp (Cyprinus carpio) testes. Our findings from whole testes indicate that the cryoprotectants MeOH (1.3 M), DMSO (1.4 M), and EG (1.4 M) resulted in high cell viability rates of 67%, 62%, and 51.5%, respectively. Notably, in the case of enriched post-thaw SSCs, DMSO exhibited the highest cell viability at 27%, followed by EG at 16% and MeOH at 7%. Additionally, we observed the successful colonization and proliferation of jundia germ cells within the recipient gonads of common carp following transplantation. Notably, Sertoli cells were identified in the recipient gonads, providing support to the stained donor germ cells and indicated the formation of cysts. Our data suggest that cryopreserving entire testicular tissue presents a viable alternative to cryopreserving isolated testicular cells, and the spermatogonial cells isolated from testes of jundia retained transplantability characteristics. Nonetheless, more investigations are required to reach the goal of functional gamete and to assess the effectiveness of transplantation using these cryopreserved tissues. Taken together, proper cryopreservation methodology and transplantation technology could aid the preservation practice of fish genetic resources. [ABSTRACT FROM AUTHOR]

Published

2023

38. Characterization of Rabbit Mesenchymal Stem/Stromal Cells after Cryopreservation.

Author

Koung Ngeun, Sai, Shimizu, Miki, and Kaneda, Masahiro

Subjects

*CRYOPRESERVATION of cells, *STROMAL cells, *MESENCHYMAL stem cells, *ADIPOSE tissues, *CELL physiology, *CRYOPROTECTIVE agents, *ADIPOGENESIS

Abstract

Simple Summary: Mesenchymal stem cells (MSCs) are prime candidates for cell-based therapies and regenerative medicine due to their trilineage differentiation potential. MSCs can differentiate into osteocytes, adipocytes, and chondrocytes. A significant number of these cells must be available for clinical application. As a result, cryopreservation becomes essential to ensure the cells are readily available and can be stored long term. However, there is a gap in our knowledge concerning the characteristics, sustainability of multipotency, and biosafety of cryopreserved MSCs in rabbits. Additionally, the functional ability of MSCs varies based on their source, which could influence their cryopreservation response. Differences in morphology, differentiation potential, and resilience to cryopreservation might also exist among various animal models and humans. To learn more, we assessed MSCs' characteristics and functional properties from rabbits before and after cryopreservation. These cells were sourced from adipose tissues and bone marrow. Our findings suggest that while bone marrow-derived MSCs retain their functional ability poorly, adipose-derived cells retain their functionality better. Adipose tissues (ADPs) are an alternative source for mesenchymal stem/stromal cells (MSCs), given that conventional bone marrow (BM) collection is painful and yields limited cell numbers. As the need for easily accessible MSCs grows, cryopreservation's role in regenerative medicine is becoming increasingly vital. However, limited research exists on the characteristics and functional properties of rabbit-derived MSCs from various anatomical sources before and after cryopreservation. We examined the effects of cryopreservation using Bambanker. We found that cryopreservation did not adversely affect the morphology, viability, and adipogenic or chondrogenic differentiation abilities of ADP MSCs or BM MSCs. However, there was a notable drop in the proliferation rate and osteogenic differentiation capability of BM MSCs post-cryopreservation. Additionally, after cryopreservation, the surface marker gene expression of CD90 was not evident in ADP MSCs. As for markers, ADIPOQ can serve as an adipogenic marker for ADP MSCs. ACAN and CNMD can act as chondrogenic markers, but these two markers are not as effective post-cryopreservation on ADP MSCs, and osteogenic markers could not be validated. The study highlights that compared to BM MSCs, ADP MSCs retained a higher viability, proliferation rate, and differentiation potential after cryopreservation. As such, in clinical MSC use, we must consider changes in post-cryopreservation cell functions. [ABSTRACT FROM AUTHOR]

Published

2023

39. Cryopreservation Cooling Rate Impacts Post-Thaw Sperm Motility and Survival in Litoria booroolongensis.

Author

Hobbs, Rebecca J., Upton, Rose, Calatayud, Natalie E., Silla, Aimee J., Daly, Jonathan, McFadden, Michael S., and O'Brien, Justine K.

Subjects

*FROZEN semen, *CRYOPROTECTIVE agents, *SPERMATOZOA, *SPERM motility, *REPRODUCTIVE technology, *SPERM banks, *COOLING, *DIMETHYL sulfoxide

Abstract

Simple Summary: The development of reproductive technologies for amphibian species has accelerated over the last decade to the point that the industry implementation of these methodologies to assist breeding and genetic management is underway globally. A conservation breeding program was established at Taronga Conservation Society (Australia) in 2019 for the critically endangered Booroolong frog (Litoria booroolongensis) following an emergency extraction from the wild. Shortly thereafter, a trial was undertaken to compare the efficacy of two sperm cryopreservation protocols with a view to creating a "sperm bank" from these genetically important founder individuals. Spermic urine samples from L. booroolongensis were successfully cryopreserved using both methods tested; however, higher numbers of sperm retained motility post-thaw when using a faster cooling method for cryopreservation. Moreover, the two cryoprotectants tested were equally effective at supporting sperm survival and function post-thaw, regardless of cooling speed. We utilized the method outlined in this paper to collect and cryopreserve spermic urine samples across three breeding seasons from all (n = 28) L. booroolongensis founder males at Taronga and are now investigating the use of these samples to create offspring via assisted fertilization. The cryopreservation and storage of gametes (biobanking) can provide a long-term, low-cost option for the preservation of population genetic diversity and is particularly impactful when applied to manage selective breeding within conservation breeding programs (CBPs). This study aimed to develop a sperm cryopreservation protocol for the critically endangered Booroolong frog (Litoria booroolongensis) to capture founder genetics within the recently established (est. 2019) CBP for this species. Hormone-induced sperm release was achieved using established protocols, and spermic urine samples were collected over a 6-h period. Pooled spermic urine samples (n = 3 males) were divided equally between two cryoprotectant (CPA) treatments and diluted by 1:5 (sperm:CPA) with either 15% (v/v) dimethyl sulfoxide + 1% (w/v) sucrose in simplified amphibian Ringer's (SAR; CPAA) or 10% (v/v) dimethylformamide + 10% (w/v) trehalose dihydrate in SAR (CPAB). The samples were cryopreserved in 0.25 mL straws using either a programmable freezer (FrA) or an adapted dry shipper method (FrB). The thawed samples were activated via dilution in water and assessed for viability and motility using both manual assessment and computer-assisted sperm analysis (CASA; 0 h, 0.5 h post-thaw). Upon activation, the survival and recovery of motility (total motility, forward progression and velocity) of cryopreserved sperm suspensions were higher for sperm preserved using FrB than FrA, regardless of CPA composition. This work supports our long-term goal to pioneer the integration of biobanked cryopreserved sperm with population genetic management to maximize restoration program outcomes for Australian amphibian species. [ABSTRACT FROM AUTHOR]

Published

2023

40. Generation of Human Regulatory Dendritic Cells from Cryopreserved Healthy Donor Cells and Hematopoietic Stem Cell Transplant Recipients.

Author

Scroggins, Sabrina M. and Schlueter, Annette J.

Subjects

*HEMATOPOIETIC stem cells, *STEM cell transplantation, *GRAFT versus host disease, *STEM cell donors, *MONOCYTES, *DENDRITIC cells, *HLA histocompatibility antigens, *CRYOPROTECTIVE agents

Abstract

Acute graft versus host disease (GVHD) remains a significant complication following hematopoietic stem cell transplant (HSCT), despite improved human leukocyte antigen (HLA) matching and advances in prophylactic treatment regimens. Previous studies have shown promising results for future regulatory dendritic cell (DCreg) therapies in the amelioration of GVHD. This study evaluates the effects of cryopreservation on the generation of DCreg, the generation of young and older DCreg in serum-free media, and the feasibility of generating DCreg from young and older HSCT patient monocytes. DCregs were generated in X-vivo 15 serum-free media from donor or patient monocytes. This study includes the use of monocytes from young and older healthy, donor, and HSCT patients with varying hematological diseases. Phenotypic differences in cell populations were assessed via flow cytometry while pro-inflammatory and anti-inflammatory cytokine production was evaluated in culture medium. The number of DCreg generated from cryopreserved monocytes of healthy donors was not significantly different from freshly isolated monocytes. DCreg generated from cryopreserved monocytes had comparable levels of co-stimulatory molecule expression, inhibitory molecule expression, and cytokine production as freshly isolated monocytes. Young and older healthy donor monocytes generated similar numbers of DCreg with similar cytokine production and phenotype. Although monocytes from older HSCT patients generated significantly fewer DCreg, DCreg from young and older HSCT patients had comparable phenotypes and cytokine production. Monocytes from young and older myelodysplastic syndrome (MDS) patients generated reduced numbers of DCreg compared to non-MDS-derived DCreg. We demonstrate that the cryopreservation of monocytes from HSCT patients of varying hematological diseases allows for the cost-effective generation of DCreg on an as-needed basis. Although the generation of DCreg from MDS patients requires further assessment, these data support the possibility of in vitro-generated DCreg as a therapy to reduce GVHD-associated morbidity and mortality in young and older HSCT recipients. [ABSTRACT FROM AUTHOR]

Published

2023

41. Dynamics of Organic Acids during the Droplet-Vitrification Cryopreservation Procedure Can Be a Signature of Oxidative Stress in Pogostemon yatabeanus.

Author

Lee, Hyoeun, Choi, Byeongchan, Oh, Songjin, Park, Hana, Popova, Elena, Paik, Man-Jeong, and Kim, Haenghoon

Subjects

OXIDATIVE stress, ENDANGERED plants, CRYOPRESERVATION of cells, CELL metabolism, GROUP dynamics, CRYOPROTECTIVE agents, GLYCOLIC acid, ORGANIC acids, PLANT shoots

Abstract

Cryopreservation in liquid nitrogen (LN, −196 °C) is a unique option for the long-term conservation of threatened plant species with non-orthodox or limitedly available seeds. In previous studies, a systematic approach was used to develop a droplet-vitrification (DV) cryopreservation protocol for Postemon yatabeanus shoot tips that includes preculture with 10% sucrose, osmoprotection with C4-35%, cryoprotection with A3-80% vitrification solution, and a three-step regrowth starting with the ammonium-free medium. The tricarboxylic acid (TCA) cycle is a crucial component of plant cell metabolism as it is involved in redox state regulation and energy provision. We hypothesized that organic acids (OAs) associated with the TCA and its side reactions indirectly indicate metabolism intensity and oxidative stress development in shoot tips under the cryopreservation procedure. In this study, the contents of 14 OAs were analyzed using gas chromatography–tandem mass spectrometry (GC-MS/MS) in P. yatabeanus shoot tips in a series of treatments including individual steps of the DV procedure, additional stress imposed by non-optimum protocol conditions (no preculture, no osmoprotection, various vitrification solution composition, using vials instead of aluminum foils, etc.) and regrowth on different media with or without ammonium or growth regulators. The possible relation of OA content with the total cryoprotectant (CPA) concentration and shoot tips regeneration percentage was also explored. Regeneration of cryopreserved shoot tips reduced in descending order as follows: standard protocol condition (91%) > non-optimum vitrification solution (ca. 68%) > non-optimum preculture (60–62%) > regrowth medium (40–64%) > no osmoprotection, cryopreservation in vials (28–30%). Five OAs (glycolic, malic, citric, malonic, and lactic) were the most abundant in the fresh (control) shoot tips. The dynamic pattern of OAs during the DV procedure highly correlated (r = 0.951) with the total CPA concentration employed: it gradually increased through the preculture, osmoprotection, and cryoprotection, peaked at cooling/rewarming (6.38-fold above control level), and returned to the fresh control level after 5 days of regrowth (0.89-fold). The contents of four OAs (2-hydroxybutyric, 3-hydroxypropionic, lactic, and glycolic) showed the most significant (10-209-fold) increase at the cooling/rewarming step. Lactic and glycolic acids were the major OAs at cooling/rewarming, accounting for 81% of the total OAs content. The OAs were categorized into three groups based on their dynamics during the cryopreservation protocol, and these groups were differently affected by protocol step modifications. However, there was no straightforward relationship between the dynamics of OAs and shoot tip regeneration. The results suggest that active modulation of OAs metabolism may help shoot tips to cope with osmotic stress and the chemical cytotoxicity\ of CPAs. Further intensive studies are needed to investigate the effect of cryopreservation on cell primarily metabolism and identify oxidative stress-related biomarkers in plant materials. [ABSTRACT FROM AUTHOR]

Published

2023

42. Effect of Different Vitrification Techniques on Viability and Apoptotic Index of Domestic Cat Testicular Tissue Cells.

Author

Carvalho, Julyne Vivian Guimarães de, Soares, Airton R. B., Leão, Danuza L., Reis, Adriana N., Santos, Regiane R., Rodrigues, Ana P. R., and Domingues, Sheyla F. S.

Subjects

*CATS, *VITRIFICATION, *FELIDAE, *SERTOLI cells, *FROZEN semen, *CELL nuclei, *CRYOPROTECTIVE agents

Abstract

Simple Summary: The vitrification process stands out among cryopreservation methods because it is a practical and fast technique that reduces the risk of intracellular ice formation and cell damage. The present study aimed to compare three devices used for the vitrification of adult cat testicular biopsies for use in preservation programs. The efficiency of the methods was evaluated by histological and viability analysis of the testicular cells after the vitrification process. It is shown that these methods are efficient and can be considered an important tool for the genetic conservation of endangered wild cats, with the domestic cat providing an experimental model for the development of reproductive biotechnology in wild cat species. Vitrification is essential for successful tissue cryopreservation and biobanking in wild cats. This study aimed to compare different methods of vitrification (Ovarian Tissue Cryosystem—OTC, Straws—STW, and Solid Surface vitrification—SSV) for testicular fragment vitrification in tom cats. Testicular fragments were recovered from five adult tom cats and subjected to equilibrium vitrification using different cryovials and methods under the same conditions of vitrification solutions and cryoprotectants. The efficiencies of the methods were evaluated using histological analysis of spermatogonia and Sertoli cell nuclei, seminiferous tubular basement membrane detachment, and the gonadal epithelium shrinkage score scale. Cell viability was assessed using Hoechst PI and Terminal deoxynucleotidyl transferase nick end labeling (TUNEL) assay. The results showed that OTC is an effective vitrification method for maintaining the distinction between spermatogonia and Sertoli cells. OTC was similar to the control for basal membrane detachment parameters (p = 0.05). Epithelial shrinkage was low in the SSV group, which showed the highest percentage of viable cells among the vitrified groups (p = 0.0023). The OTC and SSV vitrification methods were statistically similar in terms of the percentage of TUNEL-positive cells (p = 0.05). Therefore, OTC and SSV provide favorable conditions for maintaining viable cat testicular tissue cells after vitrification. [ABSTRACT FROM AUTHOR]

Published

2023

43. Development of Cryopreservation Technique for Meristems of Syringa vulgaris L. Cultivars.

Author

Koroleva, Olga Vasilevna, Molkanova, Olga Ivanovna, and Vysotskaya, Olga Nikolaevna

Subjects

*MERISTEMS, *PLANT germplasm, *CULTIVARS, *CRYOPROTECTIVE agents, *THIDIAZURON, *PLANT tissue culture, *PACLOBUTRAZOL

Abstract

Cryopreservation is considered to be one of the most effective methods for long-term storage of plant genetic resources, particularly for ornamental species. However, there is a very little research on cryopreservation of lilacs. In this study, for the first time the cryopreservation protocol (a variation of a pregrowth-dehydration method) was successfully applied to two cultivars of Syringa vulgaris: 'Aucubaefolia' and 'Polina Osipenko'. Explants of both cultivars were able to withstand the different steps of the protocol, and high survival and regrowth percentages were obtained after exposure to liquid nitrogen (67-100% and 63-88%, respectively). The current study is mainly focused on the preculture conditions of the applied method. Based on our results, we propose the use of paclobutrazol (PBZ) with the combination of 6-benzylaminopurine (BAP) and thidiazuron (TDZ) in the preculture medium for increasing explant tolerance to subsequent dehydration and freezing. During post-LN recovery, the explants appeared morphologically normal, and after 12-16 weeks after thawing, they were propagated and cultured as normal plantlets. Therefore, the reported method is effective for long-term storage of lilac meristems and could be used to create a cryobank of achievements in lilac breeding. [ABSTRACT FROM AUTHOR]

Published

2023

44. Cryopreserved Platelets in a Non-Toxic DMSO-Free Solution Maintain Hemostatic Function In Vitro.

Author

Ehn, Kristina, Wikman, Agneta, Uhlin, Michael, and Sandgren, Per

Subjects

*CRYOPROTECTIVE agents, *BLOOD volume, *PLASMA products, *DIMETHYL sulfoxide, *FROZEN semen, *CELL analysis, *BLOOD platelets

Abstract

Dimethyl sulfoxide (DMSO) is regularly used as a cryoprotectant agent for the cryopreservation of platelets. However, DMSO is considered toxic. We therefore hypothesized that saline could be used as a non-toxic medium for the cryopreservation of platelets. Double-dose buffy coat platelets (n = 10) were divided and cryopreserved at −80 °C using 5–6% dimethyl sulfoxide (DMSO) or in NaCl (9 mg/mL). Paired testing was conducted pre-freeze, post-thaw (PT 1 h). Upon analysis, each bag was thawed and reconstituted in fresh plasma. Analyses included cell counts and the metabolic, phenotypic, and functional properties of the platelets together with thromboelastometry. The cryopreserved platelets showed several biochemical and ultrastructural changes compared to pre-freezing. Platelet recovery was approximately 17% higher in DMSO-free units (p < 0.001), but the platelet viability was reduced (p < 0.001). However, using controlled freezing (n = 6), the platelet viability was improved. The clot formation time (CFT) was comparable, but DMSO-free platelets showed slightly decreased maximum clot firmness (MCF) (p = 0.034). By reducing the reconstituted plasma volume, a reduced CFT and increased MCF were obtained (p < 0.001). This study demonstrates that platelets can be cryopreserved in saline without the addition of DMSO, with high recovery and maintained hemostatic function. However, controlled freezing is required to optimize platelet quality. [ABSTRACT FROM AUTHOR]

Published

2023

45. Improved Method for Dental Pulp Stem Cell Preservation and Its Underlying Cell Biological Mechanism.

Author

Takeshita-Umehara, Mai, Tokuyama-Toda, Reiko, Takebe, Yusuke, Terada-Ito, Chika, Tadokoro, Susumu, Inoue, Akemi, Ijichi, Kohei, Yudo, Toshio, and Satomura, Kazuhito

Subjects

*DENTAL pulp, *CELL preservation, *STEM cells, *CELL migration, *REGENERATIVE medicine, *CELL culture, *FROZEN semen, *CRYOPROTECTIVE agents

Abstract

Dental pulp stem cells (DPSCs) are considered a valuable cell source for regenerative medicine because of their high proliferative potential, multipotency, and availability. We established a new cryopreservation method (NCM) for collecting DPSCs, in which the tissue itself is cryopreserved and DPSCs are collected after thawing. We improved the NCM and developed a new method for collecting and preserving DPSCs more efficiently. Dental pulp tissue was collected from an extracted tooth, divided into two pieces, sandwiched from above and below using cell culture inserts, and cultured. As a result, the cells in the pulp tissue migrated vertically over time and localized near the upper and lower membranes over 2–3 days. With regard to the underlying molecular mechanism, SDF1 was predominantly involved in cell migration. This improved method is valuable and enables the more efficient collection and reliable preservation of DPSCs. It has the potential to procure a large number of DPSCs stably. [ABSTRACT FROM AUTHOR]

Published

2023

46. Preparation and Characterization of Novel Green Seaweed Films from Ulva rigida.

Author

Sonchaeng, Uruchaya, Wongphan, Phanwipa, Pan-utai, Wanida, Paopun, Yupadee, Kansandee, Wiratchanee, Satmalee, Prajongwate, Tamtin, Montakan, Kosawatpat, Prapat, and Harnkarnsujarit, Nathdanai

Subjects

*ULVA, *HIGH performance liquid chromatography, *GLASS transition temperature, *NUCLEAR magnetic resonance, *MARINE algae, *CRYOPROTECTIVE agents, *GLYCINE receptors, *GLYCERIN

Abstract

Ulva rigida green seaweed is an abundant biomass consisting of polysaccharides and protein mixtures and a potential bioresource for bioplastic food packaging. This research prepared and characterized novel biodegradable films from Ulva rigida extracts. The water-soluble fraction of Ulva rigida was extracted and prepared into bioplastic films. 1H nuclear magnetic resonance indicated the presence of rhamnose, glucuronic and sulfate polysaccharides, while major amino acid components determined via high-performance liquid chromatography (HPLC) were aspartic acid, glutamic acid, alanine and glycine. Seaweed extracts were formulated with glycerol and triethyl citrate (20% and 30%) and prepared into films. Ulva rigida films showed non-homogeneous microstructures, as determined via scanning electron microscopy, due to immiscible crystalline component mixtures. X-ray diffraction also indicated modified crystalline morphology due to different plasticizers, while infrared spectra suggested interaction between plasticizers and Ulva rigida polymers via hydrogen bonding. The addition of glycerol decreased the glass transition temperature of the films from −36 °C for control films to −62 °C for films with 30% glycerol, indicating better plasticization. Water vapor and oxygen permeability were retained at up to 20% plasticizer content, and further addition of plasticizers increased the water permeability up to 6.5 g·mm/m2·day·KPa, while oxygen permeability decreased below 20 mL·mm/m2·day·atm when blending plasticizers at 30%. Adding glycerol efficiently improved tensile stress and strain by up to 4- and 3-fold, respectively. Glycerol-plasticized Ulva rigida extract films were produced as novel bio-based materials that supported sustainable food packaging. [ABSTRACT FROM AUTHOR]

Published

2023

47. Investigation of the Mitigation of DMSO-Induced Cytotoxicity by Hyaluronic Acid following Cryopreservation of Human Nucleus Pulposus Cells.

Author

Munesada, Daiki, Sakai, Daisuke, Nakamura, Yoshihiko, Schol, Jordy, Matsushita, Erika, Tamagawa, Shota, Sako, Kosuke, Ogasawara, Shota, Sato, Masato, and Watanabe, Masahiko

Subjects

*NUCLEUS pulposus, *HYALURONIC acid, *INTERVERTEBRAL disk, *REACTIVE oxygen species, *PROGENITOR cells, *DIMETHYL sulfoxide, *CRYOPROTECTIVE agents

Abstract

To develop an off-the-shelf therapeutic product for intervertebral disc (IVD) repair using nucleus pulposus cells (NPCs), it is beneficial to mitigate dimethyl sulfoxide (DMSO)-induced cytotoxicity caused by intracellular reactive oxygen species (ROS). Hyaluronic acid (HA) has been shown to protect chondrocytes against ROS. Therefore, we examined the potential of HA on mitigating DMSO-induced cytotoxicity for the enhancement of NPC therapy. Human NPC cryopreserved in DMSO solutions were thawed, mixed with equal amounts of EDTA-PBS (Group E) or HA (Group H), and incubated for 3–5 h. After incubation, DMSO was removed, and the cells were cultured for 5 days. Thereafter, we examined cell viability, cell proliferation rates, Tie2 positivity (a marker of NP progenitor cells), and the estimated numbers of Tie2 positive cells. Fluorescence intensity of DHE and MitoSOX staining, as indicators for oxidative stress, were evaluated by flow cytometry. Group H showed higher rates of cell proliferation and Tie2 expressing cells with a trend toward suppression of oxidative stress compared to Group E. Thus, HA treatment appears to suppress ROS induced by DMSO. These results highlight the ability of HA to maintain NPC functionalities, suggesting that mixing HA at the time of transplantation may be useful in the development of off-the-shelf NPC products. [ABSTRACT FROM AUTHOR]

Published

2023

48. Different Impacts of Cryopreservation in Endothelial and Epithelial Ovarian Cells.

Author

Marschalek, Julian, Hager, Marlene, Wanderer, Sophie, Ott, Johannes, Frank, Maria, Schneeberger, Christian, and Pietrowski, Detlef

Subjects

*EPITHELIAL cells, *GRANULOSA cells, *CELL death, *CELL lines, *ENDOTHELIAL cells, *CRYOPROTECTIVE agents, *FROZEN semen

Abstract

The aim of our laboratory-based study was to investigate the extent of delayed-onset cell death after cryopreservation in endothelial and epithelial cell lines of ovarian origin. We found differences in percentages of vital cells directly after warming and after cultivation for 48 to 72 h. A granulosa cell line of endothelial origin (KGN) and an epithelial cell line (OvCar-3) were used. In both DMSO-containing and DMSO-free protocols, significant differences in vitality rates between the different cell lines when using open and closed vitrification could be shown (DMSO-containing: KGN open vs. OvCar open, p = 0.001; KGN closed vs. OvCar closed, p = 0.001; DMSO-free: KGN open vs. OvCar open, p = 0.001; KGN closed vs. OvCar closed, p = 0.031). Furthermore, there was a marked difference in the percentage of vital cells immediately after warming and after cultivation for 48 to 72 h; whereas the KGN cell line showed a loss of cell viability of 41% using a DMSO-containing protocol, the OvCar-3 cell loss was only 11% after cultivation. Using a DMSO-free protocol, the percentages of late-onset cell death were 77% and 48% for KGN and OvCar-3 cells, respectively. Our data support the hypothesis that cryopreservation-induced damage is cell type and cryoprotective agent dependent. [ABSTRACT FROM AUTHOR]

Published

2023

49. The mTOR Inhibitor Rapamycin Counteracts Follicle Activation Induced by Ovarian Cryopreservation in Murine Transplantation Models.

Author

Bindels, Jules, Squatrito, Marlyne, Bernet, Laëtitia, Nisolle, Michelle, Henry, Laurie, and Munaut, Carine

Subjects

MTOR inhibitors, CRYOPROTECTIVE agents, RAPAMYCIN, KIDNEY transplantation, FERTILITY preservation, LABORATORY mice, OVARIES

Abstract

Background and Objectives: Ovarian tissue cryopreservation followed by autotransplantation (OTCTP) is currently the only fertility preservation option for prepubertal patients. Once in remission, the autotransplantation of frozen/thawed tissue is performed when patients want to conceive. A major issue of the procedure is follicular loss directly after grafting mainly due to follicle activation. To improve follicular survival during the OTCTP procedure, we inhibited the mTOR pathway involved in follicle activation using rapamycin, an mTOR inhibitor. Next, we compared two different in vivo models of transplantation: the recently described non-invasive heterotopic transplantation model between the skin layers of the ears, and the more conventional and invasive transplantation under the kidney capsule. Materials and Methods: To study the effects of adding rapamycin during cryopreservation, 4-week-old C57BL/6 mouse ovaries, either fresh, slow-frozen, or slow-frozen with rapamycin, were autotransplanted under the kidney capsule of mice and recovered three weeks later for immunohistochemical (IHC) analysis. To compare the ear with the kidney capsule transplantation model, fresh 4-week-old C57BL/6 mouse ovaries were autotransplanted to either site, followed by an injection of either LY294002, a PI3K inhibitor, vehicle control, or neither, and these were recovered three weeks later for IHC analysis. Results: Rapamycin counteracts cryopreservation-induced follicle proliferation, as well as AKT and mTOR pathway activation, in ovaries autotransplanted for three weeks under the kidney capsule of mice. Analyses of follicle proliferation, mTOR activation, and the effects of LY294002 treatment were similar in transplanted ovaries using either the ear or kidney capsule transplantation model. Conclusions: By adding rapamycin during the OTCTP procedure, we were able to transiently maintain primordial follicles in a quiescent state. This is a promising method for improving the longevity of the ovarian graft. Furthermore, both the ear and kidney capsule transplantation models were suitable for investigating follicle activation and proliferation and pharmacological strategies. [ABSTRACT FROM AUTHOR]

Published

2023

50. Application-Oriented Bulk Cryopreservation of Human iPSCs in Cryo Bags Followed by Direct Inoculation in Scalable Suspension Bioreactors for Expansion and Neural Differentiation.

Author

Meiser, Ina, Alstrup, Monica, Khalesi, Elham, Stephan, Bianca, Speicher, Anna M., Majer, Julia, Kwok, Chee Keong, Neubauer, Julia C., Hansson, Mattias, and Zimmermann, Heiko

Subjects

*BIOREACTORS, *VACCINATION, *CELL size, *REGENERATIVE medicine, *COMPARATIVE method, *FROZEN human embryos, *CRYOPROTECTIVE agents

Abstract

Stem cell-based therapies are promising tools for regenerative medicine and require bulk numbers of high-quality cells. Currently, cells are produced on demand and have a limited shelf-life as conventional cryopreservation is primarily designed for stock keeping. We present a study on bulk cryopreservation of the human iPSC lines UKKi011-A and BIONi010-C-41. By increasing cell concentration and volume, compared to conventional cryopreservation routines in cryo vials, one billion cells were frozen in 50 mL cryo bags. Upon thawing, the cells were immediately seeded in scalable suspension-based bioreactors for expansion to assess the stemness maintenance and for neural differentiation to assess their differentiation potential on the gene and protein levels. Both the conventional and bulk cryo approach show comparative results regarding viability and aggregation upon thawing and bioreactor inoculation. Reduced performance compared to the non-frozen control was compensated within 3 days regarding biomass yield. Stemness was maintained upon thawing in expansion. In neural differentiation, a delay of the neural marker expression on day 4 was compensated at day 9. We conclude that cryopreservation in cryo bags, using high cell concentrations and volumes, does not alter the cells' fate and is a suitable technology to avoid pre-cultivation and enable time- and cost-efficient therapeutic approaches with bulk cell numbers. [ABSTRACT FROM AUTHOR]

Published

2023