Your search keyword '"Ebrahimi, Bita"' showing total 9 results

1. Mouse preantral follicle development in two-dimensional and three-dimensional culture systems after ovarian tissue vitrification.

Author

Sadr, Seyedeh Zeynab, Ebrahimi, Bita, Shahhoseini, Maryam, Fatehi, Roya, and Favaedi, Raha

Subjects

*OVARIAN follicle, *INFERTILITY treatment, *CELL culture, *GENE expression, *LABORATORY mice, *OVARIAN physiology, *OVUM physiology, *ANIMAL experimentation, *BONE morphogenetic proteins, *CRYOPRESERVATION of organs, tissues, etc., *GROWTH factors, *RESEARCH methodology, *MICE, *OVARIES, *TISSUE culture

Abstract

Objectives: This work on follicle culture and evaluation of expression of oocyte maturation genes helps to better understand the complicated processes of folliculogenesis and to develop new approaches for infertility treatment.Study Design: Ovaries of 12-day-old female NMRI mice were divided into control and vitrification groups. After vitrification and warming procedures, ovarian tissue morphologies were histologically evaluated and compared to those of the control group. In the second stage, preantral follicles were mechanically isolated from non-vitrified and vitrified ovaries and cultured for 12 days in two-dimensional (2D) and three-dimensional (3D) systems. Finally, the survival and growth rate of follicles and quantitative expression of oocyte maturation genes (Gdf9, Bmp15 and Bmp6) were studied.Result: Morphological integrity of ovarian tissue in vitrification group was well preserved. Survival rates of cultured preantral follicles in control group during 2D and 3D systems were somewhat similar, but were significantly different between 2D and 3D systems in vitrification group. Although the growth rate of follicles was similar in the 3D system in both groups, substantially higher growth rate was observed for the control group in the 2D system. Expressions of oocyte maturation genes were, to some extent, similar between control and vitrification groups. There was a remarkable reduction in expression pattern of genes in 3D compared to 2D system in both experimental groups, during the 12th day of culture period.Conclusions: 3D in-vitro culture system could be appeared more appropriate than 2D culture system for preservation of follicles in terms of spatial morphology, growth rate and expression reduction of maturation genes. [ABSTRACT FROM AUTHOR]

Published

2015

2. Vitrification of mouse preantral follicles versus slow freezing: Morphological and apoptosis evaluation.

Author

Taghavi, Seyed Abdolvahab, Valojerdi, Mojtaba Rezazadeh, Moghadam, Mehdi Forozandeh, and Ebrahimi, Bita

Subjects

OVARIAN follicle, APOPTOSIS, CELL morphology, CRYOPRESERVATION of organs, tissues, etc., GENE expression, LABORATORY mice

Abstract

The aim of this study was evaluation of survivability, maturation rate and apoptotic gene expression of preantral follicles after vitrification and slow freezing technique. Normal mouse preantral follicles were randomly divided into three experimental groups. In the control group, follicles were cultured immediately; in the vitrification and slow freezing groups, follicles were cultured after vitrification-warming and slow freezing-thawing procedures. Follicular viability was assessed by using 0.4% trypan blue, and molecular evaluation of messenger RNA levels of apoptosis-related genes was performed by the semi-quantitative RT-PCR method after 3 h of culture. Oocyte maturation rates were also evaluated on day 14 of culture. Survival and maturation rate in the slow freezing group were significantly lower than those in control and vitrification groups (P = 0.05). Although there was no difference in Survivin expression among the three experimental groups, Bcl-2 expression was significantly lower in the slow freezing group compared to the other groups (P = 0.05). The expression of Bax, P53, Fas and Bax/Bcl-2 ratio in the slow freezing group was significantly higher than control and vitrification groups (P = 0.05). Preantral follicle vitrification seems to be better than slow freezing as seen in the survival, maturation and expression rates of apoptotic gene variants. [ABSTRACT FROM AUTHOR]

Published

2015

3. Effect of ovarian tissue vitrification method on mice preantral follicular development and gene expression.

Author

Fatehi, Roya, Ebrahimi, Bita, Shahhosseini, Maryam, Farrokhi, Ali, and Fathi, Rouhollah

Subjects

*OVARIAN follicle, *GENE expression, *MICE embryology, *CRYOPRESERVATION of organs, tissues, etc., *IN vitro studies, *ANIMAL morphology

Abstract

Abstract: Vitrification is considered a viable method for cryopreservation of ovarian tissue and selection of methods that minimize follicular damage is important. The objective of the present study was to evaluate the effects of two vitrification methods on ovarian tissue morphology, preantral follicles survival rate during in vitro culture, and relative expression of genes associated with oocyte maturation and cumulus expansion. Ovaries from 12-day-old mice were vitrified in media containing ethylene glycol, dimethyl sulphoxide, and sucrose. Before plunging in liquid nitrogen, ovaries were first loaded into an acupuncture needle (needle immersion vitrification [NIV]) or placed on a cold steel surface for 10 to 20 seconds (solid surface vitrification [SSV]). The integrity of the ovarian tissue was well-preserved after vitrification and was similar controls. Follicle viability in the SSV group was lower (P < 0.05) than in the control group after 6 days of culture and the NIV group after 10 day of culture. Follicle viability after 12 day of culture was 92.8%, 82.1%, and 58.4% in control, NIV, and SSV groups, respectively. Bmp15, Gdf9, BmprII, Alk6, Alk5, Has2, and Ptgs2 gene expression patterns were similar among groups. However, the level of gene expression in the vitrification groups during Days 6 to 10 were higher compared with the control group. In conclusion, ovarian tissue morphologic integrity was well-preserved, regardless of the vitrification method. Vitrification using the needle immersion method resulted in greater follicular survival after 12 day of culture than the SSV method. Gene expression patterns during culture did not seem to explain the reduced survival rate observed in the solid surface group. [Copyright &y& Elsevier]

Published

2014

4. Ultrastructural changes of sheep cumulus–oocyte complexes following different methods of vitrification.

Author

Ebrahimi, Bita, Valojerdi, Mojtaba Rezazadeh, Eftekhari-Yazdi, Poopak, and Baharvand, Hossein

Subjects

ULTRASTRUCTURE (Biology), OVUM, MAMMAL reproduction, SHEEP, VITRIFICATION, LIQUID nitrogen, MITOCHONDRIA, ZONA pellucida, CRYOPRESERVATION of organs, tissues, etc.

Abstract

To determine the ultrastructural changes of sheep cumulus–oocyte complexes (COCs) following different methods of vitrification, good quality isolated COCs (GV stage) were randomly divided into the non-vitrified control, conventional straw, cryotop and solid surface vitrification groups. In both conventional and cryotop methods, vitrified COCs were respectively loaded by conventional straws and cryotops, and then plunged directly into liquid nitrogen (LN2); whereas in the solid surface group, vitrified COCs were first loaded by cryotops and then cooled before plunging into LN2. Post-warming survivability and ultrastructural changes of healthy COCs in the cryotop group especially in comparison with the conventional group revealed better viability rate and good preservation of the ooplasm organization. However in all vitrification groups except the cryotop group, mitochondria were clumped. Solely in the conventional straw group, the mitochondria showed different densities and were extremely distended. Moreover in the latter group, plenty of large irregular connected vesicles in the ooplasm were observed and in some parts their membrane ruptured. Also, in the conventional and solid surface vitrification groups, cumulus cells projections became retracted from the zona pellucida in some parts. In conclusion, the cryotop vitrification method as compared with other methods seems to have a good post-warming survivability and shows less deleterious effects on the ultrastructure of healthy vitrified–warmed sheep COCs. [ABSTRACT FROM PUBLISHER]

Published

2012

5. Fertility Preservation in Cancer Patients: In Vivo and In Vitro Options.

Author

Fathi, Rouhollah, Valojerdi, Mojtaba Rezazadeh, Ebrahimi, Bita, Eivazkhani, Farideh, Akbarpour, Mahzad, Tahaei, Leila Sadat, and Abtahi, Naeimeh Sadat

Subjects

*FERTILITY preservation, *OVUM cryopreservation, *HUMAN embryos -- Preservation, *CRYOPRESERVATION of organs, tissues, etc., *CANCER patients, *CANCER

Abstract

Oocyte, embryo and ovarian tissue cryopreservation are being increasingly proposed for fertility preservation among cancer patients undergoing therapy to enable them to have babies after the cancer is cured. Embryo cryopreservation is not appropriate for single girls without any sperm partner and also because oocyte retrieval is an extended procedure, it is impossible in cases requiring immediate cancer cure. Thus ovarian tissue cryopreservation has been suggested for fertility preservation especial in cancer patients. The main goal of ovarian cryopreservation is re-implanting the tissue into the body to restore fertility and the hormonal cycle. Different cryopreservation protocols have been examined and established for vitrification of biological samples. We have used Cryopin to plunge ovarian tissue into the liquid nitrogen and promising results have been observed. Ovarian tissue re-implantation after cancer cure has one problem- the possibility of recurrence of malignancy in the reimplanted tissue is high. Xenografting-implantation of the preserved tissue in another speciesalso has its drawbacks such as molecular signaling from the recipient. In vitro follicle culturing is a safer method to obtain mature oocytes for fertilization and the various studies that have been carried out in this area are reviewed in this paper. [ABSTRACT FROM AUTHOR]

Published

2017

6. The effect of agar substrate on growth and development of cryopreserved-thawed human ovarian cortical follicles in organ culture.

Author

Ghezelayagh, Zeinab, Abtahi, Naeimeh Sadat, Khodaverdi, Sepideh, Rezazadeh Valojerdi, Mojtaba, Mehdizadeh, Aboulfazl, and Ebrahimi, Bita

Subjects

*ORGAN culture, *OVARIAN follicle, *AGAR, *TISSUE culture, *GENE expression, *OVARIES, *POLYSACCHARIDES, *RESEARCH methodology, *CRYOPRESERVATION of organs, tissues, etc.

Abstract

Objective: To preserve human ovarian tissue structure and improve follicular growth and survival during in-situ culture, various biomaterials are used. In this study we aimed to compare agar as a cultivation substrate with matrigel-coated insert in order to achieve an optimum system for in-situ human follicle culture.Study Design: Frozen-thawed human ovarian cortical tissues were cultured on either matrigel-coated inserts or agar-soaked substrates. The proportion of morphologically viable and degenerated follicles at different developmental stages, secreted hormonal levels, and apoptotic and proliferation gene expressions were compared between the cultured groups after 7-days of culture.Results: The follicular growth was not significantly different between the two cultured groups, although showing higher percentage of growing follicles in agar cultured group. The secreted hormonal levels didn't have any difference between two cultured groups. Although the apoptotic gene expressions didn't show any difference between the cultured groups, the apoptotic index was lower in agar cultured group. In addition, Ki67 gene expression, a proliferative marker, showed a significantly higher expression in agar cultured group.Conclusion: Based on the results, agar is as suitable as matrigel-coated inserts for the survival and growth of follicles during culture. Therefore, agar can be an inexpensive alternative substrate for culturing frozen-thawed human ovarian cortical strips. [ABSTRACT FROM AUTHOR]

Published

2021

7. Effect of Different Thawing Rates on Post-Thaw Viability, Kinematic Parameters and Chromatin Structure of Buffalo (Bubalus bubalis) Spermatozoa.

Author

Rastegarnia, Abdolreza, Shahverdi, Abdolhossein, Topraggaleh, Tohid Rezaei, Ebrahimi, Bita, and Shafipour, Vahid

Subjects

*CHROMATIN, *LIQUID nitrogen, *ANALYSIS of variance, *WATER buffalo, *CRYOPRESERVATION of organs, tissues, etc.

Abstract

Objective: The aim of the present study was to evaluate three thawing rates on the post thaw motility, viability and chromatin structure of buffalo semen frozen in 0.5-ml straws. Materials and Methods: In this experimental study semen was collected with artificial vagina (42°C) from four buffalo bulls.Split pooled ejaculates (n=4) were extended at 37°C with a Bioxcell® extender. Semen was cooled to 4°C within 2 hours, equilibrated at 4°C for 4 hours, then filled in 0.5 ml French straws, and frozen in programmable cell freezer before plunging into liquid nitrogen. Straws were thawed at water bath temperatures of 37, 50 or 70°C for 30, 15 and 6 seconds, respectively. Semen was incubated at 37°C for 2 hours and evaluated for post thaw motility, viability, acrosomal and DNA integrity of spermatozoa. Analysis of variance (ANOVA) was used for comparisons of means. When the ANOVA test showed statistical differences, the mean of the treatments were compared using Duncan's multiple range tests. Results: The initial postthaw motility (0 hour) averaged 62.7 ± 7.2%, 73.1 ± 9.77%, and 74.9 ± 8.58% for the three thaw rates, respectively. Kinematic parameters such as average path velocity, linearity and beat/cross frequency in the thaw rate of 70°C for 6 seconds were superior to other rates studied (p<0.05). After 2 hours of incubation, proportions of progressive motility and Kinematic parameters decreased in all groups (p>0.05). A positive correlation was detected between sperm motility and thawing rate after two hours incubation times. The percentage of viable spermatozoa and spermatozoa with an intact acrosome and plasma membrane integrity were not different between the groups of samples thawed at different temperatures (p>0.05). The percentage of spermatozoa with chromatin dispersion forthe thaw rate of 70°C for 6 seconds was significantly higher than for the to other rates studied (p< 0.05). In contrast with motility and viability, the DNA integrity of post thaw spermatozoa remained unaffected during 2 hours incubation. Conclusion: The post thaw motility and kinematic parameters of buffalo spermatozoa were significantly improved immediately after thawing by increasing the thawing rate from 37°C in 30 seconds to70°C in 6 seconds. However, this relative advantage had disappeared after incubation in a water bath at 37°C for two hours.A thaw rate of 70°C for 6 seconds was associated with higher chromatin dispersion than the other thaw rates studied. Sperm thawing over at 50 degrees could be safely used to improve motility recovery after sperm cryopreservation in buffalo bulls. [ABSTRACT FROM AUTHOR]

Published

2012

8. Development of 4-cell mouse embryos after re-vitrification

Author

Fathi, Rouhollah, Valojerdi, Mojtaba R., Yazdi, Poopak E., Ebrahimi, Bita, Alipour, Hiva, and Hassani, Fatemeh

Subjects

*EMBRYOS, *CELL physiology, *CRYOPRESERVATION of organs, tissues, etc., *LABORATORY mice, *CULTURE media (Biology), *BLASTOCYST

Abstract

Abstract: This paper reports studies on the effects of re-vitrification by the CPS (Closed Pulled Straw) method on the development of 4-cell stage mouse embryos. The procedure involved culturing 2-cell mouse embryos in G-1 medium until the 4-cell stage followed by the division of the normal 4-cell stage embryos into a control group (non-vitrified) and two experimental subgroups (vitrified and re-vitrified). Embryos in the vitrified subgroup were cryopreserved by the CPS vitrification method. In the second experimental subgroup (re-vitrified), embryos that were already vitrified were warmed and cryopreserved again by the same method. There was no significant reduction in the rate of blastocyst formation after vitrification and re-vitrification. However, re-vitrification reduced the total cell number, ICM (inner cell mass) percent and blastocyst diameter (P <0.05). These results showed that vitrification and re-vitrification by the CPS method did not negatively affect the development of vitrified-warmed 4-cell mouse embryos, whereas re-vitrification significantly reduced both the cell number and diameter of blastocysts. [Copyright &y& Elsevier]

Published

2012

9. Primary follicles grew in Erythropoietin and HMGs treated human xenotransplanted vitrified ovary.

Author

Tafti, Elahe Dehghani, Tahaei, Leila Sadat, Fatehi, Roya, Abtahi, Naeimeh Sadat, Farideh eivazkhani, null, Ebrahimi, Bita, Eimani, Hussein, Khodaverdi, Sepideh, Nasrollah, Mostafa Haji, Shojaei, Bahador, Tootian, Zahra, and Fathi, Rouhollah

Subjects

*FOLLICLE-stimulating hormone, *ERYTHROPOIETIN, *XENOTRANSPLANTATION, *CRYOPRESERVATION of organs, tissues, etc., *LABORATORY mice

Published

2018