survivaland developmentofmouse 8-cells embryos after vitrification in glycerolsucrose and ethylen glycolbased solutions

نویسندگان

پرویز تاجیک

موسسه تحقیقات واکسن و سرم سازی رازی محمدحسن متدین

موسسه تحقیقات واکسن و سرم سازی رازی حبیب الله ناظم

گروه فیزیو لوژی جانوری علی محمدپور

فارغ التحصیل دانشگاه پیام نور پرویز تاجیک

چکیده

nowadays gamete and embryo freezing is an appropriate approach for preserving of genetic traits in laboratory animals, rare and endangered species. frozen cells are suitable replace for actively breeding animals colony. the aim of this study was to perserve laboratory mouse embryo, using vitrification method and comparing effect of two cryoprotectants, glycerol-sucrose(gs) and ethylene glycol-ficoll-sucrose (efs40) on 8-cells and morula stage embryos of the mouse. following mice superovulation 258(73.5%) out of 351 embryos were in 8-cell and moroula stages. 188 morphologically intact embryos were exposed in the gs and efs40 drops and then each 4 of them transferred to one special micro tube and after ends sealing, finally were cooled up to-196°c with liquid nitrogen vapors and immediately plunged into liquid nitrogen. one to three months later, embryos were thawed, recovered and cultured. the recovery rate of post-thawing embryos from efs group (90%) was more than percentage of embryos recoverd from gs (85%)group. in also survival rate of embryos undergoing further cleavage post-culturing to blastocyte stage, from efs and gs groups were 53/7% and 19/6% respectively. this difference was significant at p

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survival and development of mouse 8-cells embryos after vitrification in glycerol-sucrose and ethylen glycol based solutions

nowadays gamete and embryo freezing is an appropriate approach for preserving of genetic traits in laboratory animals, rare and endangered species. frozen cells are suitable replace for actively breeding animals colony. the aim of this study was to perserve laboratory mouse embryo, using vitrification method and comparing effect of two cryoprotectants, glycerol-sucrose(gs) and ethylene glycol-f...

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Cryopreservation of Day 8 equine embryos after blastocyst micromanipulation and vitrification.

Pregnancy rates after cryopreservation of large equine blastocyst stage embryos have remained lower than other domesticated livestock species. It is generally accepted that the embryonic capsule is the primary barrier to cryoprotectant entry into the embryo proper and techniques need to be developed to circumvent this obstacle. Therefore, the objective of this study was to develop an efficient ...

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the co-culture with vero cells and the development of two cell mouse embryos after vitrification

introduction: the mouse embryos can successfully be vitrified using ethylene glycol as cryoprotectant, however their development differs significantly from the non-vitrified embryos. the ability of their development can be improved when they co-culture with somatic cells. in the present study, the effects of co-culturing with vero cells on the development of vitrified two cell mouse embryos wer...

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Vitrification of Oocytes and Embryos

Currently, controlled ovarian hyperstimulation protocols commonly provide embryos in excess of those needed for fresh transfer. Therefore, techniques have been developed to store these surplus embryos in liquid nitrogen (referred to as cryopreservation) for an indefinite period of time without significant compromise of their quality. Based on data from the Centers for Disease Control and Preven...

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

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-vitrifie...

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Vitrification of Mouse and Sheep Embryos

Vitrification is a method of storing cells in a supercooled state, and is particularly useful for the cryostorage of embryos. With a supply of liquid nitrogen and simple apparatus, vitrification in the field situation is feasible and is potentially simpler and cheaper than the standard freezing processes. However, survival of embryos after vitrification has not yet proved better than after free...

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تحقیقات دامپزشکی

جلد ۶۵، شماره ۱، صفحات ۲۵-۳۰

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