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自1985年胚胎玻璃化冷冻(v itrification)保存技术发明以来,玻璃化法先后在小鼠、兔、绵羊、牛、猪、山羊等动物胚胎上获得成功,近年来有关哺乳动物胚胎玻璃化冷冻保存的研究主要集中在冷冻和解冻方法上,相继发明了一些新的玻璃化冷冻方法:冷环玻璃化法(cryo loop)和开放式细管法(open pu lled straw,OPS),并且对解冻后细管内直接脱除防冻剂进行了广泛深入的研究,使得冷冻胚胎移植更易于在生产上推广应用。现将胚胎玻璃化冷冻的原理、冷冻保护剂、冷冻方法、解冻后保护剂脱除方法的最新研究进展作一综述。 相似文献
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牛胚胎冷冻保存的研究进展 总被引:6,自引:0,他引:6
目前,牛的胚胎冷冻保存巳成为一种较成熟的常规技术,广泛应用于牛的繁殖科研与生产。本文回顾了牛胚冷冻保存技术的发展概况,对牛胚胎的常规冷冻技术、直接冷冻法及玻璃化冷冻技术的进展作了简要论述。 相似文献
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哺乳动物胚胎冷冻保存的研究进展 总被引:3,自引:0,他引:3
哺乳动物胚胎冷冻保存技术按其进展分为缓慢冷冻法、快速冷冻法和玻璃冷冻法。玻璃化冷冻法又分为常规细管法和OPS法。本文综述了缓慢冷冻法、快速冷冻法以及玻璃化冷冻法的操作过程及所需的抗冻保护剂,并对各种方法的优缺点进行了初步分析。 相似文献
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卵巢玻璃化冷冻是一种操作简单、冷冻效果好的卵巢组织冷冻降温技术,对动物繁殖能力保存、物种保护、生物多样性保存,以及动物胚胎工程和人类临床医学研究与应用等具有重要意义。卵巢组织冷冻保存较卵母细胞冷冻保存,具有明显的优点。在冷冻保护剂的选择、冷冻材料、冷冻平衡及冷冻方法上都有其特殊之处。卵巢组织冷冻保存技术已在人类医学临床上发挥其应用价值。 相似文献
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猪胚胎冷冻保存研究现状 总被引:1,自引:0,他引:1
猪胚胎超低温冷冻对地方猪种的长期保存意义重大。长期以来,由于猪胚胎脂质含量较高等原因,进展一直较为缓慢(相对于牛、羊等动物)。近年来,由于玻璃化冷冻技术(特别是OPS玻璃化冷冻技术)的突破,使胚胎超低温冷冻保存成功率大幅度提高。本是法国国家农业科学院Francoise Berthelot教授对该领域的最新研究进展作的总结。 相似文献
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澳洲波尔山羊胚胎3种冷冻方法对其胚胎移植效果的影响 总被引:2,自引:0,他引:2
在25℃室温下,采用细管法(一步法、二步法)和OPS法,以不同浓度的EFS、EDFS为玻璃化冷冻液,对澳洲波尔山羊致密桑椹胚和囊胚进行玻璃化冷冻保存。同时利用1.5mol/LEG为抗冻保护剂对胚胎进行常规法冷冻保存。分别将上述3种方法冷冻解冻后的胚胎移植于同期发情后6~7d的云南黑山羊受体。结果表明,细管法胚胎玻璃化冷冻保存效果均以EFS40组为佳,解冻后胚胎移植产羔率分别为40.54%(15/37;一步法)和51.35%(19/37;二步法)。与新鲜胚胎移植产羔率(52.50%,21/40)和常规法冷冻保存的胚胎移植产羔率(45.16%,14/31)相比无显著性差异(P>0.05)。另外,用EDFS30玻璃化溶液,OPS法冷冻解冻后的胚胎移植产羔率高达51.43%(18/35),为整个玻璃化冷冻试验的最佳值。玻璃化冷冻方法简便、迅速,无论是细管法还是OPS法均获得了比较理想的胚胎移植效果。 相似文献
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Many years of poor results of equine embryo cryopreservation has produced a lack of confidence in this technique. Embryo cryopreservation has been successfully used for more than 20 years in other species like bovine and human. The large size of the embryos and the presence of a capsule impermeable to cryoprotectants have been the two main reasons for the failure. In the last few years, a mayor breakthrough for this technique was obtained when large equine embryos could be successfully cryopreserved after breaching the capsule and collapsing the blastocoel cavity. In the present study, we compared the pregnancy rates obtained by vitrification or cryopreservation by slow freezing of embryos smaller than 300 μm. No difference was found between vitrification and slow freezing of embryos <180 μm (pregnancy rate on day 16: 34/61, 55.7%; 6/8, 75%) but produced very low results for embryos between 180 and 300 μm in diameter (0/11, 0%; 1/7, 14.3%). Embryos larger than 300 μm were collapsed before cryopreservation, and two different types of carriers, hemi-straw or Stripper-Tip, were used for vitrification. High pregnancy rates were obtained when the hemi-straw was used as a carrier (7/10, 70% vs. 0/5, 0%), demonstrating that a minimum vitrification volume was essential to preserve the embryo viability. These findings establish that, due to the large range in diameter, equine embryos need to be cryopreserved using different protocols depending on their size. 相似文献
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不同冷冻和解冻方法对小鼠桑椹胚发育的影响 总被引:1,自引:0,他引:1
本试验以2种程序化冷冻液和2种玻璃化冷冻液对昆明白系小鼠的桑椹胚进行细管法冷冻保存,比较程序化冷冻-管外解冻和玻璃化冷冻-管内解冻对胚胎体内、外发育的影响。胚胎体外培养结果表明:玻璃化冷冻组及程序化冷冻组胚胎发育率(95.3% ̄95.8%,98.9%)无显著(P>0.05)差异。将程序化冷冻、EFS30玻璃化冷冻以及新鲜的胚胎各168枚移植给假孕受体鼠,妊娠受体产活仔率各组间相比(50.8%,58.3%,54.9%)无显著性(P>0.05)差异。结果证明,玻璃化冷冻保存的胚胎管内解冻效果好,为生产中家畜的胚胎移植提供了理论和技术参考。 相似文献
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A. Massip 《Reproduction in domestic animals》2001,36(2):49-55
This review contains two parts. The first part is devoted to the significant steps in cryopreservation of mammalian embryos with emphasis on cattle and sheep that serve as models of reference. These steps are: (1) shortening of cooling and warming processes; (2) addition and dilution of cryoprotectant in one step; (3) introduction of plastic straw as a freezing and dilution container; (4) the choice of ethylene glycol as the quite universal cryoprotectant because of its low toxicity and high permeability; (5) vitrification, a cryopreservation method which enable passage from the liquid to the solid state by extreme elevation of viscosity due to high concentration of cryoprotectants and very rapid cooling. There are several vitrification solutions which contain dimethyl sulphoxide, glycerol, ethylene glycol, or a mixture of them, as basic cryoprotectants. The second part considers some factors affecting the efficiency of cryopreservation concerning (i) the origin of embryos and (ii) the stage of development and species. The origin of embryos (in vivo versus in vitro): in vitro embryos show a chilling and freezing sensitivity associated with their lipid content which can be modified by the culture conditions. Both conventional freezing and vitrification have been used and it seems that vitrification is more adapted to in vitro embryos when some modifications of initial protocols are carried out, particularly the rate of cooling. Thus considerable progress has been achieved by using the open pulled straw method of Vajta which enables the use of a minimum volume of freezing medium (0.5 μl) and a very high cooling rate that permits rapid traversal of the damaging temperature zone, corresponding to chilling sensitivity. The stage of development and species: not only are there differences between species at the same stage of development but in the same species all stages of development do not survive equally under the same freezing protocol. In cattle for example, oocytes and early stages of development in vivo or in vitro do not survive whereas compacted morulae and blastocysts survive very well. In the pig hatched blastocysts survive better than the other stages. Horse embryos have special characteristics that pose problems for successful freezing. In conclusion, a lot of work remains to be done to define fundamental characteristics of embryos of certain species (pig, horse) and of embryos of some stages or of oocytes. 相似文献
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探讨程序化冷冻与玻璃化冷冻对小鼠GV期卵母细胞及二细胞期胚胎的复苏率及其发育潜能的影响。通过小鼠的卵母细胞与早期胚胎的不同冷冻方法的比较,为后续阿旺绵羊的胚胎冷冻保存提供参考。采用程序化冷冻与玻璃化冷冻技术,分别冷冻小鼠GV期卵母细胞及二细胞期胚胎,复苏后培养,比较不同冷冻处理后的复苏率、成熟率与囊胚率。小鼠GV期卵母细胞程序化冷冻复苏率(48.00%±5.29%)显著低于玻璃化冷冻复苏率(65.00%±5.00%),有统计学差异(P=0.0147<0.05);而程序化冷冻后复苏卵母细胞的发育成熟率略高于玻璃化冷冻组,但无统计学意义。小鼠二细胞期胚胎程序化冷冻组复苏率(76.00%±2.00%)显著高于玻璃化冷冻组复苏率(70.00%±2.00%),有统计学差异(P=0.0213<0.05);冷冻后复苏胚胎发育的囊胚率程序化冷冻略低于玻璃化冷冻及对照组,但无统计学意义。 相似文献
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Luis B. Ferré Michael E. Kjelland Ahmed M. Taiyeb Fernando Campos-Chillon Pablo J. Ross 《Reproduction in domestic animals》2020,55(6):659-676
Cryopreservation of in vitro-derived bovine embryos is a crucial step for the widespread reproduction and conservation of valuable high-merit animals. Given the current popularity of bovine in vitro embryo production (IVP), there is a demand for a highly efficient ultra-low temperature storage method in order to maximize donor ovum pickup (OPU) turn-over, recipient availability/utilization and domestic/overseas commercial trading opportunities. However, IVP bovine embryos are still very sensitive to chilling and cryopreservation, and despite recent progress, a convenient (simple and robust) protocol has not yet been developed. At the moment, there are two methods for bovine IVP embryo cryopreservation: slow programmable freezing and vitrification. Both of the aforementioned techniques have pros and cons. While controlled-rate slow cooling can easily be adapted for direct transfer (DT), ice crystal formation remains an issue. On the other hand, vitrification solved this problem but the possibility of successful DT commercial incorporation remains to be determined. Moreover, simplification of the vitrification protocol (including warming) through the use of an in-straw dilution without the use of a microscope is a prerequisite for its use under farm conditions. This review summarizes the bovine IVP embryo cryopreservation achievements, strengths and limitations of both freezing systems and prospective improvements to enhance cryosurvival, as well as perspectives on future directions of this assisted reproductive technology. 相似文献
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Numerous reproductive technologies have been developed in the past several decades, which have dramatically changed the way mares are bred. This review will focus on embryo recovery and transfer, cooled-shipped embryos, embryo freezing, oocyte freezing, oocyte collection and transfer, intracytoplasmic sperm injection (ICSI), and sexed semen. Embryo transfer procedures have been constant for many years and the costs have not changed. The major change has been the ability to store embryos at 5 C for 12–24 hours and transport them to recipient stations. Embryo freezing has become more common using the technique of vitrification of embryos >300 μm or deflating embryos >300 μm before freezing. Oocyte vitrification has resulted in poor pregnancy rates although the technique works well in women. The ability to collect oocytes from mares and fertilize them by sperm injection has revolutionized the veterinarian’s approach to infertility in the mare and/or stallion. A transvaginal approach can be used to collect oocytes from preovulatory follicles and unstimulated follicles 5–25 mm in size. Although traditional in vitro fertilization does not work well in the horse, ICSI can be used to produce blastocysts which, upon nonsurgical transfer into recipients, provide a pregnancy rate similar to fresh embryos collected from donor mares. Sorting sperm by flow cytometry into X- and Y-bearing spermatozoa has been shown to provide about a 50% pregnancy rate with freshly sorted sperm but only 12% with sorted, frozen/thawed stallion sperm. It is likely that more advanced reproductive techniques will be developed in the future. Their acceptance will depend on how well they work, perceived need, cost, and, to some extent, the breed associations. 相似文献
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选取奶牛体内生产胚胎93枚(其中囊胚54枚,桑椹胚39枚),比较研究了不同冷冻方法和保护剂对其的保护效果。结果表明:乙二醇处理组对奶牛囊胚的保护效果优于One-Step-Freezing组、甘油组和玻璃化组(回收率、形体正常率和继续发育率四组分别为91.0%、82.0%、66.6%;91.0%、91.0%、88.8%;86.6%、85.0%、83.3%和80.0%、66.7%、50.0%),其中继续发育率在乙二醇组、甘油组和玻璃化组间差异显著(P<0.05);而桑椹胚的各项指标以乙二醇处理组最高,玻璃化组最低,但各组间差异不显著。结果说明乙二醇处理组对胚胎的保护效果优于其它几个处理组。 相似文献