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核移植技术是指通过显微操作技术将供体细胞核转移到去核卵母细胞,进而获得重构胚胎的过程。从上世纪50年代开始到现在,核移植技术得到了广泛的发展和深入的研究,并在生命科学的多个领域发挥重要的作用。核移植技术的建立与发展可分为两个阶段:起始阶段开始于卵体积较大的两栖动物。这一阶段核移植技术主要用来研究细胞核的功能及与胞质之间相互作用。其后核移植技术在哺乳动物中的应用促进了该技术的更深入发展。相对于两栖动物,核移植技术在哺乳动物中的研究和应用也呈现更加深入、多元的特点。主要包括:不同哺乳动物物种及不同供体细胞类型的克隆研究;显微操作技术的发展和完善;重编程机制的研究及核移植效率的提高;核移植在濒危物种保护、个性化干细胞治疗及遗传修饰动物模型构建方面的应用等。该文将就这两个阶段核移植技术的发展历程进行综述并对其在非人灵长类动物模型构建中的应用进行展望。 相似文献
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哺乳动物核移植中线粒体命运 总被引:1,自引:0,他引:1
线粒体是哺乳动物细胞中一种重要的产能、供能细胞器,与生长、发育、衰老和凋亡等多种细胞事件以及多种疾病有关.哺乳动物核移植中,供体细胞和受体卵胞质两种来源的线粒体在重构胚胎发育进程中的变化一直是科学家们研究的热点.对哺乳动物同种胚胎细胞核移植、同种体细胞核移植、异种核移植研究中线粒体的变化进行了综述. 相似文献
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哺乳动物体细胞核移植技术在农业、生物技术、医药生产和濒危动物保护等方面具有很大的潜力和应用价值,已成为目前发育生物学研究的重要方法。但是核重编程仍是核移植技术的关键因素,制约了重构胚胎干细胞的研究。只有供核发生完全重编程,重构胚胎才能正常发育。核重编程与供核者的年龄,供核细胞的组织来源、分化状态、细胞周期、传代次数,供核细胞的表观遗传标记以及供卵者的年龄、卵子的成熟度等因素有关。创造各种适于核重编程的条件有利于从更高的起点开展核移植胚胎干细胞的研究,提高重枸胚胎干细胞建系效率。 相似文献
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体细胞核移植后核重编程的影响因素 总被引:4,自引:0,他引:4
近年来,人类核移植胚胎干细胞建系成为一项炙手可热的研究,用再生医学的理念治疗退行性疾病及器官移植为这一研究带来无穷的魅力和生命力;但是核重编程仍是核移植技术的瓶颈,制约了重构胚胎干细胞的研究。核重编程是指供体细胞核移入卵母细胞后必须停止本身的基因表达程序并恢复为胚胎发育所必需的特定的胚胎表达程序。只有供核发生完全重编程,重构胚胎才能正常发育。核重编程与供核者的年龄,供核细胞的组织来源、分化状态、细胞周期、传代次数,供核的表遗传标记以及供卵者的年龄、卵子的成熟度等因素有关。一般来说,颗粒细胞作为核供体最易被核重编程。供核者为胎体或新生体,供核细胞处于低分化状态或已传数代,供核细胞经过去表遗传标记处理,供卵者性成熟且年龄轻、卵子核与胞浆都成熟等均为有利于核重编程的因素。重构胚胎的培养方法对核重编程也至关重要,目前主张使用序贯培养及体细胞化培养。创造各种适于核重编程的条件有利于从更高的起点开展核移植胚胎干细胞研究,提高重构胚胎干细胞建系效率。 相似文献
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人-兔异种核移植构建克隆胚的实验研究 总被引:1,自引:0,他引:1
“治疗性克隆”是人类最关注的课题之一,而人体细胞核移植是治疗性克隆的基础和前提。异种核移植的方法虽已被引入人体细胞克隆胚的构建,但供体细胞的类型、培养代数及准备方法与其效率之间的关系尚有待探讨。本实验以不同培养代数和不同准备方法的人卵丘细胞、皮肤成纤维细胞和软骨细胞为供体构建了克隆胚,对其发育情况的比较表明,以卵丘细胞为供体时重构胚的体外发育率高于其余二者,差异显著(P〈0.05);不同培养代数的成纤维细胞克隆胚和不同冷藏天数供体细胞克隆胚体外发育率无明显差异。此外,本实验还尝试用荧光原位杂交法检测所构建的异种克隆胚核遗传物质的来源,结果显示来自人体细胞。本研究表明,人一兔异种核移植构建克隆胚切实可行;体细胞的类型与核移植效率相关;供体细胞的体外培养传代对克隆胚的发育并无影响;而冷藏是一种简便有效的供体细胞准备方法;此外,用FISH方法对重构胚进行核遗传物质的鉴定切实可行。 相似文献
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哺乳动物体细胞核移植技术研究进展 总被引:2,自引:0,他引:2
体细胞核移植技术具有十分诱人的应用前景,在农业、物种保护、医疗等领域已显示出优越性。然而核重构等核移植基础理论方面的研究还很薄弱,致使核移植技术还不很完善,克隆动物还存在着甲基化酶异常调节、不正确的印迹基因表达、X染色体异常激活等错误的表观遗传现象,移植成功率较低,在一定程度上限制了它的发展。根据近几年的研究进展,对核移植技术的应用、方法以及存在的问题作一综述 。 相似文献
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为了提高异种间核移植重构胚的发育率,本研究以体内排放的奶山羊成熟卵为供胞质的受体细胞,以人、兔、波尔山羊等的异种或亚种体细胞的原代核移植(Primary Somatic Cell Nuclear Transfer,PSCNT)重构早胚(8-16细胞期)的卵裂球作供核体,观察经亚种或异种卵胞质体短期“修饰”的核再移植产生的继代(Secondary SCNT,SSCNT)重构胚的着床前发育潜能。结果:人、兔、波尔山羊的继代桑椹/囊胚发育率均显著地高于其PSCNT胚胎(人,14.81%VS.7.79%;兔,23.53%VS.12.50%;波尔羊,55.35%VS.24.53%);这些早胚的各阶段发育时程仍遵循供核体动物正常受精卵的发育时程。结果启示:奶山羊成熟卵胞质对异种体细胞核亦具一定的去分化能力,能支持重构胚发育到囊胚;异种重构胚的发育特征是由供体核所决定的;继代核移植几乎能够成倍提高异种间重构胚的着床前发育率,提示核的去分化完全是在母型信息主导的调控之下完成的,而进一步发育的时序似乎是由核决定的:成倍延长在含母型信息主导调控环境中的时间能成倍提高SCNT重构胚的着床前发育率。 相似文献
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本实验用小鼠血液淋巴细胞为核供体进行了核移植研究。用淋巴细胞分离液(比重1.088)分离出小鼠血液中的淋巴细胞,直接用作核移植供体细胞,采用胞质内注射法成功构建的重构胚经常规培养2h后,SrCl_2激活处理6h,然后添加mM16培养液和小鼠输卵管上皮细胞饲养层共培养。把发育至早期囊胚阶段的重构胚转移至小鼠胎儿成纤维细胞饲养层上,添加ES细胞培养液继续培养。对孵化出的内细胞团进行消化,然后接种培养。结果显示,小鼠血液淋巴细胞可以支持体细胞核移植重构胚的发育,核移植重构胚2-细胞率41.03%(128/312),桑葚胚和囊胚发育率分别为9.29%(29/312),1.92%(6/312)。重构囊胚在小鼠胎儿成纤维细胞饲养层上分离出2个内细胞团,分离率为0.64%(2/312)。实验证实利用小鼠血液淋巴细胞进行体细胞核移植是可行的,可用于深入研究。 相似文献
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Jingjuan Ji Tonghang Guo Xianhong Tong Lihua Luo Guixiang Zhou Yingyun Fu Yusheng Liu 《生物学前沿》2007,2(1):80-84
Therapeutic cloning,which is based on human somatic cell nuclear transfer,is one of our major research objectives.Though inter-species nuclear transfer has been introduced to construct human somatic cell cloned embryos,the effects of type,passage,and preparation method of donor cells on embryo development remain unclear.In our experiment,cloned embryos were reconstructed with different passage and preparation methods of ossocartilaginous cell,skin fibroblast,and cumulus cells.The cumulus cell embryos showed significantly higher development rates than the other two (P<0.05).The development rate of embryos reconstructed with skin fibroblasts of different passage number and somatic cells of different chilling durations showed no significant difference.Also,fluorescence in situ hybridization (FISH)was conducted to detect nuclear derivation of the embryos.The result showed that the nuclei of the inter-species cloned embryo cells came from human.We conclude that (1)cloned embryos can be constructed through human-rabbit interspecies nuclear transfer;(2)different kinds of somatic cells result in different efficiency of nuclear transfer,while in vitro passage of the donor does not influence embryo development;(3)refrigeration is a convenient and efficient donor cell preparation method.Finally,it is feasible to detect DNA gcnotype through FISH. 相似文献
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Ji Jingjuan Guo Tonghang Tong Xianhong Luo Lihua Zhou Guixiang Fu Yingyun Liu Yusheng 《Frontiers of Biology in China》2007,2(1):80-84
Therapeutic cloning, which is based on human somatic cell nuclear transfer, is one of our major research objectives. Though
inter-species nuclear transfer has been introduced to construct human somatic cell cloned embryos, the effects of type, passage,
and preparation method of donor cells on embryo development remain unclear. In our experiment, cloned embryos were reconstructed
with different passage and preparation methods of ossocartilaginous cell, skin fibroblast, and cumulus cells. The cumulus
cell embryos showed significantly higher development rates than the other two (P < 0.05). The development rate of embryos reconstructed with skin fibroblasts of different passage number and somatic cells
of different chilling durations showed no significant difference. Also, fluorescence in situ hybridization (FISH) was conducted to detect nuclear derivation of the embryos. The result showed that the nuclei of the
inter-species cloned embryo cells came from human. We conclude that (1) cloned embryos can be constructed through human-rabbit
interspecies nuclear transfer; (2) different kinds of somatic cells result in different efficiency of nuclear transfer, while
in vitro passage of the donor does not influence embryo development; (3) refrigeration is a convenient and efficient donor
cell preparation method. Finally, it is feasible to detect DNA genotype through FISH.
Translated from Zoological Research, 2005, 26(4): 416–421 [译自: 动物学研究] 相似文献
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We have compared the effect of the genetic background of recipient oocytes on the in vitro and in vivo development of nuclear transfer reconstructed embryos in goats. Adult fibroblast cells from Boer goats were used as donor cells, and recipient oocytes were obtained from Boer goats and Boer cross-breeds (Boer♂×Huanghuai♀). Nuclear transfer reconstructed embryos were cultured in vitro, or transferred into recipient goats. The mitochondrial origin of 2 cloned Boer goats was investigated by analysing the D-loop region based on polymorphisms via DNA sequencing. There was no significant difference in the fusion rate and cleavage rate of reconstructed embryos (P>0.05), when using Boer and cross-breeding goat oocytes as recipient cytoplast respectively. However, in vitro morula development of reconstructed embryos from Boer oocytes was significantly higher than that of cross-breeding embryos (34.1% versus 19.1%, P<0.05). There was no significant difference in the rate of pregnancy and foetus loss between the 2 breeds. However, the live-birth rate was significantly higher with Boer goat oocyte recipients than the cross-breeds (3.1% versus 0.8%, P<0.05). Mitochondrial analysis showed that the 2 cloned goats were similar to their respective oocyte donor goats, and significantly different from the nucleus donor. In conclusion, genetic background of recipient oocytes affected in vitro and in vivo development of reconstructed embryos, with the homologous background of cytoplast and nuclear donor benefiting development of reconstructed embryos. The mitochondrial origin of the 2 cloned Boer goats came from recipient oocytes, not donors. 相似文献
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目前动物克隆技术体系极待完善,其极低的成功率及克隆动物普遍存在的早衰、早天现象是阻碍研究深入进行的首要问题,其突破的关键在于对核移植后的细胞核再程序化机制的阐明。从移植核在结构上的重塑、移植核与受体卵细胞质所处的细胞周期及其相互作用、重构胚与两性胚在分子水平的变化等多方面研究表明:受体细胞质的环境对于细胞核的再程序化至关重要,处于有丝分裂各时期的细胞作为核供体一旦移植到卵母细胞后,移植核在卵质环境里将出现结构上的重塑和分子的再程序化;移植核与受体卵问细胞周期的相容性、重构胚的染色体倍性的正确与否,可能是决定重构胚发育率高低的重要因素;合子型基因激活是基因表达再程序化的关键事件之一;印记基因对于体细胞克隆动物移植核的再程序化过程可能起着非常独特的作用。 相似文献
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Gao S McGarry M Priddle H Ferrier T Gasparrini B Fletcher J Harkness L De Sousa P McWhir J Wilmut I 《Molecular reproduction and development》2003,66(2):126-133
Mice have been successfully cloned from somatic and embryonic stem (ES) cells using the "Honolulu method." In the present study, different donor oocytes and different culture conditions were compared to evaluate the developmental potential of nuclear transfer embryos reconstructed with an inbred ES cell line HM-1. Oocytes were recovered from two different F1 donors B6D2F1 (C57BL/6 x DBA/2) and B6CBAF1 (C57BL/6 x CBA). There was no effect of oocyte origin on development of cloned embryos to the morulae/blastocyst stage (B6D2F1 44.1% vs. B6CBAF1 45.0%), and the transferred embryos could develop to term. Two culture conditions were compared to show their ability to support development to the morulae/blastocyst stage of reconstructed embryos with B6D2F1 oocytes. The total cell number in the cloned blastocysts cultured in M16 with 20% oxygen was much higher than that observed in CZB with 20% oxygen. Low oxygen concentration during culture of nuclear transfer embryos in CZB medium showed no beneficial effect on pre-implantation development, no embryos developed to term after transfer to surrogate mothers. Our results demonstrated that not only B6D2F1, but B6CBAF1 oocytes, can be used for nuclear transfer. M16 medium is superior for culture of nuclear transfer embryos and low oxygen concentration with CZB medium during culture shows no benefit on development of cloned embryos. 相似文献