615小鼠ES细胞集落的分离及初步鉴定

目的　分离和培养 6 15小鼠的ES细胞集落 ,为建系打下基础。方法　以PMEF为饲养层分离 6 15小鼠的ES细胞集落 ,进行无饲养层培养 ,并对其进行初步鉴定。结果　ES细胞集落的出现率和传代成功率为 2 2 6 %和 0 94 % ,其ALP染色阳性 ,具有稳定的二倍体核型 ,可自发分化为多种类型的细胞。结论　成功分离和培养了6 15小鼠的ES细胞集落     

改进的培养体系在小鼠体细胞核移植及重构胚ES细胞分离培养中的应用

取8周后的雌性昆明小鼠进行超排,取卵母细胞用作核受体,收集卵母细胞周围的卵丘细胞作核供体,进行体细胞核移植。核移植重构胚经SrCl2激活处理6h后,与改良的M16培养液和小鼠输卵管上皮细胞共培养;将发育到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,添加含心肌细胞培养液的ES细胞培养液;把孵出的ICM进行消化接种培养,对孵出的ES细胞集落进行鉴定培养。结果显示,以小鼠卵丘细胞为核供体,体细胞核移植重构胚激活率为65．23％,囊胚发育率为11．69％;9个核移植重构囊胚中分离出ES细胞集落,分离率为2．77％;分离出的核移植ES细胞集落具有岛屿状团状隆起结构、碱性磷酸酶染色呈阳性,体外分化可形成类胚体,并能分化成上皮样或梭形细胞。ES细胞集落经常规冻存和复苏后,显示出同冻存前相似的集落形态,并具有较强的增殖能力。实验证实小鼠输卵管上皮细胞、改良的M16培养液及含心肌细胞培养液的ES细胞培养液可以更为成功地运用于小鼠的体细胞核移植及ES细胞的分离培养研究。     

用饲养层分离胚胎干细胞集落的实验初探

目的 用饲养层分离胚胎干细胞集落。方法 用胚龄为13~14 d的小鼠胚胎分离原代成纤维细胞,制成饲养层,用于囊胚的培养。结果 小鼠原代胚胎成纤维细胞（PMEF）贴壁能力较好,增殖快,易铺层。囊胚和内细胞团（ICM）在饲养层上贴壁生长良好,当培养4~5 d时,其增殖率为16/28（57%）。在ICM离散48 h后,各种胚胎干细胞（ES）集落开始出现。此种集落经碱性磷酸酶染色成阳性。结论 用饲养层分离胚胎干细胞获得初步成功。     

慢病毒介导Nanog基因在小鼠ES细胞的表达

试验尝试构建小鼠Nanog基因慢病毒表达载体,培养表达外源Nanog基因的小鼠ES细胞。结果显示通过RT-PCR扩增出918bp的小鼠Nanog基因,测序正确的小鼠Nanog基因通过慢病毒介导在小鼠ES细胞表达后,表达外源Nanog基因的小鼠ES细胞生长状态同普通ES细胞无明显差异,在无LIF的ES细胞培养液培养条件下,表达外源Nanog基因的小鼠ES细胞保持正常的ES细胞集落,碱性磷酸酶、Oct4和SSEA-1免疫细胞化学检测为阳性,相同情况下未表达外源Nanog基因的小鼠ES细胞集落退化消失。试验证实了通过慢病毒载体介导培养了表达外源Nanog基因的小鼠ES细胞。试验尝试构建小鼠Nanog基因慢病毒表达载体,培养表达外源Nanog基因的小鼠ES细胞。根据小鼠Nanog基因m RNA序列设计Nanog基因引物,引物两端带有Nhe I和Xho I酶切位点。Trizol试剂处理小鼠ES细胞,通过RT-PCR扩增出小鼠Nanog基因,小鼠Nanog基因用Nhe I和Xho I酶切后连入pcDNA3.1载体中,PCR检测阳性的细菌克隆进行测序,测序正确的Nanog基因片段连接入PLL-IRES-Neo慢病毒表达载体中,包装含有Nanog基因的慢病毒感染小鼠ES细胞,在SNL细胞饲养层上G418筛选2周后,添加普通ES细胞培养液在普通小鼠胎儿成纤维细胞饲养层上培养。结果显示通过RT-PCR扩增出918 bp的小鼠Nanog基因,测序正确的小鼠Nanog基因通过慢病毒介导在小鼠ES细胞表达后,表达外源Nanog基因的小鼠ES细胞生长状态同普通ES细胞无明显差异,在无LIF的ES细胞培养液培养条件下,表达外源Nanog基因的小鼠ES细胞保持正常的ES细胞集落,碱性磷酸酶、Oct4和SSEA-1免疫细胞化学检测为阳性,相同情况下未表达外源Nanog基因的小鼠ES细胞集落退化消失。试验证实了通过慢病毒载体介导培养了表达外源Nanog基因的小鼠ES细胞。     

昆明白小鼠胚胎干细胞分离与体外培养

为探索昆明白小鼠胚胎干细胞建系方法,将受孕4.5天的昆明白小鼠囊胚用免疫手术法去除滋胚层,然后将内细胞团(ICM)接种于胎鼠成纤维细胞饲养层上培养,形成的胚胎干细胞样集落用胰蛋白酶-EDTA消化法传代,培养后进行相差显微镜观察及碱性磷酸酶染色。结果饲养层上生长的ICM细胞呈典型的ES样细胞集落,传至第8代碱性磷酸酶染色呈强阳性。实验表明免疫手术法适用于昆明白小鼠ES细胞建系,获得的细胞集落具有ES细胞的主要生物学性状。     

大鼠心脏细胞条件培养基对小鼠ES细胞特性的维持

以C19-2和MESPU-13为供试细胞,用克隆测试、传代培养等方法对17种细胞的条件培养基进行了筛选,结果表明,大鼠心脏细胞的条件培养基（RH-CM）具有显著抑制小鼠ES细胞分化、维持其二倍体核型、促进ES细胞贴壁生长的作用。经RH-CM培养10代和20代的小鼠ES细胞在体内外分化能力上仍保留了原ES细胞的多方向分化潜能和特征;RH-CM也可作为小鼠ES细胞培养基的添加物,用含70%RH-CM的ES细胞培养基和小鼠胚胎原代成纤维细胞饲养层（PMEF）培养ES细胞,可长期有效地维持其未分化状态和二倍体核型。RT-PCR检测到大鼠心脏细胞有LIF mRNA表达。     

免疫外科法分离克隆BALB/c小鼠胚胎干细胞

目的　使用免疫外科法分离克隆BALB c小鼠胚胎干细胞 (embryonicstemcells,ES细胞 ) ,为进一步建立BALB c小鼠ES细胞系打下基础。方法　用免疫外科法从 4 5枚BALB c小鼠囊胚中分离得到 2 0枚去除滋养层细胞的ICM ,接种在MEF饲养层上 ,使用DMEM(高糖 ) 15 ?S 0 1mmol Lβ 巯基乙醇 0 0 1mmol L非必需氨基酸 10 0 0IU mlLIF 10 0IU mL青霉素 10 0IU ml链霉素培养液 ,17枚形成典型的ICM集落 (85 0 % ) ,有一枚胚胎传至第 10代。用于全胚培养的BALB c小鼠胚胎共 10 2枚 ,使用与免疫外科相同的培养方法 ,6 6枚形成典型的ICM集落 (6 4 7% ) ,其中一枚胚胎传至第 8代。结果　免疫外科法较全胚培养法有利于小鼠ES细胞的分离与克隆 ;添加LIF(10 0 0IU ml)有利于小鼠ES细胞的分离与传代 (P <0 0 5 ) ;0 0 5 %胰酶 0 0 0 8?TA是较好的ES细胞消化液 ,对细胞综合损伤力小 ,且传代后ES细胞集落形成能力也较高 (P <0 0 5 )。结论　分离得到的ES细胞经形态学观察 ,AKP染色 ,体外分化实验 ,核型分析等证明其具有胚胎干细胞的诸多特性。     

昆明小鼠胚胎干细胞的体外分离培养

利用昆明小鼠13.5dpc的胚胎制备小鼠胚胎成纤维细胞,并以小鼠胚胎成纤维细胞作为饲养层;收集3.5dICR小鼠的囊胚和桑椹胚进行体外培养,筛选纯化ES细胞集落,使其稳定传代后,对其形态学和生物学性状进行初步鉴定,获得阳性细胞集落。     

牛体细胞克隆胚胎类ES细胞集落的筛选及其核移植

对第7d的牛体细胞克隆囊胚进行体外增殖培养,分离筛选类ES细胞,并对其进行了传代培养,接种在饲养层上的体细胞克隆囊胚细胞,在传代的24h内增殖形成小集落,2～3d有雀巢状的集落出现,筛选形态相同的细胞集落进行传代培养,4～5代后,皿底出现多个大小不等的多细胞单层集落,将传4～5代的细胞集落接种到无饲养层的4孔培养皿中培养,24h出现多细胞单层集落,4～7d长满皿底,并形成上皮样细胞,呈网状,将其作为核供体细胞进行核移植实验。结果有80%（40/50）核-质融合的移核重构胚发生卵裂,5%（2/40）发育至桑椹胚期,2.5%（1/40）发育至囊胚期,92.5%（37/40）停止在2～4细胞期,结果表明：采用牛体细胞克隆胚胎的类ES细胞进行核移植,具发育形成早期胚胎的潜能。     

不同培养体系对绵羊类胚胎干细胞分离、传代的影响

以小鼠胚胎成纤维细胞(MEF)为饲养层, 研究了用Knockout血清替代品(Knockout serum replacement, KSR)代替胚胎干细胞(Embryonic stem cells, ES cell)培养液中的胎牛血清(FBS)和向含KSR的基础培养液中添加40%的小鼠ES细胞条件培养液(ES cell conditioned medium, ESCCM)对绵羊类ES细胞分离、克隆效率的影响。发现使用含FBS的基础培养液最多可以把绵羊类ES细胞传至3代, 而使用KSR和添加ESCCM能促进绵羊类ES细胞的分离和克隆, 所获得的类ES细胞分别可稳定传至第5和8代。同时对类ES细胞进行核型分析、AKP染色及体外分化能力检测, 证实所分离的类ES细胞符合ES细胞的主要特征。由此认为, 与FBS相比KSR更加适于绵羊类ES细胞的分离与培养; 而小鼠ES细胞在生长过程中可能分泌某些重要的细胞因子, 从而达到促进绵羊ES细胞增值的作用。     

Establishment of the Embryo-derived Stem (ES) Cell Lines from Mouse Blastocysts: Effects of the Feeder Cell Layer.

The ES ceii lines are embryo-derived stem cell lines directly isolated from the inner cell mass of mouse blastocysts using feeder cell layer. We have established a number of ES cell lines from 129 or C57BL/6 strain mice by using the feeder layer of the STO cells (from ATCC) or the primary embryonic fibroblasts, which was obtained by trypsinizing the 16-day-old BALB/c mouse fetus. The ES cell lines established on the STO feeder layer showed differentiation into various tissues in solid tumors when injected into syngenic mice. Karyotype was, however, nearly tetraploid. The ES cell lines established on the primary fibroblasts exhibited differentiation into larger variety of tissues in solid tumors. Karyotype was almost diploid and majority of the cells kept normal set of chromosomes in G-banding. We conclude that the primary fibroblasts are better feeder layer than the STO cells for establishment and maintenance of the ES cell lines.     

Isolation of embryonic stem (ES) cells in media supplemented with recombinant leukemia inhibitory factor (LIF)

The isolation of pluripotent murine embryonic stem (ES) cells has previously been achieved by coculturing the ES cells with fibroblast feeder cells. In this report we demonstrate that ES cell lines can be isolated from murine 129/Sv He blastocysts in the absence of feeder cells in culture medium supplemented with recombinant leukemia inhibitory factor (LIF). Three of the ES cell lines (MBL-1, MBL-2, and MBL-3) were isolated by directly explanting blastocysts, whilst two ES cell lines (MBL-4 and MBL-5) were isolated from blastocysts pretreated by immunosurgery. Three of the ES cell lines contained the Y chromosome (MBL-1, MBL-2, and MBL-5) with a high proportion of the cells displaying a normal diploid karyotype with a modal chromosome number of 40. All of the ES cell lines tested expressed the stem cell markers ECMA-7 and alkaline phosphatase, which were lost on removal of LIF when the ES cells differentiated into a variety of cell types. The full developmental potential of the ES cells was determined by injecting cells from two of the independently derived ES cell lines, MBL-1 and MBL-5, into C57BL/6J blastocysts. A high proportion of the pups born were chimeric as judged by coat pigmentation. Subsequent breeding established that the ES cells had contributed to the germ line. These results demonstrate that feeder cells are not essential for the isolation of pluripotent ES cell lines.     

小鼠胚胎干细胞的培养

目的:建立小鼠胚胎干细胞(embryonic stem cells,ES)的培养方法。方法:制备G418抗性的原代小鼠胚胎成纤维细胞,经丝裂霉素C处理后成滋养层细胞,将小鼠胚胎干细胞复苏后,应用含白血病抑制因子的ES细胞培养液,培养小鼠ES细胞,观察集落的生长情况,并在光镜下观察细胞形态。结果:小鼠胚胎成纤维细胞生长良好,ES细胞呈克隆状生长,且保持未分化状态。结论:建立了小鼠胚胎干细胞培养的有效方法,为下一步基因打靶奠定基础。     

鸡胚胎干细胞的分离、培养和鉴定

SNL cells (permanent line of irradiated mouse fibroblast cells), primary mice embryonic fibroblasts (PMEF) cells and primary chicken embryonic fibroblasts (PCEF) cells were respectively used as the feeder cells for chicken embryonic stem cell culture. The isolated blastoderm cells front the stage X embryos of chicken were cultured in Dulercco‘‘ s Modified Eagle Medium (DMEM) supplemented with leukemia inhibitory factor (LIF, 1 000 IU/ml), basic fibroblast growth factor (bFGF 10 ng/ml) and stem cell factor (SCF, 5 ng/ml). The alkaline phosphatase (AKP) test, differentiation experiment in vitro and chimeric chicken production were carried out. The resuts showed that culture on feeder layer of PMEF yielded high quality CES cell colonies. The shape of typical CES clone showed as follows: nested aggregation (clone) with clear edge and round surface as well as close arrangement within the clone. Strong positive AKP reactive cellswere observed. On the other hand, the fourth passage CES cells could differentiate into various cells in the absence of feeder layer cells and LIF in vitro. The third and fourth passage cells were injected into the subgerminal cavity of recipient embryos at stage X. The manipulated embryos were incubated until hatching. Of 269 Hailan embryos injected with CES cells of Shouguang Chickens, 8.2 % (22/269) survived to hatching, 3 feather chimeras had been produced, which suggests that an effective culture systems were established and it could promote the growth of CES cells and maintain them in an undifferentiated state .     

Establishment of a germ-line competent C57BL/6 embryonic stem cell line

Embryonic stem (ES) cell lines have been derived from blastocysts of the inbred mouse strain C57BL/6. The highest frequencies of ES cell colonies were observed when blastocysts were explanted directly onto growth-arrested feeder layers of 5637 human bladder carcinoma cells in the presence of conditioned medium. One of the male ES cell lines tested (BL/6-III) was shown to be karyotypically stable and germ-line competent when introduced into BALB/c host blastocysts. These results demonstrate that ES cell lines from inbred mouse strains other than 129/Sv may be used as vectors to introduce selected mutations into the germ-line of mice.     

Effect of leukemia inhibitory factor (LIF) on in vitro produced bovine embryos and their outgrowth colonies

In vitro produced (IVP) bovine embryos were subjected to in vitro culture with or without 1000 U/ml human recombinant leukemia inhibitory factor (LIF) added to the culture medium from Days 5 to 8 post insemination (p.i.). Resulting blastocysts were subsequently plated intact on mouse feeder cells in a medium with or without LIF. Significantly more embryos reached the hatched blastocyst stage, and the number of blastocysts with excellent morphology was significantly higher, when LIF was omitted. At Day 8 p.i., total cell count (TCC) and inner cell mass (ICM) cell count was significantly higher in embryos cultured without LIF. In embryos cultured with LIF, cytoplasmic vesicles and lipid droplets were abundant and a decreased expression of both Oct4 and laminin could be observed. Initial hypoblast formation was revealed in almost 1/3 of the LIF-cultured blastocysts whereas this feature was evident in 2/3 of the blastocysts cultured in the absence of LIF. Overall, almost 60% of the blastocysts cultured without LIF formed outgrowth colonies (OCs) when plated on feeders, whereas this phenomenon was only observed in 30% of the blastocysts cultured in the presence of LIF. A tendency for retaining a tightly packed central growth of putative ICM-derived cells was observed, when attachment to the feeder layer was initiated close to the embryonic pole of the blastocyst. At Day 8 of outgrowth culture, approximately 20% of the colonies contained a central core of putative ICM-derived cells appearing large enough for mechanical isolation and further subculture. Immunohistochemical labeling for Oct4 revealed staining of both trophectodermal and ICM-derived cells. The presence of LIF in the outgrowth culture medium did not have any apparent effect on the plating efficiency or colony type. In conclusion, LIF had an adverse effect on in vitro embryonic development when added to the culture medium in the period from Days 5 to 8 p.i., whereas it had no apparent effect on the OCs subsequently formed from such embryos.