共查询到17条相似文献,搜索用时 203 毫秒
1.
山羊类ES细胞的分离与克隆 总被引:6,自引:0,他引:6
采集山羊交配后6~8d的桑椹胚、囊胚和孵化囊胚,将桑椹胚和囊胚分别放在小鼠原代胎儿成纤维细胞(PMEF)饲养层和同源原代胎儿成纤维细胞(PGEF)饲养层上比较其脱带时间及脱带率。脱带后,将各自一半胚胎切割,把含ICM的半胚分别放在相应饲养层上进行培养,另一半整胚在各自饲养层上继续培养,而孵化囊胚直接于PGEF饲养层上培养。当ICM增殖一定程度时进行传代,以比较其类ES细胞分离与克隆的效果。结果表明,在2种不同饲养层上,囊胚的脱带时间均短于桑椹胚,囊胚的脱带率均高于桑椹胚,而饲养层的种类对胚胎的脱带时间以及脱带率影响不大。脱带切割囊胚不论在PMEF还是在PGEF饲养层上,其贴壁时间均短于脱带整胚及孵化囊胚,而贴壁率高于脱带整胚,与孵化囊胚相似。脱带整胚及脱带切割胚在PMEF饲养层上所获类ES细胞只能维持3代,而在PGEF饲养层上,脱带切割半胚和孵化囊胚所获类ES细胞传至5代。由此认为,对脱带后的胚胎进行切割处理,有利于ICM的贴壁和增殖;应用同源原代胎儿成纤维细胞饲养层培养系统,有利于类ES细胞的分离与克隆。 相似文献
2.
为了提高猪孤雌囊胚贴壁率,试验从饲养层及培养液两方面研究猪孤雌囊胚贴壁能力;用小鼠、猪和牛的胎儿成纤维细胞制作饲养层,分别添加DMEM、NCSU-23、DMEM/NCSU-23培养液,探讨猪孤雌囊胚在3种饲养层上的发育效果。结果表明,BEF饲养层能更好地促进猪孤雌囊胚贴壁生长,其囊胚贴壁率为33.67%,与MEF饲养层组的囊胚贴壁率(19.08%)之间差异显著(P0.05),与PEF饲养层组之间囊胚贴壁率差异不显著(P0.05),MEF饲养层组和PEF饲养层组之间囊胚贴壁率差异不显著(P0.05);在BEF牛胎儿成纤维细胞饲养层组,用猪胚胎培养液NCSU-23培养猪孤雌囊胚后,囊胚贴壁率(22.53%)显著高于DMEM培养液组(10.41%)和DMEM/NCSU-23培养液半量混合组(12.05%)(P0.05),DMEM培养液组和DMEM/NCSU-23培养液半量混合组之间差异不显著(P0.05)。牛胎儿成纤维细胞饲养层和猪胚胎培养液NCSU-23能更好地促进猪孤雌囊胚后期贴壁。 相似文献
3.
以昆明系小鼠为对象,经过丝裂霉C处理成纤维细胞(Mouse embryonic fibroblast,MEF)制备饲养层,对影响小鼠胚胎干细胞(Embryonic stem cell,ES细胞)分离培养的相关因素进行研究。分别收集小鼠3.5d的囊胚(扩张囊胚)和4.5d囊胚(孵化囊胚)进行培养,比较扩张囊胚和孵化囊胚的贴壁率、原代克隆率及传代率的情况。收集3.5d胚龄的囊胚,通过全胚法和免疫外科法对内细胞团(Inner cell mass,ICM)进行分离培养ICM集落,确定离散ICM的适宜时间。用0.25%胰酶+0.04%EDTA,0.125%胰酶+0.02%EDTA和0.25%胰酶+1%小鸡血清等方法对小鼠ES细胞集落进行传代,观察不同酶浓度对ES细胞分离克隆的影响。结果显示,孵化囊胚的贴壁率高于扩张囊胚(P0.05),但传代率则相反(P0.05),原代克隆率差异不显著(P0.05);一般ICM增殖培养2~3d(免疫外科法)或4~5d(全胚培养法)后,出现典型的克隆集落,再挑取ICM;0.125%胰酶+0.02%EDTA及0.25%胰酶+1%小鸡血清,形成ES原代克隆率较高,2组没有显著性差异(P0.05);结果表明,分离得到的ES细胞经形态学观察,AKP染色,体外分化试验等表明其具有胚胎干细胞的特性。 相似文献
4.
系统地掌握猪早期胚胎体内外发育规律是进行猪胚胎冷冻、胚胎分割、鲜胚移值、长途运输引种以及基因转移等生物技术研究和应用的基础。本研究包括2个实验,实验1,利用89头超排母猪和19头自然发情母猪,于配种后第2、3、4、5、6、7、8、9和10天手术采得胚胎1612枚,系统地观察猪早期胚胎体内发育规律,即:2日龄胚胎中原核胚占77.39%(397/513),3日龄胚胎中4和6细胞胚占79.05%(83/105),4日龄胚胎中4~8细胞占40%(35/76),5日龄胚胎多为桑椹和囊胚83.12%(64/77),6日龄胚多为膨胀囊胚42.09%(181/430)和孵化囊胚34.19%(147/430),7和8、9、10日龄胚发育到孵化囊胚分别为76.34/oo(71/93)和100%(77/77),而自然发情的5日龄胚胎中桑椹和囊胚仅占32.5%(13/40),6日龄胚胎中膨胀囊胚仅占11.11%(17/153),孵化胚仅占19.61%(30/153)。各发育阶段的胚胎比例均明显低于5、6日龄超排供体(P<0.05)。实地2,将138枚囊胚和膨胀囊胚,分别体外培养24和12小时,囊胚发育阶段的胚胎50%(48/96)? 相似文献
5.
6.
通过在鸭胚上增殖规律的研究,证实了鸡减蛋综合症病毒在尿囊腔接种10日龄鸭胚,接种后24h以前病毒未增殖,24h后才开始增殖,120h ,病毒增殖到高峰,以后随时间延长下跌;同时还表明,鸡减蛋综合症病毒在尿囊膜、尿囊液、羊水中含量较高,病毒纯化及其他研究提供了依据。 相似文献
7.
小鼠胚胎成纤维细胞的分离和饲养层细胞的制备 总被引:11,自引:0,他引:11
通过实验确定分离小鼠胚胎成纤维细胞的最适胚龄,探讨小鼠胚胎成纤维细胞饲养层的效果及其寿命。结果表明,从10 、11 d 小鼠胚胎所获的胚胎成纤维细胞中混有大量神经母细胞和红细胞;用14 、15 d 的胚胎则基本不能获得胚胎成纤维细胞;消化3 ~4 个12 ~13 d 胚胎所获细胞悬液可接种8~9 个25 cm2 的培养瓶。从一只孕鼠的所有胚胎所获的成纤维细胞可接种约20 个25 cm2 的培养瓶。所获细胞悬液的活细胞百分率可达90% ,接种成活率达85 % 。胚胎成纤维细胞贴壁时间为5~6 h ,12 h 后进入增殖期,48 h 形成细胞单层。ES细胞克隆在小鼠胚胎成纤维细胞饲养层上形态典型、增殖迅速、不分化。饲养层寿命可维持2 ~3 周。 相似文献
8.
9.
采集家兔自然交配后96h的早期囊胚,以低糖DMEM+150mL/L胎牛血清+0.1mmol/L非必需氨基酸+100IU/mL青霉素+100IU/mL链霉素为基础培养基,比较了不同胚胎处理方法、不同饲养层以及培养液中添加不同成分对兔早期囊胚贴壁和增殖的影响,以完善兔胚胎干细胞的建系方法。结果表明,以胚胎分割法和链霉蛋白酶-E(proteinaseE)处理掉黏蛋白及部分透明带的胚胎容易贴壁和增殖;在小鼠成纤维细胞饲养层和兔胎儿成纤维细胞饲养层上,胚胎的脱带率差别不大,但在小鼠成纤维细胞饲养层上贴壁率明显提高,且贴壁后内细胞团增殖较快;添加胰岛素、白血病抑制因子和伊巯基乙醇均利于抑制ES的分化和促进内细胞团的增殖。 相似文献
10.
昆明系小鼠饲养层细胞制备条件的优化 总被引:2,自引:0,他引:2
通过分离不同胚龄的小鼠胚胎成纤维细胞(MEF),对MEF进行连续传代培养,并对MEF不同的消化时间进行探讨,研究影响小鼠胚胎成纤维细胞分离与培养的因素.结果表明,分离小鼠胚胎成纤维细胞的最适胚龄是12.5 d~14.5 d;37℃条件下,用2.5 g/L胰蛋白酶作用PMEF,作用时间不应超过15min;离散贴壁的成纤维细胞,作用时间以2 min~3 min为宜;MEF在第2代~第5代增殖旺盛,7代以后细胞出现急剧下降.所以选择第3代MEF是制做饲养层的最佳时机.MEF分离方法简单,来源方便,增殖迅速,是用于胚胎干细胞分离培养的有效培养体系. 相似文献
11.
以猪孤雌激活囊胚为材料,囊胚透明带消化后采用全胚培养,培养液中添加不同培养成分或因子(如FGF2,LIF,2i等),以及选择不同的初始培养液体积来筛选猪胚胎干细胞(embryonic stem cell,ES细胞)建系的优化培养体系。囊胚内细胞团形成的细胞集落采用胰酶消化传代。结果显示:透明带消化后,囊胚贴壁率显著升高(19.4%VS.8.8%)(P〈0.05);初始培养液体积比平常培养液体积(0.30mL/孔,24孔培养板)减半条件下,能显著提高其贴壁率(91.7%VS 20.0%)(P〈0.01),而且获得了可传至7代的类ES细胞系2株,碱性磷酸酶染色成阳性;当用2i因子(CHIR99021和PD03025901)去替代培养液中的FGF2,囊胚贴壁率(29.400VS53.3%)和原代集落形成率(20.0%VS 87.5%)反而显著下降(P〈0.01)。这表明培养液添加了FGF2和LIF(不舍2i因子),用24孔板培养,最初培养体积为0.15mL,透明带消化的培养体系比较适合猪孤雌激活胚的ES细胞建系。 相似文献
12.
The standard washing and trypsin treatment procedures to remove viruses adhering to the zona pellucida (ZP) were evaluated. Mouse embryos at the early blastocyst stage were exposed to Sendai virus, and then washed or treated with trypsin. Even after washing or trypsin treatment, Sendai virus was detected in the twelfth and final wash. The virus was still shown to adhere to the ZP by immunofluorescence assay. The embryos developed into expanded blastocysts following 24 hours of in vitro culture. Viral antigen was clearly demonstrated in the cells forming the expanded blastocysts, indicating that viral replication occurred in these cells. The present results suggest that the standard washing or trypsin treatment are not sufficient to remove Sendai virus adhering to the ZP of mouse embryos. 相似文献
13.
The objective of this study was to use mouse embryos as a model system to investigate the effect of co-culture of cumulus cells in Sydney IVF sequential media (Cook) on embryo development, based on the hypothesis that feeder cells in co-culture with a sequential medium could work synergistically to further improve in vitro culture conditions for mammalian preimplantation embryos. The culture systems described here were evaluated by the ability to consistently produce high blastocyst formation rates and high cell number per blastocyst. The role of embryo-to-cell contact was assessed by using Transwell inserts with transparent microporous membranes. Pronuclear embryos of ICR mice were cultured to blastocysts in Cook sequential media, with and without mouse primary cultures of cumulus cells, and with or without inserts. Blastocyst formation rates and cell numbers of in vitro developing embryos in the different culture systems were compared to each other, and to in vivo derived blastocysts. Blastocyst formation rates for Cook medium only was 27.8% (without inserts) and 32.9% (with inserts), whereas Cook-Cumulus cells in identical culture systems was significantly higher at 45.8% (without inserts, P<0.05) and 55.6% (with inserts, P<0.05). When the embryos are suspended above the bottom of the well, for Cook medium significantly lower blastocyst formation rates were observed at 4.2% compared to Cook-Cumulus cells at 17.5% (P<0.05). Mean cell numbers of blastocysts obtained in all co-culture systems were significantly higher (P<0.05) compared to those developing in culture medium only. Although the putative mechanism is as yet unexplained, the improved blastocyst formation rates and cell numbers in co-culture when there is direct contact between the embryo and the cell monolayer suggest that the close proximity between the feeder cells and embryos is in part responsible for these effects. 相似文献
14.
T. OTOI N. KOYAMA K. YAMAMOTO N. HORIKITA S. TACHIKAWA T. SUZUKI 《Veterinary journal (London, England : 1997)》2000,159(3):392-286
Two-hundred-and-thirty-one fair-quality embryos at the compacted morula stage collected from 89 superovulated cows were cultured in TCM199 or Brinster's BMOC-3 medium with or without 100 microM beta-mercaptoethanol (beta-ME). After 24 h culture, a total of 142 fair-quality embryos developed to the blastocyst stage, of which 106 were subsequently frozen with 1.8 M ethylene glycol. The mean cell number and development rates of frozen-thawed blastocysts from the fair-quality embryos cultured in TCM199 containing beta-ME were higher than those of the fair-quality embryos directly frozen without culture. The pregnancy rates obtained with frozen blastocysts from fair-quality embryos tended to be lower than those of non-cultured fresh fair-quality embryos and cultured fresh blastocysts. These results indicate that the inclusion of beta-ME in pre-freezing culture media improve the development of frozen-thawed blastocysts from fair-quality embryos, but not the pregnancy rate. 相似文献
15.
Otoi T Koyama N Yamamoto K Horikita N Tachikawa S Suzuki T 《Veterinary journal (London, England : 1997)》2000,159(3):282-286
Two-hundred-and-thirty-one fair-quality embryos at the compacted morula stage collected from 89 superovulated cows were cultured in TCM199 or Brinster's BMOC-3 medium with or without 100 microM beta-mercaptoethanol (beta-ME). After 24 h culture, a total of 142 fair-quality embryos developed to the blastocyst stage, of which 106 were subsequently frozen with 1.8 M ethylene glycol. The mean cell number and development rates of frozen-thawed blastocysts from the fair-quality embryos cultured in TCM199 containing beta-ME were higher than those of the fair-quality embryos directly frozen without culture. The pregnancy rates obtained with frozen blastocysts from fair-quality embryos tended to be lower than those of non-cultured fresh fair-quality embryos and cultured fresh blastocysts. These results indicate that the inclusion of beta-ME in pre-freezing culture media improve the development of frozen-thawed blastocysts from fair-quality embryos, but not the pregnancy rate. 相似文献
16.
ICR小鼠胚胎干细胞建系初步研究 总被引:1,自引:0,他引:1
实验旨在探讨消化方式和胚胎发育阶段对ICR小鼠胚胎干细胞(ES细胞)建系效率的影响。ICR小鼠3.5 d囊胚在饲养层上贴壁后采用单一酶消化或机械化与酶消化法相结合分离隆起的细胞集落,进行传代培养;然后选择二者中较优消化方式对不同发育时期囊胚所形成的细胞集落进行处理。结果表明:采用机械化与胰酶消化相结合的方式,形成的类ES细胞超过7代的比率(85.0%)要显著高于单一的胰酶消化(15.0%)(P<0.05);当用二者相结合的方式对ICR小鼠3.5 d(早期囊胚)、4.0 d(扩张囊胚)和4.5 d(孵化囊胚)所形成的细胞集落进行消化传代培养,三者在贴壁率和形成原代细胞集落率上均无显著差别(P>0.05),但传代超过7代的效率上早期囊胚和扩张囊胚均高于孵化囊胚(P<0.05)。结果提示,采用机械化与酶消化法相结合更适合于3.5~4.0 d ICR小鼠囊胚的ES细胞建系。 相似文献
17.
Soo-Kyung Jung Hyun-Jung Kim Chan-Lan Kim Joo-Hyeong Lee Jin-Young You Eun-Song Lee Jeong-Mook Lim Seon Jong Yun Jae-Young Song Sang-Ho Cha 《Journal of veterinary science (Suw?n-si, Korea)》2014,15(4):519-528
The present study was conducted to develop an effective method for establishment of porcine parthenogenetic embryonic stem cells (ppESCs) from parthenogenetically activated oocyte-derived blastocysts. The addition of 10% fetal bovine serum (FBS) to the medium on the 3rd day of oocyte culturing improved the development of blastocysts, attachment of inner cell masses (ICMs) onto feeder cells, and formation of primitive ppESC colonies. ICM attachment was further enhanced by basic fibroblast growth factor, stem cell factor, and leukemia inhibitory factor. From these attached ICMs, seven ppESC lines were established. ppESC pluripotency was verified by strong enzymatic alkaline phosphatase activity and the expression of pluripotent markers OCT3/4, Nanog, and SSEA4. Moreover, the ppESCs were induced to form an embryoid body and teratoma. Differentiation into three germ layers (ectoderm, mesoderm, and endoderm) was confirmed by the expression of specific markers for the layers and histological analysis. In conclusion, data from the present study suggested that our modified culture conditions using FBS and cytokines are highly useful for improving the generation of pluripotent ppESCs. 相似文献