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Novel sericin-based hepatocyte serum-free medium and sericin's effect on hepatocyte transcriptome
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作者 Yun Huang Qing Peng +3 位作者 Hai-Yan Li Zhi-Dong Jia Yang Li Yi Gao 《World Journal of Gastroenterology》 SCIE CAS 2018年第30期3398-3413,共16页
AIM To develop a novel hepatocyte serum-free medium based on sericin,and to explore the effect of sericin on the hepatocyte transcriptome.METHODS A controlled trial comparing novel serum-free medium and other media: C... AIM To develop a novel hepatocyte serum-free medium based on sericin,and to explore the effect of sericin on the hepatocyte transcriptome.METHODS A controlled trial comparing novel serum-free medium and other media: C3 A cells were cultured in our novel serum-free medium,Hepato ZYME,complete medium(DMEM/F12 with 100 m L/L FBS),and DMEM/F12,andthen cell attachment,proliferation,and function as well as the biocompatibility of the media were assessed.A comparative study of serum-free media with or without 2 mg/m L sericin: the effect of sericin on C3 A growth was assessed by cell viability and proliferation,the effect of sericin on C3 A cell cycle distribution was determined by flow cytometry,and the effect of sericin on the C3 A transcriptome was assessed by gene-chip array and RT-q PCR.RESULTS More C3 A cells attached to the plate containing our serum-free medium than to those containing Hepato ZYME and DMEM/F12 at 24 h post-seeding.Both the viability and proliferation rate of C3 A cells in sericin-based serum-free medium were superior to those of cells in Hepato ZYME and DMEM/F12(P < 0.001).The content of albumin and urea in our serum-free medium was significantly higher than that in Hepato ZYME and DMEM/F12 throughout the whole culture period(P < 0.001) and was similar to that in complete medium at day 3,4,and 5.In part 2,cell viability and proliferation were greater in the presence of 2 mg/m L sericin(P < 0.001),as was the proportion of cells in S phase(16.21% ± 0.98% vs 12.61% ± 0.90%,P < 0.01).Gene-chip array analysis indicated that the expression of CCR6,EGFR,and FOS were up-regulated by 2 mg/m L sericin,and RT-q PCR revealed that the expression of CCR6,EGFR,FOS,AKT1,JNK1,NFk B1,MMP-9,MEK2,ERK1/2 and MYC was upregulated by 2 mg/m L sericin(P < 0.05).CONCLUSION We developed a novel hepatocyte serum-free medium.Sericin probably enhances cell attachment through the CCR6-Akt-JNK-NF-κB pathway and promotes cell proliferation through CCR6-mediated activation of the ERK1/2-MAPK pathway. 展开更多
关键词 SERICIN serum-free medium MAPK pathway Bioartificial liver support system CCR6
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Some biological characteristics of hybridomas and parental myelomas cultivated in serum-free medium for long-term period
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作者 李纪良 李英杰 +2 位作者 巢穗 欧阳明辉 彭一兵 《Journal of Medical Colleges of PLA(China)》 CAS 1992年第3期246-250,共5页
It has been developed in this laboratory that a serum-free medium, designated asDMI,is adaptive for long-term culture,freezing and resurgence in liquid nitrogen,and cloningof hybridoma and parental myelomas as well as... It has been developed in this laboratory that a serum-free medium, designated asDMI,is adaptive for long-term culture,freezing and resurgence in liquid nitrogen,and cloningof hybridoma and parental myelomas as well as for cell fusions.In this report,it is describedthat the myeloma cells grown in DMI for more than 3 months maintained their biological charac-teristics such as induction of aseites and subcutaneous somatic tumor in BALB/c mice and toler-ance toward 8-azaguanine,ete..However,the ability of the tumor cells to attach to glass wallwas decreased.The selecting assay of these cells in HAT medium(medium containing hypoxan-thine,aminopterin and thymidine)showed that the death time in DMI was similar to that in theconventional 15% newborn calf serum-supplemented medium(RPS15).The hybridoma cellsadapted in DMI secrete monoclonal antibodies in quantities comparable to those produced inRPS15. 展开更多
关键词 MYELOMA HYBRIDOMA serum-free medium MONOCLONAL antibody
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Cholesterol requirement for growth of rodent parental myeloma cells in serum-free medium
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作者 李纪良 李英杰 +4 位作者 林来兴妹 欧阳明辉 巢穗 彭一兵 常文生 《Journal of Medical Colleges of PLA(China)》 CAS 1991年第2期135-140,共6页
Cholesterol,a major lipid component of plasma membrane,is thoughtto have profound effects on the structure and function of cells.Mostanimal tis-sues are capable of synthesizing cholesterol de novo from acetate;however... Cholesterol,a major lipid component of plasma membrane,is thoughtto have profound effects on the structure and function of cells.Mostanimal tis-sues are capable of synthesizing cholesterol de novo from acetate;however,thereare relatively few mammalian cells in vitro expressing an absolute requirement foran exogenous source of cholesterol.In this paper,it was shown that IR983F(983)rat myeloma cells and P3X63-AgS-U1(P3U1)and P3X63-Ag8.653(653)mousemy eloma cells which had been cultivated in serum-free medium for more than 6months required cholesterol in vitro for growth in serum-free medium.Optimalgrowth of P3U1,653 and 983 occurred in cholesterol concentration of 5,10 and15μg/ml,respectively.Moreover,it was demonstrated that the cholesterol couldbe replaced by human low density lipoprotein in a concentration of 10μg/ml butnot by mevalonic acid lactone.In contrast to the parental myeloma cells,hybridoma cells derived from the mouse myeloma cells which had been cultivatedin serum-free medium for more than 6 months did not require cholesterol. 展开更多
关键词 CHOLESTEROL serum-free medium MYELOMA
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Pilot-Scale Production of Lyophilized Inactivated Rabies Vaccine Candidate in Vero Cells under Fully Animal Component-Free Conditions Using Microcarrier Technology and Laboratory Animal Trials
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作者 Engin Alp Onen Srinivas Bezawada 《Journal of Biomedical Science and Engineering》 2022年第6期157-178,共22页
The upstream process was carried out in an animal component-free medium on Cytodex 1 microcarriers. Recombinant trypsin is a non-animal derived protease used as an alternative to animal-derived trypsin. To inactivate ... The upstream process was carried out in an animal component-free medium on Cytodex 1 microcarriers. Recombinant trypsin is a non-animal derived protease used as an alternative to animal-derived trypsin. To inactivate recombinant trypsin, a soybean trypsin inhibitor (STI) should be added to the medium. A protocol was first tested in T-flasks and then passaged to 500 mL and 3 L spinner flasks. Cell detachment was completed in 10 - 12 min, and 0.4 g/L STI was added to a 3L spinner, and cells were transferred into a 30 L stirred tank bioreactor. On day 5, the cell density had reached its maximum (around 1.8 × 106 cells/mL). At an MOI of 0.3 with serum-free medium conditions, cell infection yielded a maximal rabies virus titer of 1.82 × 10<sup>7</sup> FFU/mL at 5 days. All cell culture conditions and virus growth kinetics in serum-free media were investigated. In conclusion, Vero cells were grown on Cytodex 1 with serum-free media and a high amount of rabies virus was obtained. A mouse challenge was used to determine the immune response to an inactivated rabies virus vaccine candidate. Also, we evaluated inactive rabies vaccine candidate safety, and immunogenicity in mice, sheep, horses, and cattle. We found that no horses, sheep, or cattle who were given vaccine IM at 3.2 IU/dose exhibited any clinical sign of disease and all developed high VNA titers (up to 10.03 IU/mL) by 3 - 4 WPI. After the accelerated stability studies, the lyophilized inactivated rabies vaccine candidate showed enough antigenic potency (2.6 IU/mL) in the mouse challenge test. Also, 18-month long-term stability studies showed enough immune response (1.93 IU/mL) on day 14. The activity of the vaccine candidate showed a good immune response and safety criteria that meet WHO requirements. This is the first pilot-scale mammalian cell-based viral rabies vaccine production study in Türkiye that used microcarriers. 展开更多
关键词 LYSSAVIRUS RABIES VIROLOGY Inactivated Vaccine Potency Test MICROCARRIERS TEM Analysis Vero Cell Culture serum-free medium Non-Animal Derived Recombinant Trypsin Preclinical Trials
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多孔微载体无血清培养rCHO细胞生产u-PA 被引量:17
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作者 胡显文 肖成祖 +5 位作者 李佐虎 郭志霞 高丽华 张正光 胥照平 王菲 《生物工程学报》 CAS CSCD 北大核心 2000年第3期387-391,共5页
在 30L搅拌式反应器中无血清培养分泌尿激酶型纤溶酶原激活剂 (u PA)的DNA重组CHO细胞 ,定期部分更换Cytopore多孔微载体 ,使生长在多孔微载体中的细胞不断更新繁殖 ,解决大规模细胞培养中的细胞凋亡问题。在 91d连接换液培养过程中 ,... 在 30L搅拌式反应器中无血清培养分泌尿激酶型纤溶酶原激活剂 (u PA)的DNA重组CHO细胞 ,定期部分更换Cytopore多孔微载体 ,使生长在多孔微载体中的细胞不断更新繁殖 ,解决大规模细胞培养中的细胞凋亡问题。在 91d连接换液培养过程中 ,细胞密度可维持在 (1 3~ 2 6 )× 10 7/mL ,活细胞比率维持在 90 %以上。在7 5L搅拌罐中培养细胞 ,利用外部周期性压力振荡刺激并结合载体更新技术 ,可减轻密度效应对细胞生长和表达的影响 ,在一定程度上提高细胞在高密度培养条件下的表达水平。在 6 7d连续换液培养中 ,细胞最高密度为 2 6 4× 10 7/mL ,活细胞比率维持在 95 %以上。与稳压操作相比 ,利用周期变压刺激技术可提高产量 10 %~ 2 0 % ,且可降低葡萄糖厌氧代谢生成乳酸的转化率 ,利用 4步纯化工艺 ,从含u PA约 135g的 2 10 0L上清中获得约 80 gu PA(单链比例约为 90 % )。 展开更多
关键词 动物细胞培养 微载体更新 U-PA RCHO细胞
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MDCK细胞无血清悬浮培养技术在流感疫苗研究与生产中的应用进展
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作者 靳莉武 张震宇 +4 位作者 靳冬武 马花 马玉梅 乔自林 王家敏 《生物技术通报》 CAS CSCD 北大核心 2024年第2期38-47,共10页
流感是一种常见的呼吸道疾病,由流感病毒引起,接种疫苗是预防流感的有效手段。MDCK细胞(Madin-Darby Canine Kidney Cells)具有易于培养和高产量的特点,可以支持流感病毒的复制和增殖,被广泛用于流感疫苗的研究和生产。随着对流感病毒... 流感是一种常见的呼吸道疾病,由流感病毒引起,接种疫苗是预防流感的有效手段。MDCK细胞(Madin-Darby Canine Kidney Cells)具有易于培养和高产量的特点,可以支持流感病毒的复制和增殖,被广泛用于流感疫苗的研究和生产。随着对流感病毒研究的不断深入,为了进一步拓展MDCK细胞用于流感病毒研究和工业应用的能力,研究人员开始发展MDCK细胞无血清全悬浮培养技术。通过长期的培养和优化,驯化的MDCK悬浮细胞株可以更好地适应流感病毒的生长环境,提高流感病毒的产量和感染性。总之,MDCK细胞无血清悬浮培养技术在流感病毒研究和工业应用中发挥着重要作用,为流感疫苗生产和抗流感药物研发提供更好的工具。同时也必须重视MDCK细胞的安全性,采取合适的措施来确保其应用的安全性和可靠性。 展开更多
关键词 MDCK细胞 细胞悬浮驯化 无血清培养基 流感疫苗 安全性
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A-NK细胞培养和活化方法的改进 被引量:9
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作者 王志华 王贺元 +1 位作者 张彦 吴长有 《中国免疫学杂志》 CAS CSCD 北大核心 2005年第6期431-434,共4页
目的:比较A-NK细胞在完全培养基(CM)和无血清培养基(AIMV)中体外扩增及杀伤肿瘤细胞作用,同时探讨IL-12对于A-NK/IL-2治疗的辅助作用及其杀伤的形态学观察。方法:用MTT法比较不同培养条件下的A-NK细胞体外增殖能力,并测定细胞体外杀伤... 目的:比较A-NK细胞在完全培养基(CM)和无血清培养基(AIMV)中体外扩增及杀伤肿瘤细胞作用,同时探讨IL-12对于A-NK/IL-2治疗的辅助作用及其杀伤的形态学观察。方法:用MTT法比较不同培养条件下的A-NK细胞体外增殖能力,并测定细胞体外杀伤肿瘤细胞的活性。通过做扫描和透射电镜,对A-NK细胞杀伤的肿瘤细胞进行形态学观察。结果:不同培养条件下的A-NK细胞均可在短期内大量扩增(P<0.05),且均有很强的杀伤肿瘤的活性(P<0.05)。被A-NK细胞杀伤的肿瘤细胞的死亡形式是溶解坏死(necrosis)和凋亡(apoptosis)。结论:AIMV可替代CM用于A-NK细胞的培养。联合应用IL-12和IL-2激活A-NK细胞优于单独使用IL-2,可减轻高剂量IL-2带来的副作用。此研究为A-NK细胞的实验室研究和将来临床应用推广奠定了新的实验基础。 展开更多
关键词 A-NK AIMV IL-12 MTT
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小鼠骨髓内皮细胞条件培养液复合FL及TPO对HPP-CFC及CFU-GM增殖的影响 被引量:5
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作者 那晓东 王绮如 《生理学报》 CAS CSCD 北大核心 2001年第4期316-320,共5页
通过传代培养小鼠骨髓内皮细胞 ,收集无血清条件培养液 (ECM) ,并经超滤得到大于 10kD的浓缩液 ,分别观察ECM和大于 10kD的浓缩液复合flt3ligand (FL)及thrombopoietin (TPO)对体外培养HPP CFC、CFU GM的影响。结果表明 :ECM或大于 10k... 通过传代培养小鼠骨髓内皮细胞 ,收集无血清条件培养液 (ECM) ,并经超滤得到大于 10kD的浓缩液 ,分别观察ECM和大于 10kD的浓缩液复合flt3ligand (FL)及thrombopoietin (TPO)对体外培养HPP CFC、CFU GM的影响。结果表明 :ECM或大于 10kD的浓缩液对HPP CFC、CFU GM的生长均有支持作用 ;FL或 /和TPO与ECM或大于 10kD的浓缩液合用能加强对HPP CFC、CFU GM生长的刺激作用 ;FL加TPO与ECM或大于 10kD的浓缩液合用对HPP CFC、CFU GM生长的刺激作用更加明显 ;选择FL和TPO特异性的引物 ,用RT PCR技术未能检测到小鼠骨髓内皮细胞有FL和TPOmRNA的表达。 展开更多
关键词 骨髓内皮细胞 无血清条件培养液 造血调控 小鼠 祖细胞 CFU-GM
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无血清培养胆囊癌GBC-SD细胞形成肿瘤细胞球的鉴定 被引量:2
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作者 石程剑 秦仁义 +3 位作者 王敏 田锐 张志发 宫伟强 《世界华人消化杂志》 CAS 北大核心 2010年第9期865-870,共6页
目的:分离扩增肿瘤干细胞,并鉴定其生物学性质.方法:用无血清培养基培养人胆囊癌GBC-SD细胞得到肿瘤细胞球.将肿瘤细胞球传代扩增,并用含血清培养基培养促使其分化;将肿瘤球和普通GBC-SD细胞分别种入96孔板,MTT检测增殖能力,并将肿瘤球... 目的:分离扩增肿瘤干细胞,并鉴定其生物学性质.方法:用无血清培养基培养人胆囊癌GBC-SD细胞得到肿瘤细胞球.将肿瘤细胞球传代扩增,并用含血清培养基培养促使其分化;将肿瘤球和普通GBC-SD细胞分别种入96孔板,MTT检测增殖能力,并将肿瘤球和普通GBC-SD细胞分别植入裸鼠皮下,观察移植瘤的形成;流式细胞术检测CD15s和CD24在肿瘤球细胞和普通GBC-SD细胞中的表达,筛选细胞表面标志物.结果:在无血清培养基中,胆囊癌细胞可以形成少量的肿瘤细胞球,并显示很强的自我更新和增殖能力,含血清环境能够诱导其分化而贴壁生长;在动物实验中,肿瘤球细胞较普通GBC-SD细胞显示更强的致瘤能力(80.00%vs10.00%,P<0.05);标志物CD15s在肿瘤球的表达较普通GBC-SD细胞明显增高(2.56%±0.38%vs10.77%±0.93%,t=18.25,P<0.05).结论:人胆囊癌细胞GBC-SD的肿瘤干细胞可以通过无血清培养环境来分离和扩增,CD15s可能为其细胞表面标志物. 展开更多
关键词 胆囊癌 GBC-SD细胞系 无血清培养基 肿瘤干细胞 细胞表面标志物
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无血清培养基对体外激活的A-NK细胞的支持作用
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作者 蓝毓滨 王志华 张彦 《实用肿瘤学杂志》 CAS 2005年第6期405-407,共3页
目的多方面比较无血清培养基AIMV与完全培养基对体外细胞因子激活的NK细胞的支持作用。方法分别用AIMV及完全培养基培养粘附NK细胞(A-NK)和非粘附NK细胞(NA-NK),比较细胞的增殖能力、杀伤肿瘤细胞的能力、表达粘附分子CD11C的能力。结... 目的多方面比较无血清培养基AIMV与完全培养基对体外细胞因子激活的NK细胞的支持作用。方法分别用AIMV及完全培养基培养粘附NK细胞(A-NK)和非粘附NK细胞(NA-NK),比较细胞的增殖能力、杀伤肿瘤细胞的能力、表达粘附分子CD11C的能力。结果与完全培养基培养细胞相比,AIMV培养细胞增殖能力、杀伤肿瘤细胞的能力、表达CD11C的能力与之相当;在同一培养条件下A-NK细胞的增殖能力、杀伤活性高于NA-NK细胞。结论无血清培养基可替代完全培养基用于A-NK细胞的培养;A-NK细胞用于治疗肿瘤的过继免疫疗法要优于NA-NK细胞。 展开更多
关键词 粘附NK细胞 无血清培养基 细胞培养 四甲基偶氮唑盐比色法
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结肠癌Caco-2细胞株无血清培养技术研究
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作者 陈小燕 吴应强 +1 位作者 赵逵 朱蓉 《现代医药卫生》 2019年第2期176-178,共3页
目的探索人结肠癌Caco-2细胞株肿瘤干细胞的分选方法。方法应用无血清悬浮培养法培养Caco-2细胞,产生肿瘤细胞球,并对肿瘤细胞球从形态学、分化、自我更新及交替培养等方面进行鉴定。结果 Caco-2细胞在无血清培养基(SFM)中可存活,24 h... 目的探索人结肠癌Caco-2细胞株肿瘤干细胞的分选方法。方法应用无血清悬浮培养法培养Caco-2细胞,产生肿瘤细胞球,并对肿瘤细胞球从形态学、分化、自我更新及交替培养等方面进行鉴定。结果 Caco-2细胞在无血清培养基(SFM)中可存活,24 h后可产生少量体积较小松散的悬浮肿瘤球,肿瘤球体积随时间延长而增大;将肿瘤球接种于完全培养基中12 h后细胞贴壁生长,细胞形态与传统培养形成的单细胞层无明显差异,重新消化贴壁细胞后再次悬于SFM中24~72 h后仍可形成悬浮细胞球,其形态与原代相同。结论结肠癌Caco-2细胞在SFM中可生成悬浮肿瘤细胞球,采用无血清悬浮培养法可达到富集肿瘤干细胞的目的。 展开更多
关键词 培养基 无血清 结肠肿瘤 肿瘤干细胞 CACO-2细胞
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重组CHO-GS细胞降低氨毒副作用的代谢研究 被引量:2
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作者 张芳 易小萍 +1 位作者 孙祥明 张元兴 《生物工程学报》 CAS CSCD 北大核心 2006年第1期94-100,共7页
在重组CHOGS细胞无血清批培养过程中,由于GS系统的引入,使氨对细胞的毒副作用显著降低,从而引起细胞生长和代谢途径发生变化。当起始氨浓度为1.42mmolL时,细胞最高密度可达到15.6×105cellsmL,随着氨浓度的增加,尽管细胞生长受到一... 在重组CHOGS细胞无血清批培养过程中,由于GS系统的引入,使氨对细胞的毒副作用显著降低,从而引起细胞生长和代谢途径发生变化。当起始氨浓度为1.42mmolL时,细胞最高密度可达到15.6×105cellsmL,随着氨浓度的增加,尽管细胞生长受到一定的抑制,但在氨浓度为12.65mmolL时,细胞密度仍可达到8.9×105cellsmL。当起始氨浓度从0.36mmolL增加到12.65mmolL时,细胞对葡萄糖的得率系数和乳酸对葡萄糖的得率系数降低,己糖激酶(HK)、丙酮酸激酶(PK)和乳酸脱氢酶(LDH)酶活分别提高了43%、140%和25%,表明细胞对葡萄糖的利用增加,糖代谢更倾向于高能量生成途径。在谷氨酰胺代谢途径中,氨促进了谷丙转氨酶(GPT)酶活,谷氨酸到α酮戊二酸的转化逐渐倾向于谷丙转氨途径,谷氨酸脱氢酶(GDH)酶活降低,脱氨途径相应受到抑制。此外,氨浓度的增加使细胞群体处于G0G1期的比例逐渐升高,当氨浓度为12.65mmolL时,重组蛋白比生产速率比氨浓度为0.36mmolL时提高了2.1倍。 展开更多
关键词 重组CHO细胞 谷氨酰胺合成酶 无血清培养 代谢
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Mixture与响应面法结合开发BHK-21细胞无血清悬浮培养基 被引量:2
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作者 汪梁 刘旭平 谭文松 《生物技术通报》 CAS CSCD 北大核心 2015年第9期70-78,共9页
采用Mixture与响应面实验设计相结合的方法开发BHK-21细胞无血清悬浮培养基。在实验室已知配方的6种培养基A-F的基础上,通过Mixture实验筛选出BHK-21细胞无血清培养基的最优组合为A∶B∶C∶D∶E∶F=0∶0∶11∶0∶9∶0。利用响应面法针... 采用Mixture与响应面实验设计相结合的方法开发BHK-21细胞无血清悬浮培养基。在实验室已知配方的6种培养基A-F的基础上,通过Mixture实验筛选出BHK-21细胞无血清培养基的最优组合为A∶B∶C∶D∶E∶F=0∶0∶11∶0∶9∶0。利用响应面法针对培养基中的几种关键组分进行浓度优化,确定谷氨酰胺、酪氨酸、牛血清白蛋白和钙离子的最优浓度分别为3 mmol/L、2.5 g/L、0 g/L和0 mmol/L。该无血清悬浮培养基能很好地支持BHK细胞悬浮生长,培养时细胞最大活细胞密度可达140.21×105个/m L,比商业培养基提高了1.95倍。采用Mixture试验设计和响应面分析法能够在较短的时间内开发出适合BHK-21细胞生长的无血清悬浮培养基,为采用BHK-21细胞大规模工业化生产口蹄疫疫苗奠定了基础。 展开更多
关键词 BHK-21细胞 无血清悬浮培养基 Mixture实验设计 响应面分析
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人肺癌NCI-H446细胞生成肿瘤干细胞球 被引量:2
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作者 乐涵波 刘晓光 曾芳 《解剖学报》 CAS CSCD 北大核心 2012年第4期500-505,共6页
目的探索人肺癌NCI-H446细胞系干细胞球体的培养,并鉴定其生物学特性。方法用无血清培养基培养人肺癌NCI-H446细胞得到肿瘤细胞球。将肿瘤细胞球传代扩增,并用含血清培养基培养促使其分化;四甲基偶氮唑盐(MTT)比色检测肿瘤球和普通NCI-H... 目的探索人肺癌NCI-H446细胞系干细胞球体的培养,并鉴定其生物学特性。方法用无血清培养基培养人肺癌NCI-H446细胞得到肿瘤细胞球。将肿瘤细胞球传代扩增,并用含血清培养基培养促使其分化;四甲基偶氮唑盐(MTT)比色检测肿瘤球和普通NCI-H446细胞的增殖能力,并将肿瘤球和普通NCI-H446细胞分别植入裸鼠皮下,观察肿瘤形成;Transwell侵袭实验检测肿瘤球和普通NCI-H446细胞的侵袭能力的不同;流式细胞术检测CD133、CD44在肿瘤球和普通NCI-H446细胞中的表达,并筛选细胞表面标志物。结果在无血清培养基中,人肺癌NCI-H446细胞可以形成少量的肿瘤细胞球,并显示很强的自我更新和增殖能力,在含血清环境中能够诱导肿瘤球分化而贴壁生长;在动物实验中,接种5×105个细胞时,肿瘤球细胞较普通NCI-H446细胞显示更强的致瘤能力;在侵袭实验中,肿瘤球细胞的侵袭能力高于普通NCI-H446细胞;干细胞标志物CD133及CD44在肿瘤球细胞的表达较普通NCI-H446细胞明显增高。结论人肺癌细胞NCI-H446中存在癌干细胞,且可以通过无血清培养、分离和富集。 展开更多
关键词 肺癌 NCI-H446细胞系 无血清培养 癌干细胞 细胞表面标志 流式细胞术
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支持高密度BHK-21细胞培养和高产FMD病毒的无血清培养基开发与优化 被引量:2
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作者 陈敏 刘旭平 赵亮 《生物技术通报》 CAS CSCD 北大核心 2020年第10期62-71,共10页
优化无血清培养基,以实现BHK-21悬浮细胞的超高密度生长和口蹄疫病毒高效扩增。依据BHK-21细胞的代谢特点和动力学分析识别无血清培养基中的关键营养成分,优化组分浓度,对比优化前后细胞的生长和产毒能力,并在生物反应器中验证。优化后... 优化无血清培养基,以实现BHK-21悬浮细胞的超高密度生长和口蹄疫病毒高效扩增。依据BHK-21细胞的代谢特点和动力学分析识别无血清培养基中的关键营养成分,优化组分浓度,对比优化前后细胞的生长和产毒能力,并在生物反应器中验证。优化后的无血清培养基支持批培养模式下最高活细胞密度达到1.78×107 cells/mL,代谢副产物积累的情况得到改善;口蹄疫病毒TCID50与含低比例血清的培养基相比具有相似水平,约为7.25 lgTCID50/0.1mL;146s含量与低血清培养基相比提高50.7%,达到15.6μg/mL。以细胞的生长需求和代谢规律为基础,优化营养成分和降低代谢副产物积累能有效解除“细胞密度效应”,实现超高细胞密度接毒和高产口蹄疫病毒。 展开更多
关键词 BHK-21悬浮细胞 无血清培养基 高细胞密度 高产口蹄疫病毒
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STUDY ON REPRODUCTIVE ENDOCRINOLOGY OF HUMAN PLACENTA--CULTURE OF HIGHLY PURIFIED CYTOTROPHOBLAST CELL IN SERUM-FREE HORMONE SUPPLEMENTED MEDIUM 被引量:9
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作者 李荣皓 庄临之 《Science China Chemistry》 SCIE EI CAS 1991年第8期938-946,共9页
A new method of long-term culture of cytotrophoblast cells in serum-free medium has been developed. Cytotrophoblast cells were isolated with cold trypsin and purified by unit gravity sedimentation through BSA density ... A new method of long-term culture of cytotrophoblast cells in serum-free medium has been developed. Cytotrophoblast cells were isolated with cold trypsin and purified by unit gravity sedimentation through BSA density gradients. The cells were cultured in the FD medium with supplement of EGF, insulin, transferrin and sodium selenite. They could survive over three weeks. The results showed that both EGF and insulin stimulated hCG and progesterone secretion and that sodium selenite elevated hCG output but not progesterone secretion. Transferrin produced synergistic effect with EGF and insulin on hCG and progesterone secretion but it was ineffective when used alone. This study demonstrates that the four growth factors mentioned above are essential for the survival of cytotrophoblast cells in vitro. It is therefore suggested that EGF, insulin and selenium may possibly be involved in the regulation of hCG and progesterone secretion in the human placenta. 展开更多
关键词 CYTOTROPHOBLAST cell HORMONAL regulation serum-free medium growth factors.
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Enrichment of breast cancer stem cells using a keratinocyte serum-free medium 被引量:6
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作者 LIU Zhen-zhen CHEN Ping +2 位作者 LU Zhen-duo CUI Shu-de DONG Zi-ming 《Chinese Medical Journal》 SCIE CAS CSCD 2011年第18期2934-2936,共3页
Background Keratinoyte serum-free medium (K-SFM) is a defined medium used to support the growth of primary keratinocytes and embryonic stem cell. The aim of this research was to optimize enrichment of breast cancer ... Background Keratinoyte serum-free medium (K-SFM) is a defined medium used to support the growth of primary keratinocytes and embryonic stem cell. The aim of this research was to optimize enrichment of breast cancer stem cells (CSCs) using K-SFM. Methods' A K-SFM was used to enrich CSCs from two breast cancer cell lines and a primary culture of breast cancer. RPMI-1640 supplemented with 10% fetal calf serum (FCS) was used as a control. CSCs were identified with flow cytometry using CD44+/CD24-as molecular markers. The expression of a variety of CSC markers (Oct-4, ABCG2, Nanog, N-cadherin, and E-cadherin) was analyzed with real-time PCR. Results Much higher percentage of CSCs was achieved with K-SFM: 17.3% for MCF-7 cells, 17.4% for SKBR-3, and 20.0% for primary breast cancer culture. Less than 1% CSC was achieved using RPMI-1640 supplemented with 10% FCS. In comparison to the CSCs obtained with RPMI-1640, CSCs in the K-SFM expressed higher levels of Oct-4, ABCG2, Nanog and N-cadherin, and lower level of E-cadherin. Conclusion K-SFM is an optimal culture medium to maintain and to enrich breast CSCs. 展开更多
关键词 breast cancer cancer stem cells keratinocyte serum-free medium defined medium enrichment
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Application of Serum-Free Culture Medium for Preparation of A-NK Cells 被引量:6
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作者 Zhihua Wang Zhibin Zhang Hui Zhang Yan Zhang 《Cellular & Molecular Immunology》 SCIE CAS CSCD 2006年第5期391-395,共5页
To compare the differences between proliferation and cytotoxicity of adherent natural killer (A-NK) cells cultured with serum-free medium AIMV and standard serum-containing medium in vitro, and also observe the assi... To compare the differences between proliferation and cytotoxicity of adherent natural killer (A-NK) cells cultured with serum-free medium AIMV and standard serum-containing medium in vitro, and also observe the assisting effect of IL-12 on the activation and the morphology character of IL-2-treated A-NK cells, cellular proliferation was evaluated by MTT method in vitro. The morphology of the target cells killed by A-NK cells was observed through electroscope. All of the A-NK cells cultured in serum-free medium AIMV could rapidly proliferate and keep high cytotoxicity compared with that in standard serum-containing medium. A-NK cells activated by both moderate-dose IL-2 and IL-12 were superior to the high-dose IL-2-treated A-NK cells. These data indicated that serum-free medium AIMV could replace standard serum-containing medium for culturing A-NK cells, and moderate-dose IL-2 and IL-12 could reduce side effects caused by high-dose IL-2. The study provided a new experimental basis for experimental and clinical preparation of A-NK cells. Cellular & Molecular Immunology. 展开更多
关键词 A-NK cell serum-free medium AIMV IL-12
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Marc-145细胞的无血清悬浮培养基开发
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作者 程成 王玉红 +3 位作者 李敏捷 刘旭平 谭文松 赵亮 《黑龙江畜牧兽医》 CAS 北大核心 2022年第17期121-126,132,共7页
为开发适合Marc-145细胞生长的无血清悬浮培养基,试验将贴壁Marc-145细胞转入Celer-S001培养基中进行悬浮适应,通过混料试验和水解物筛选试验获得适应Marc-145细胞快速扩增的无血清悬浮培养基,对悬浮培养的Marc-145细胞进行猪繁殖与呼... 为开发适合Marc-145细胞生长的无血清悬浮培养基,试验将贴壁Marc-145细胞转入Celer-S001培养基中进行悬浮适应,通过混料试验和水解物筛选试验获得适应Marc-145细胞快速扩增的无血清悬浮培养基,对悬浮培养的Marc-145细胞进行猪繁殖与呼吸综合征病毒感染并检测病毒效含量,评价悬浮培养的Marc-145细胞的病毒扩增能力。结果表明:Marc-145细胞可以在Celer-S001培养基中悬浮培养,其比生长速率为(0.25±0.06)/d;适应Marc-145细胞快速扩增的最优无血清悬浮培养基由B3和B8培养基以0.54∶0.46比例混合,并添加2 g/L的水解物H3构成,Marc-145细胞的比生长速率为(0.51±0.03)/d,密度为3.73×10^(6) cells/mL;细胞接毒后的病毒含量最高可达(5.25±0.25)lgTCID_(50)/mL,表明细胞仍然保持着病毒扩增能力。说明试验成功开发了适合Marc-145细胞生长的无血清悬浮培养基,Marc-145细胞在该培养基中生长良好,具有病毒扩增能力。 展开更多
关键词 MARC-145细胞 无血清悬浮培养 混料设计 水解物 培养基
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CHO-K1细胞的悬浮驯化及无血清培养 被引量:2
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作者 刘华敏 漆彦斌 雷志斌 《顺德职业技术学院学报》 2019年第4期1-3,8,共4页
以CHO-K1细胞为研究对象,首先对贴壁细胞进行了悬浮驯化,之后比较了自配无血清培养基CHO-SFM、Sigma Ex-CELL CD CHO培养基和Gibco CD CHO培养基驯化悬浮细胞CHO-K1-S的培养效果。在相同实验条件下,统计细胞的增长率和存活率。结果表明... 以CHO-K1细胞为研究对象,首先对贴壁细胞进行了悬浮驯化,之后比较了自配无血清培养基CHO-SFM、Sigma Ex-CELL CD CHO培养基和Gibco CD CHO培养基驯化悬浮细胞CHO-K1-S的培养效果。在相同实验条件下,统计细胞的增长率和存活率。结果表明,自配无血清培养基CHO-SFM优于Sigma CD-CHO和Gibco CD-CHO两种商业化培养基。 展开更多
关键词 CHO-K1-S细胞 悬浮培养 无血清培养基 增长率
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