Gatifloxacin inducing apoptosis of stromal fibroblasts through cross-talk between caspase-dependent extrinsic and intrinsic pathways

AIM: To reveal the cytotoxicity and related mechanisms of gatifloxacin(GFX) to stromal fibroblasts(SFs) in vitro.METHODS: SFs were treated with GFX at different concentrations(0.009375%-0.3%), and their viability was detected by MTT method. The cell morphology was observed using light/transmission electron microscope. The plasma membrane permeability was measured by AO/EB double-staining. Then cell cycle, phosphatidylserine(PS) externalization, and mitochondrial transmembrane potential(MTP) were analyzed by flow cytometry. DNA damage was analyzed by electrophoresis and immunostaining. ELISA was used to evaluate the caspase-3/-8/-9 activation. Finally, Western blotting was applied for detecting the expressions of apoptosis-related proteins.RESULTS: Morphological changes and reduced viability of GFX-treated SFs demonstrated that GFX above 0.009375% had cytotoxicity to SFs with dependence of concentration and time. GFX-treating cells also showed G1 phase arrest, increased membrane permeability, PS externalization and DNA damage, which indicated that GFX induced apoptosis of SFs. Additionally, GFX could activate the caspase-8, caspase-9, and caspase-3, induce MTP disruption, downregulate B-cell leukemia-2(Bcl-2) and B-cell leukemiaXL(Bcl-XL), and upregulate Bcl-2 assaciated X protein(Bax), Bcl-2-associated death promoter(Bad), Bcl-2 interacting domain(Bid) and cytoplasmic cytochrome C in SFs, suggesting that caspase-dependent extrinsic and intrinsic pathways were related to GFX-contributed apoptosis of SFs.CONCLUSION: The cytotoxicity of GFX induces apoptosis of SFs through triggering the caspase-dependent extrinsic and intrinsic pathways.

Hierarchy of mesenchymal stem cells: Comparison of multipotentmesenchymal stromal cells with fibroblast colony forming units

The organization of the compartment of mesenchymal stem cells is still obscure. Two types of human stromal precursor cells are known. Both of them are analyzed in in vitro system: mesenchymal multipotent stromal cells (MMSC) and fibroblast colony forming units (CFU-F). The aim of this study was to compare the main characteristics of MMSC and CFU-F derived from the bone marrow of 24 healthy donors. Growth and differentiation parameters, as well as relative expression levels of different genes were analyzed in MMSC and CFU-F. MMSC were cultivated for 5 passages. CFU-F concentration was determined for each bone marrow sample. The data obtained demonstrated the heterogeneity and hierarchical organization of both studied populations of stromal precursor cells-MMSC and CFU-F. These two types of stromal precursor cells turned to be different in most parameters studied. Altogether MMSC seemed to be more immature cells than CFU-F and took up the higher position in hierarchical tree of mesenchymal stem cells. The rate of differentiation and proliferative potential decreased with the donor’s age in both populations MMSC and CFU-F.

Hematopoietic stem cell-derived adipocytes and fibroblasts in the tumor microenvironment

The tumor microenvironment(TME) is complex and constantly evolving. This is due, in part, to the crosstalk between tumor cells and the multiple cell types that comprise the TME, which results in a heterogeneous population of tumor cells and TME cells. This review will focus on two stromal cell types, the cancerassociated adipocyte(CAA) and the cancer-associated fibroblast(CAF). In the clinic, the presence of CAAs and CAFs in the TME translates to poor prognosis in multiple tumor types. CAAs and CAFs have an activated phenotype and produce growth factors, inflammatory factors, cytokines, chemokines, extracellular matrix components, and proteases in an accelerated and aberrant fashion. Through this activated state, CAAs and CAFs remodel the TME, thereby driving all aspects of tumor progression, including tumor growth and survival, chemoresistance, tumor vascularization, tumor invasion, and tumor cell metastasis. Similarities in the tumorpromoting functions of CAAs and CAFs suggest that a multipronged therapeutic approach may be necessary to achieve maximal impact on disease. While CAAs and CAFs are thought to arise from tissues adjacent to the tumor, multiple alternative origins for CAAs and CAFs have recently been identified. Recent studies from our lab and others suggest that the hematopoietic stem cell, through the myeloid lineage, may serve as a progenitor for CAAs and CAFs. We hypothesize that the multiple origins of CAAs and CAFs may contribute to the heterogeneity seen in the TME. Thus, a better understanding of the origin of CAAs and CAFs, how this origin impacts their functions in the TME, and thetemporal participation of uniquely originating TME cells may lead to novel or improved anti-tumor therapeutics.

lncRNA GAS6-AS1靶向调控IL-11对子宫内膜基质细胞向成纤维细胞分化的影响

目的探讨长链非编码RNA(lncRNA)生长停滞特异基因转录的反义RNA(GAS6-AS1)靶向调控白细胞介素11(IL-11)对子宫内膜基质细胞(ESCs)向成纤维细胞分化的影响。方法体外传代培养ESCs,取传3~6代、对数生长期、生长状态良好的ESCs,随机分为TGF-β_(1)未干预组和TGF-β_(1)干预组。TGF-β_(1)未干预组不予TGF-β_(1)干预,TGF-β_(1)干预组用无血清培养基饥饿培养后予TGF-β_(1)干预,收集细胞,采用RT-qPCR法检测lncRNA GAS6-AS1、IL-11及纤维化标志物α平滑肌肌动蛋白(α-SMA)、Ⅰ型胶原蛋白α1(COL1A1)mRNA表达。另取传3~6代、对数生长期、生长状态良好的ESCs,分别转染三条si-GAS6-AS1序列以及si-Control序列,采用RT-qPCR法验证转染效率。将转染si-GAS6-AS1的ESCs用无血清培养基饥饿培养后予TGF-β_(1)干预,收集细胞,采用Western blotting法检测IL-11、α-SMA、COL1A1蛋白表达,采用CCK-8法检测细胞增殖活性,采用Annexin V-FITC/PI双染法检测细胞凋亡率。结果与TGF-β_(1)未干预组比较,TGF-β_(1)干预组lncRNA GAS6-AS1、IL-11、α-SMA、COL1A1 mRNA相对表达量均显著升高(P均<0.01)。转染si-GAS6-AS1-1、si-GAS6-AS1-2、si-GAS6-AS1-3及si-Control序列的ESCs GAS6-AS1 mRNA相对表达量分别为0.22±0.04、0.27±0.06、0.81±0.07、1.00±0.00。与转染si-Control序列的ESCs比较,转染si-GAS6-AS1-1、si-GAS6-AS1-2序列的ESCs GAS6-AS1 mRNA相对表达量显著降低(P均<0.01),而转染si-GAS6-AS1-3序列的ESCs GAS6-AS1 mRNA相对表达量降低不明显(P>0.05)。因此,选择si-GAS6-AS1-1、si-GAS6-AS1-2序列进行后续实验。与si-Control+TGF-β_(1)组比较,si-GAS6-AS1-1+TGF-β_(1)组和si-GAS6-AS1-2+TGF-β_(1)组IL-11、α-SMA、COL1A1蛋白相对表达量及细胞增殖活性均显著降低,细胞凋亡率均显著升高(P均<0.01)。结论lncRNA GAS6-AS1通过靶向调控IL-11表达抑制ESCs向成纤维细胞分化。

Generation and characterization of novel stromal specific antibodies

Rheumatoid synovial fibroblasts were used as an immunogen to produce monoclonal antibodies selected for their reactivity with stromal cell antigens. Mice were immunised with low passage whole cell preparations and the subsequent hybridomas were screened by immunohistochemistry on rheumatoid synovium and tonsil sections. The aim was to identify those antibodies that recognised antigens that were restricted to stromal cells and were not expressed on CD45 positive leucocytes. A significant number of antibodies detected antigen that identified endothelial cells. These antibodies were further characterised to determine whether the vessels identified by these antibodies were vascular or lymphatic. From five fusions clones were identified with predominant reactivity with: 1) fibroblasts and endothelial cells; or 2) broad stromal elements (fibroblast, endothelium, epithelium, follicular dendritic cells). A fibroblast-specific antibody that did not also identify vessels was not generated. Examples of each reactivity pattern are discussed.

肿瘤间质成纤维细胞对体外培养唾液腺多形性腺瘤细胞生物学行为的影响

目的探讨肿瘤间质成纤维细胞(TSF)对体外培养唾液腺多形性腺瘤(SPA)细胞增殖、侵袭和迁移的影响。方法采用组织块培养法培养唾液腺多形性腺瘤细胞(SPAC)、TSF和瘤旁正常成纤维细胞(NF),并通过免疫细胞化学染色法进行细胞鉴定。选取对数期TSF、NF制备条件培养液,培养SPAC并命名为TSF-SPAC组和NF-SPAC组,单纯培养SPAC作为对照组(SPAC组)。采用MTT实验、Transwell实验和划痕实验分别检测3组细胞的增殖、侵袭和迁移能力;酶联免疫吸附测定(ELISA)检测3组培养液中血管内皮生长因子(VEGF)的表达量。结果免疫细胞化学染色显示:波形蛋白(Vimentin)在TSF和NF中为阳性,而α-平滑肌肌动蛋白(α-SMA)和成纤维细胞活化蛋白(FAP)在NF中为阴性,在TSF中为弱阳性。MTT结果显示:TSF-SPAC组细胞增殖与NF-SPAC组和SPAC组的差异有统计学意义(P<0.05),NF-SPAC组与SPAC组的细胞增殖的差异无统计学意义(P>0.05)。Transwell侵袭实验和迁移实验显示:3组细胞的侵袭和迁移的差异无统计学意义(P>0.05)。ELISA检测结果显示:3组VEGF的表达量的差异均无统计学意义(P>0.05)。结论TSF可能参与了SPA的生物学行为,促进体外培养的SPAC增殖,对其体外侵袭和迁移无促进作用,为SPA寻找新的治疗靶点提供了方向。

不同浓度碱性成纤维细胞生长因子对兔骨髓基质细胞的影响

目的:观察骨髓基质细胞的培养及不同浓度碱性成纤维生长因子(bFGF)对其生长的影响。方法:采用全麻下抽取兔股骨骨髓,经体外培养的方法并在培养液中加入4种不同浓度的bFGF(0,60,120,240ng/ml)培养后经倒置显微镜观察;并用试剂盒测定细胞碱性磷酸酶的含量。结果:60、120ng/ml的bFGF能明显促进骨髓基质细胞的生长(P<0.01),其余两组无明显差异。而4组之间的细胞碱性磷酸酶含量在3天时无明显差异,6天时加入bFGF组的细胞碱性磷酸酶含量明显下降。结论:bFGF对骨髓基质细胞的影响是复杂和多方面的;不同剂量浓度对骨髓基质细胞生长的影响亦不一样,并不呈正相关,合适的有效浓度为60～120ng/ml。

bFGF和TGF-β1对原代培养的前列腺间质细胞的作用

目的:探讨碱性成纤维细胞生长因子(bFGF)和转化生长因子β1(TGF-β1)在良性前列腺增生(BPH)中的作用。方法:培养了人BPH间质细胞,采用MTT法检测无血清培养的间质细胞的增殖,用免疫组化方法检测平滑肌细胞表型变化,观察不同浓度bFGF和TGF-β1对培养的人BPH间质细胞的影响。结果:bFGF促进间质细胞增殖(P<0.05、P<0.01),较高浓度时(10μg/L)降低平滑肌细胞表型表达;TGF-β1(>0.1μg/L)抑制间质细胞增殖并增加平滑肌细胞表型表达(P<0.05、P<0.01);5μg/L的bFGF与0.001μg/L和0.01μg/L TGF-β1作用间质细胞,促进细胞增殖(P<0.01),与0.1μg/L,1μg/L及10μg/L TGF-β1作用间质细胞,抑制细胞增殖,0.1μg/L时对细胞的抑制作用轻微(P>0.05),1μg/L及10μg/L时出现明显的抑制(P<0.01),同时TGF-β1在较高浓度时(>1μg/L),平滑肌细胞表型表达明显增加(P<0.01)。结论:bFGF以时间和浓度依赖的方式促进培养的增生前列腺间质细胞的增殖,并减少平滑肌细胞表型表达;TGF-β1抑制间质细胞的生长并诱导间质细胞向平滑肌细胞分化,两者共同在BPH的形成机制中发挥着重要作用。

Identification of the involvement of LOXL4 in generation of keratocystic odontogenic tumors by RNA-Seq analysis

Keratocystic odontogenic tumors （KCOT） are benign, locally aggressive intraosseous tumors of odontogenic origin. KCOT have a higher stromal microvessel density （MVD） than dentigerous cysts （DC） and normal oral mucosa. To identify genes in the stroma of KCOT involved in tumor development and progression, RNA sequencing （RNA-Seq） was performed using samples from KCOT and primary stromal fibroblasts isolated from gingival tissues. Seven candidate genes that possess a function potentially related to KCOT progression were selected and their expression levels were confirmed by quantitative PCR, immunohistochemistry and enzyme-linked immunosorbent assay. Expression of lysyl oxidase-like 4 （LOXL4）, the only candidate gene that encodes a secreted protein, was enhanced at both the mRNA and protein levels in KCOT stromal tissues and primary KCOT stromal fibroblasts compared to control tissues and primary fibroblasts （P〈0.05）. In vitro, high expression of LOXL4 could enhance proliferation and migration of the human umbilical vein endothelial cells （HUVECs）. There was a significant, positive correlation between LOXL4 protein expression and MVD in stroma of KCOT and control tissues （r=0.882）. These data suggest that abnormal expression of LOXL4 of KCOT may enhance angiogenesis in KCOT, which may help to promote the locally aggressive biological behavior of KCOT.

骨髓基质细胞转化成骨细胞修复骨缺损:成纤维细胞生长因子和骨形成蛋白-2的作用

目的探讨成纤维细胞生长因子（ bFGF）和重组人骨形成蛋白－ 2（ rhBMP－ 2）单独和联合作用对骨髓基质细胞（ BMSC）的增殖和分化的影响。方法利用四唑盐比色法（ MTT），细胞总蛋白考马斯亮蓝测定法，碱性磷酸酶（ ALP）试剂盒分别测定不同浓度的 bFGF和 rhBMP单独和联合作用后 BMSC的增殖和分化情况。结果 bFGF单独作用促进 BMSC的增殖，但高浓度抑制 ALP表达， rhBMP对 BMSC的增殖和 ALP和总蛋白含量均有促进作用，而 bFGF和 rhBMP联合作用后 BMSC的增殖和 ALP活性较单独作用有更明显的升高。结论 bFGF和 rhBMP联合作用对于促进 BMSC的增殖和向成骨细胞分化有协同作用。

碱性成纤维细胞生长因子对体外培养的兔骨髓基质细胞生长特性的影响

目的:研究骨髓基质细胞(BMSC)在体外培养条件下分化为成骨细胞的能力,及碱性成纤维细胞生长因子(bFGF)对其贴附、增殖、分化的影响。方法:将各组BMSC传代后加入bFGF,其浓度分别为0、5、10、50、1002、00 ng/ml,用倒置相差显微镜、电镜、四唑盐比色法、碱性磷酸酶(ALP)染色、钙染色和电子探针等方法观察其形态、贴附、生长增殖活性、分化成熟和体外钙化的状况。结果:经10 ng/ml bFGF诱导后,BMSC贴附细胞数量明显增加。当100 ng/ml时,bFGF对BMSC的促增殖作用达到最大值。当加入bFGF时,ALP染色阳性率降低,当bFGF浓度为100μg/L时阳性率最低(P<0.01)。传代细胞连续培养30 d后钙染色结果呈阳性,电子探针检测矿化区的Ca/P值与羟基磷灰石结晶中Ca/P值相符。电镜观察可见培养的细胞具有典型的成骨细胞形态特征,并能产生胶原纤维。结论:BMSC在体外培养条件下具有分化为成骨细胞的能力,bFGF能够促进细胞的贴壁和增殖,但对其分化成熟具有抑制作用。

自固化磷酸钙复合兔自体骨髓基质细胞和bFGF异位成骨的研究

目的探讨自固化磷酸钙(CPC)复合自体骨髓基质细胞(BMSC)和碱性成纤维细胞生长因子(bFGF)异位成骨的可行性及其成骨效应。方法取兔骨髓,分离骨髓基质细胞,选取松质骨粒型自骨化磷酸钙置于板孔内,A组复合BMSC(3ml)和bFGF(100滋g/ml);B组仅复合BMSC(3ml);C组仅为CPC;置于培养箱中培养24h后植入兔骶棘肌内。分别于术后3天、4周、8周、12周行双能X线骨密度测定仪测定骨粒密度,光镜组织病理检测及图像分析并以激光共聚焦显微镜进一步观察,12周时行扫描电镜观察。结果术后8周A、B组骨粒的密度明显比C组高,12周时A、B两组也有显著性差异,光镜检测并以激光共聚焦显微镜观察术后8周A、B组有大量成骨样细胞,12周时有大量的板层状骨形成;而C组仍有较多的空泡,仅有少量的骨样组织。术后4周时A、B、C组的成骨面积差异有显著性。术后12周扫描电镜观察到A组的表面空隙内有明显的骨样组织填充,同时有多量的钙颗粒的沉积;B组次之,C组最少。结论bFGF可促进BMSC的增殖,BMSC能与自固化磷酸钙相容生长,自固化磷酸钙复合BMSC和bFGF可明显诱导新骨的形成。

不同浓度bFGF对犬骨髓基质细胞增殖、分化影响的实验研究

目的:研究不同浓度的碱性成纤维细胞生长因子(basic fibroblast growth factor,bFGF)对体外培养的beagle犬骨髓基质细胞(bone marrow stromal cells,BMSCs)增殖和分化的影响。方法:体外培养第2代BMSCs的培养液中分别加入不同浓度(25、50、100、200 ng/mL)的bFGF,连续6 d倒置显微镜下动态观察BMSCs的形态和生长情况,行MTT比色、碱性磷酸酶(alkaline phosphatase,ALP)活性定量检测、ALP和Von Kossa染色。结果:浓度为50 ng/mL的bFGF可明显促进犬的BMSCs增殖(P<0.05),但无显著促进犬BMSCs分化的作用(P>0.05)。结论:bFGF能有效促进犬BMSCs的增殖,且与bFGF剂量有关。

低氧诱导胎肝间质细胞表达碱性成纤维生长因子

目的:观察低氧培养条件下小鼠胎肝间质细胞中碱性成纤维生长因子(basic fibroblast growth factor,bFGF)的表达情况,为其用于脑缺血治疗提供依据。方法:取孕14.5 d小鼠胚胎肝细胞进行贴壁培养及传代,生长至次融合状态的第5代细胞在95%N2和5%CO2混合气体条件下培养,在2、4、8、163、2 h时应用半定量RT-PCR和Western印迹法检测其bFGF基因表达。结果:在常氧条件下培养的胎肝间质细胞中,bFGF mRNA及其蛋白水平均较低;而低氧培养则可显著提高胎肝间质细胞bFGF基因的mRNA及其蛋白水平。bFGF mRNA在低氧培养2 h时即显著增高,16 h时达到高峰水平。PCR产物bFGF与-βactin信号比从常氧培养的(5.94±2.65)%增加到(32.86±9.57)%(P<0.01),升高5.52倍;bFGF蛋白在低氧培养4 h时显著增高,16h时达到高峰水平,Western印迹法检测bFGF与-βactin信号从常氧培养的(4.73±2.23)%增加到(23.96±7.83)%(P<0.01),升高5.07倍。结论:低氧可诱导bFGF在小鼠胎肝间质细胞中的表达,提示小鼠胎肝间质细胞在脑缺血中的治疗作用。

bFGF真核表达质粒的构建及骨髓基质细胞转染

目的探讨bFGF基因转染骨髓基质干细胞的方法及可行性。方法构建bFGF基因真核表达质粒,用脂质体法介导转染骨髓基质细胞,通过形态学观察、免疫组化、ELISA法、及RT-PCR方法检测bFGF基因转染骨髓基质干细胞的成功性,以及转染后骨髓基质干细胞的生物学特性。结果bFGF基因成功转染骨髓基质干细胞,并能持续稳定的分泌bFGF蛋白,可诱导骨髓基质干细胞向成软骨方向分化。结论bFGF基因可以转染骨髓基质干细胞,并能诱导骨髓基质干细胞向成软骨方向分化。

几种细胞因子对骨髓基质成纤维细胞集落形成的影响及意义

目的 :观察细胞因子粒 巨噬细胞集落刺激因子 (GM CSF)、干细胞因子 (SCF)、白细胞介素 3(IL 3)、肿瘤坏死因子 (TNF)及其联合应用对骨髓基质成纤维细胞集落生成单位 (CFU F)形成的作用。方法 :应用体外骨髓基质细胞贴壁培养的方法 ,分别加入不同的细胞因子 ,进行培养 2周时的CFU F计数和培养 4周时贴壁细胞的增殖状态观察。结果 :GM CSF、SCF及TNF对骨髓基质细胞的增殖有明显的促进作用。结论 :体外加入某些细胞生长因子对骨髓基质细胞具有明显的扩增作用 ,提示基质细胞在体外适当细胞因子作用下扩增后进行回输 。

妊娠期糖尿病患者产后血清相关细胞因子与糖代谢异常的关系

目的:探讨妊娠期糖尿病患者产后血清脂蛋白相关磷脂酶(A2Lp-PLA2)、基质细胞趋化因子-1α(SDF-1α)、成纤维细胞生长因子(FGF21)表达特征及与糖代谢异常关系。方法:选取妊娠期糖尿病孕产妇138例作为研究对象,根据产后血糖筛查结果分为糖尿病组30例,糖耐量受损组41例、糖耐量正常组67例。测定血糖指标及各血清细胞因子水平,并分析其相关性。结果:空腹血糖(FBG)、三酰甘油(TG)、胰岛素抵抗指数(HOMA-IR)以及Lp-PLA2、SDF-1α、FGF21水平比较,糖尿病组>糖耐量受损组>糖耐量正常组(均P<0.05)。Lp-PLA2、SDF-1α、FGF21均与血糖指标呈正相关(P<0.05)。结论:Lp-PLA2、SDF-1α、FGF21表达与糖代谢异常密切相关,可将其作为临床筛查妊娠期糖尿病孕妇产后糖代谢异常的辅助指标。

衰老的卵巢间质成纤维细胞对肿瘤细胞增殖、侵袭能力的影响

目的探讨衰老的卵巢间质成纤维细胞对卵巢癌细胞系SKOV3的增殖、侵袭能力的影响。方法原代培养人卵巢正常成纤维细胞(NOF),在体外持续传代诱导细胞衰老,用衰老相关的β半乳糖苷酶染色(SA-b-gal)试验检测细胞是否发生衰老。收集正常成纤维细胞的条件培养基(CMn)及衰老成纤维细胞的条件培养基(CMs)。用CMn和CMs分别处理SKOV3细胞,利用CCK8试剂盒、Tra ns we ll小室及三维培养试验检测细胞的增殖、侵袭能力的变化。结果卵巢正常成纤维细胞在体外持续传代会导致细胞复制性衰老,在SA-b-gal试验中有明显的深蓝色沉淀产物。用CMs处理SKOV3细胞,CCK8试验显示细胞培养第5天的OD(2.067±0.058)高于CMn组(1.073±0.056)(t=21.19,P<0.01),表明细胞的增殖能力增强。Tra ns we ll试验显示CMs组穿透Ma trig e l胶的细胞数(235.00±29.68)个,较CMn组的(129.30±15.52)个明显增多(t=5.47,P<0.01);三维培养中形成的克隆球CMs组较CMn组明显增大、数量明显增多(27.00±2.16 vs 11.67±2.50;t=8.04,P<0.01),向外侵袭能力增强。结论衰老的卵巢间质成纤维细胞在体外培养中能促进卵巢癌细胞的增殖和侵袭能力。

不同滋养层对维持人胚胎干细胞的生长作用

目的比较不同滋养层对保持连续传代培养的人胚胎干细胞(hESC)不分化和高增殖能力作用的差异。方法分别用小鼠胚胎成纤维细胞(MEF)、人包皮成纤维细胞(hFF)、人骨髓间充质细胞(hMSC)作为滋养层培养hESC系H9细胞,采用碱性磷酸酶染色和台盼蓝染色观察不同滋养层支持的hESC的碱性磷酸酶阳性克隆数、细胞产量和细胞存活率,并采用免疫荧光染色对传代5代以后的hESC进行生物学鉴定。结果3种滋养层细胞均可维持hESC呈克隆样生长,但是不同滋养层支持的克隆的形态差异大。3种滋养层细胞支持的hESC的大鼠抗阶段特异性胚胎抗原-3及碱性磷酸酶染色均呈阳性。MEF支持的hESC的碱性磷酸酶阳性克隆数、细胞产量和细胞存活率均显著高于人来源滋养层(均P<0.01)。hMSC支持的hESC的碱性磷酸酶阳性克隆数、细胞产量均显著高于hFF的hESC(均P<0.01)。结论3种滋养层细胞均可支持hESC的正常生长。MEF最有利于hESC的增殖,但是两种人来源滋养层细胞为去除动物源性的hESC培养体系奠定了基础。在维持hESC增殖方面,hMSC优于hFF。

一种新的人胚胎干细胞无饲养层培养方法的建立

目的:以转染碱性成纤维细胞生长因子(bFGF)的人胎肝基质细胞株(FLSC)培养人胚胎干细胞(hESC),寻找更加安全、有效的体外培养扩增方法。方法:通过ELISA方法定量检测转基因的人FLSC条件培养基中bFGF的分泌量;以商业化的mTeSR1无血清无饲养层培养基、常规小鼠胚胎成纤维细胞(MEF)条件培养基,以及转染bFGF的人FLSC条件培养基(bFGF/FLSC-CM)分别培养扩增H9细胞。通过观察hESC形态、免疫荧光染色、流式细胞检测及RT-PCR,检测hESC全能性标志物的表达。结果:ELISA方法检测bFGF/FLSC-CM中bFGF因子的分泌量为(770.09±17.28)pg/mL,而MEF-CM中bFGF因子的分泌量为(55.59±0.61)pg/mL,两者存在显著差异(P<0.01);在3种培养体系下,免疫荧光检测hESC全能性标志Oct-4、Tra-1-81抗体的表达均呈阳性,流式检测细胞表面阶段特异性胚胎抗原4(SSEA-4)抗体阳性细胞的比例均在99%左右;RT-PCR检测到hESC特异的转录因子Oct-4、Nanog、Sox-2的表达。结论:以转染bFGF的人FLSC条件培养基可以有效扩增hESC,可为临床应用提供一种安全、高效、低成本的无饲养层培养方法。