Noggin versus basic fibroblast growth factor on the differentiation of human embryonic stem cells

The difference between Noggin and basic fibroblast growth factor for the neural precursor differen- tiation from human embryonic stem cells has not been studied. In this study, 100 tJg/L Noggin or 20 IJg/L basic fibroblast growth factor in serum-free neural induction medium was used to differen- tiate human embryonic stem cells H14 into neural precursors using monolayer differentiation. Two weeks after induction, significantly higher numbers of neural rosettes formed in the Noggin-induced group than the basic fibroblast growth factor-induced group, as detected by phase contrast micro- scope. Immunofluorescence staining revealed expression levels of Nestin, [3-111 Tubulin and Sox-1 were higher in the induced cells and reverse-transcription PCR showed induced cells expressed Nestin, Sox-1 and Neurofilament mRNA. Protein and mRNA expression in the Noggin-induced group was increased compared with the basic fibroblast growth factor-induced group. Noggin has a greater effect than basic fibroblast growth factor on the induction of human embryonic stem cell differentiation into neural precursors by monolayer differentiation, as Noggin accelerates and in- creases the differentiation of neural precursors.

Xeno-free culture of human spermatogonial stem cells supported by human embryonic stem cell-derived fibroblast-like cells

Spermatogonial stem cells （SSCs） divide continuously to support spermatogenesis throughout postnatal life and transmit genetic information to the next generation. Here, we report the successful establishment of the method for the isolation and identification of human SSCs from testicular tissue, and to determine the culture conditions required to expand SSCs on human embryonic stem cell-derived fibroblast-like cells （hdFs）. Large-scale cultures of SSCs were maintained on hdF feeder layers and expanded in the presence of a combination of cytokines and glial cell line-derived neurotrophic factor for at least 2 months. Cell surface marker analysis showed that SSCs retained high levels of alkaline phosphatase activity and stained strongly for anti-stage-specific embryonic antigen （SSEA）-1, OCT4 and CD49f. They also expressed the genes OCT4, SOX3 and STRA8 as detected by reverse transcription polymerase chain reaction （RT-PCR） analysis. These data clearly illustrate a novel approach for the growth of human SSCs using hdFs as feeder cells, potentially eliminating xenogeneic contaminants. This system provides a new opportunity for the study of the regulatory mechanism of the ‘niche＇ that governs SSC self-renewal, and will be a valuable source of SSCs for potential clinical applications.

Mitofusion 2 Overexpression Decreased Proliferation of Human Embryonic Lung Fibroblasts in Acute Respiratory Distress Syndrome through Inhibiting RAS-RAF-1-ERK1/2 Pathway

Acute respiratory distress syndrome(ARDS)is one of the most fatal diseases worldwide.Pulmonary fibrosis occurs early in ARDS,and its severity plays a crucial role in ARDS mortality rate.Some studies suggested that fibroproliferation is an essential mechanism in ARDS.Mitofusion2(Mfn2)overexpression plays a role in inhibiting cell proliferation.However,the role and potential mechanism of Mfn2 on the proliferation of fibroblasts is still unknown.In this study,we aimed at exploring the effect of Mfn2 on the human embryonic lung fibroblasts(HELF)and discussed its related mechanism.The HELF were treated with the Mfn2 overexpressing lentivirus(adv-Mfn2).The cell cycle was detected by flow cytometry.MTT,PCR and Western blotting were used to investigate the effect of Mfn2 on the proliferation of the HELF,collagen expression,the RAS-RAF-1-ERK1/2 pathway and the expression of cycle-related proteins(p21,p27,Rb,Raf-1,p-Raf-1,Erk1/2 and p-Erk1/2).The co-immunoprecipitation assay was used to explore the interaction between Mfn2 and Ras.The results showed that the overexpression of Mfn2 inhibited the proliferation of the HELF and induced the cell cycle arrest at the G0/G1 phase.Meanwhile,Mfn2 also inhibited the expression of collagen I,p-Erk and p-Raf-1.In addition,an interaction between Mfn2 and Ras existed in the HELF.This study suggests that the overexpression of Mfn2 can decrease the proliferation of HELF in ARDS,which was associated with the inhibition of the RAS-RAF-1-ERK1/2 pathway.The results may offer a potential therapeutic intervention for patients with ARDS.

Development of neural precursor cells from mouse embryonic stem cells

Objective:To exploretheserum-freecultureconditionsfordifferentiatingmouseembryonicstemcells(ES cells)intoneuralprecursorcells(NPC)andcomparetheeffectsof humanembryonicfibroblasts(HEF)as thefeederlayer of ES withthatof mouseembryonicfibroblasts(MEF)in vitro.Methods:MouseES cellswereculturedin or notin feederlayer cellsmediumcontainingor notleukemiainhibitoryfactorto suppresstheirdifferentiation.Immunocytochemicalmethod was usedto identifyNPCby detectingnestinantigenandalkalinephosphatase.Results: TheES cellsculturedin HEF werepositiveto alkalinephosphatase.Serum-freemediumallowedthedifferentiationof ES cellsintoNPC.Conclusion:HEFcouldreplaceMEFandkeeptheundifferentiatedconditionof ES cellswithmorebenefits.NPCof highpuritycould be culturedfromEScellsby serum-freeculturemethod.

Low level of activin A secreted by fibroblast feeder cells accelerates early stage differentiation of retinal pigment epithelial cells from human pluripotent stem cells

Human pluripotent stem cells (hPSC) differentiated to retinal pigment epithelial cells (RPE) provide a promising tool for cell replacement therapies of retinal degenerative diseases. The in vitro differentiation of hPSC-RPE is still poorly understood and current differentiation protocols rely on spontaneous differentiation on fibroblast feeder cells or as floating cell aggregates in suspension. The fibroblast feeder cells may have an inductive effect on the hPSC-RPE differentiation, providing variable signals mimicking the extraocular mesenchyme that directs the differentiation in vivo. The effect of the commonly used fibroblast feeder cells on the hPSCRPE differentiation was studied by comparing suspension differentiation in standard RPEbasic (no bFGF) medium to RPEbasic medium conditioned with mouse embryonic (mEF-CM) and human foreskin (hFF-CM) fibroblast feeder cells. The fibroblast secreted factors were found to enhance early hPSC-RPE differentiation. The onset of pigmentation was faster in the conditioned media (CM) compared to RPEbasic for both human embryonic (hESC) and induced pluripotent (iPSC) stem cells, with the first pigments appearing around two weeks of differentiation. After four weeks of differentiation, CM conditions consistently contained higher number of pigmented cell aggregates. The ratio of PAX6 and MITF positive cells was quantified to be clearly higher in the CM conditions, with mEFCM containing most positive cells. The mEF cells were found to secrete low levels of activin A growth factor that is known to regulate eye field differentiation. As RPEbasic was supplemented with corresponding, low level (10 ng/ml) of recombinant human activin A, a clear increase in the hPSC-RPE differentiation was achieved. Thus, inductive effect provided by feeder cells was at least partially driven by activin A and could be substituted with a low level of recombinant growth factor in contrasts to previously reported much higher concentrations.

Anti-senescence effect and molecular mechanism of the major royal jelly proteins on human embryonic lung fibroblast(HFL-I) cell line

Royal jelly (R J)from honeybee has been widely used as a health promotion supplement.The major royal jelly proteins (MRJPs)have been identified as the functional component of RJ.However,the question of whether MRJPs have anti-senescence activity for human cells remains.Human embryonic lung fibroblast (HFL-I)cells were cultured in media containing no MRJPs (A),MRJPs at 0.1mg/ml (B),0.2mg/ml (C),or 0.3mg/ml (D),or bovine serum albumin (BSA)at 0.2mg/ml (E).The mean population doubling levels of cells in media B,C,D,and E were increased by 12.4%,31.2%,24.0%,and 10.4%,respectively,compared with that in medium A.The cells in medium C also exhibited the highest relative proliferation activity,the lowest senescence,and the longest telomeres.Moreover, MRJPs up-regulated the expression of superoxide dismutase-1(SOD1)and down-regulated the expression of mammalian target of rapamycin (MTOR),catenin beta like-1(CTNNB1),and tumor protein p53(TP53).Raman spectra analysis showed that there were two unique bands related to DNA synthesis materials,amide carbonyl group vibrations and aromatic hydrogens.These results suggest that MRJPs possess anti-senescence activity for the HFL-I cell line,and provide new knowledge illustrating the molecular mechanism of MRJPs as anti-senescence factors.

Preliminary study on human fibroblasts as feeder layer for human embryonic stem cells culture in vitro

To avoid the direct contact with mouse cells and possible heterogeneous pathogen in future application, we need to replace mouse embryonic fibroblasts with human fibroblasts as the feeder layer to maintain human embryonic stem cells growth in the undifferentiated state. We success-fully use human fibroblasts derived from aborted fetus and adult prepuce as feeder layer to maintain human embryonic stem cells growth. During the passage and growth on this feeder layer, the human embryonic stem cells can keep their undifferentiated state.

以STO细胞和hELF作为胚胎生殖细胞培养饲养层的比较

目的：比较以STO细胞和人胚胎肺成纤维细胞（hELF）作为饲养层对人胚胎生殖嵴细胞（EG）生长的影响以及经丝裂酶素C处理后的两种饲养层的变化．方法：分离、培养3—4mohELF，观察经丝裂酶素C处理STO细胞和hELF后形态学变化，以STO细胞和hELF作为饲养层培养人EG细胞，计数EG细胞集落的形成率以及免疫组化检测EG细胞表面标志物抗阶段特异性胚胎抗原-1（SSEA-1）和抗阶段特异性胚胎抗原-4（SSEA-4）．结果：经丝裂霉素c处理后hELF较STO细胞生存时间明显长，形态维持更好；以hELF和STO细胞作为饲养层培养人EG细胞，集落形成率没有明显差异；两种饲养层上形成的集落免疫学特征无明显差异．结论：在培养人EG细胞时，hELF饲养层较STO细胞饲养层更有优势．

miR-155对人胚肺成纤维细胞HELF增殖、凋亡和胶原蛋白合成的影响

目的:探讨miR-155对人胚肺成纤维细胞HELF增殖、凋亡和胶原蛋白合成的影响。方法:通过转染miR-155抑制剂构建miR-155低表达的HELF细胞株,采用qRT-PCR检测转染效果,CCK-8法和流式细胞仪检测miR-155低表达对HELF细胞增殖、凋亡的影响,Western blot检测miR-155低表达对Col-Ⅰ和Col-Ⅲ胶原蛋白表达的影响。采用TargetScan软件预测并通过双荧光素酶报告基因实验检测miR-155和Smad5的靶向关系,qRT-PCR和Western blot检测miR-155和Smad5的调控关系。将si-Smad5和miR-155抑制剂共同转染HELF细胞后,观察Smad5沉默是否影响miR-155对HELF细胞增殖、凋亡和胶原蛋白合成的作用。结果:转染miR-155抑制剂成功下调了HELF细胞中miR-155的表达,miR-155低表达能够明显抑制HELF细胞增殖和Col-Ⅰ、Col-Ⅲ胶原蛋白的合成,并促进HELF细胞凋亡(P<0.05)。miR-155可与Smad53′UTR区域结合并负向调控Smad5表达(P<0.05)。Smad5沉默可逆转miR-155低表达对HELF细胞增殖、凋亡和胶原蛋白合成的调控作用(P<0.05)。结论:miR-155低表达可通过靶向调控Smad5抑制HELF细胞增殖和胶原蛋白合成,并促进HELF细胞凋亡。

沙利度胺抑制TGF-β_1诱导的HELF细胞中结缔组织生长因子基因启动子的激活

目的:探讨沙利度胺(thalidomide,THD)对转化生长因子β1(transforming growth factorβ1,TGF-β1)诱导的人胚肺成纤维细胞(human embryonic lung fibroblast,HELF)结缔组织生长因子(connective tissue growth factor,CTGF)基因启动子激活的影响。方法:构建含有人类CTGF基因启动子的报告基因载体pGL3-CTGFP,将其瞬时转染HELF细胞,通过检测萤光素酶的活性,观察TGF-β1和THD对CTGF基因启动子活性的影响。结果:TGF-β1能以剂量依赖方式和时间依赖方式显著增加HELF细胞中报告基因的活性(P<0.05),最佳剌激浓度是5μg/L,萤光素酶相对活性为对照组的2.16倍,最佳剌激时间为12 h,萤光素酶相对活性为对照组的2.52倍;THD对报告基因的基础活性无明显影响(P>0.05),但以剂量依赖方式显著抑制TGF-β1上调报告基因活性的效应(P<0.05)。结论:TGF-β1能以剂量依赖方式和时间依赖方式上调HELF细胞中CTGF基因启动子的活性,而THD能以剂量依赖方式抑制此过程。

麻杏石甘汤对3型腺病毒感染HELF部分细胞因子mRNA基因表达的影响

目的:探讨麻杏石甘汤含药血清对3型腺病毒感染的人胚肺成纤维细胞(HELF)之转化生长因子-β1(TGF-β1)、血小板衍生生长因子-BB(PDGF-BB)、肿瘤坏死因子-α(TNF-α)mRNA基因表达的影响。方法:以3型腺病毒分别攻击体外培养的HELF,制备麻杏石甘汤含药血清,作用于该细胞,另设正常细胞组、病毒对照组、利巴韦林组,采用原位杂交法检测不同组细胞TGF-β1、PDGF-BB、TNF-α的mRNA基因表达,进行各组间比较。结果:病毒对照组较正常细胞组之TGF-β1、PDGF-BB、TNF-αmRNA的表达均明显升高(P<0.01),含药血清组对腺病毒攻击后的TGF-β1、PDGF-BB、TNF-αmRNA表达均有显著降低作用(P<0.01)。结论:麻杏石甘汤可下调TGF-β1、PDGF-BB、TNF-α的mRNA表达,这可能是其治疗病毒性肺炎的作用机制之一。

麻杏石甘汤对腺病毒感染的HELF细胞因子蛋白表达影响的实验研究

目的探讨麻杏石甘汤含药血清对3型腺病毒感染的人胚肺成纤维细胞(HELF)之转化生长因子-β1(TGF-β1)、血小板衍生生长因子-BB(PDGF-BB)、肿瘤坏死因子-α(TNF-α)蛋白表达的影响。方法以3型腺病毒攻击体外培养的HELF,制备麻杏石甘汤含药血清,作用于该细胞,另设正常细胞组,病毒对照组,利巴韦林组,采用酶联免疫吸附试验(ELISA法)检测不同组细胞TGF-β1、PDGF-BB、TNF-α的蛋白表达,并进行比较。结果病毒对照组较正常细胞组之TGF-β1、PDGF-BB、TNF-α蛋白表达均明显增强(P<0.01),含药血清组可显著降低3型腺病毒攻击后HELF的TGF-β1、PDGF-BB、TNF-α的蛋白表达(P<0.01)。结论麻杏石甘汤可下调3型腺病毒感染后TGF-β1、PDGF-BB、TNF-α的蛋白表达,这可能是其治疗病毒性肺炎的作用机制之一。

HELF中IL-33/ST2L-TRAF-6信号通路的激活对其增殖、活化及胶原合成的影响

目的观察rhIL-33对人胚肺成纤维细胞增殖及其间充质细胞标记物的影响,探讨IL-33/ST2L-TRAF信号通路在肺纤维化形成过程中的作用。方法培养HELF细胞,PCR检测IL-33受体ST2L m RNA;不同浓度梯度的rh IL-33刺激细胞,MTT法检测不同时间点（24、48、72 h）IL-33对HF细胞增殖的影响;Real-time PCR方法检测IL-33刺激HELF后不同时间点（0、6、12、24、48、72 h）细胞标志性基因α-SMA m RNA、Vimentin m RNA、collagn I m RNA及TRAF-6 m RNA的变化;Western blot法检测细胞标志性蛋白α-平滑肌肌动蛋白（α-SMA）、波形蛋白（Vimentin）、I型胶原（collagen I）及关键性信号分子TRAF-6与下游信号分子ERK1/2、JNK、NF-kappa B等的改变。结果 IL-33能促进HELF的增殖,10 ng/ml的IL-33促增殖作用最强,且72 h最为明显;随着IL-33刺激细胞时间的逐渐延长,在0～72 h内α-SMA、Vimentin、collagen I在基因与蛋白水平均先上调后下调,信号分子TRAF-6、ERK1/2、JNK、NF-kappa B（P65）等亦呈现先上调后下调的趋势。结论 IL-33能促进HELF细胞增殖、活化及合成胶原,IL-33/ST2L-TRAF-6通路在此过程中起了关键作用,尤其是在病变早期炎症过程中作用最为明显。

稳定转染Dicer基因对HELF细胞功能的影响

目的观察正常人胚肺成纤维细胞(HELF)在稳定转染Dicer基因后增殖能力及迁移能力的变化。方法应用脂质体介导方法转染Dicer基因表达载体于HELF细胞,G418筛选,PCR检测整合情况,RT-PCR检测表达情况,Western-blot检测蛋白表达水平,确定稳定转染细胞株,MTT方法检测细胞增值能力,Transwell方法检测细胞迁移能力。结果Dicer基因稳定转染HELF细胞系建立,用RT-PCR和Western-blot方法检测到Dicer基因mRNA和蛋白表达水平都明显增强。与转染空载体的HELF细胞相比,转染Dicer基因的HELF细胞48、72、96h的MTT光吸收值明显升高(P<0.05),并且穿过人工重构基底膜的细胞数明显增多。结论Dicer基因稳定转染HELF细胞后,HELF细胞增殖能力和迁移能力都明显增强。

沙利度胺对TGF-β1诱导HELF细胞CTGF基因启动子结合蛋白变化的干预作用

目的:探讨沙利度胺(thalidomide,THD)和转化生长因子β_1(transformation growth factor-β_1,TGF-β_1)对人胚肺成纤维细胞(human embryonic lung fibroblasts,HELF)中结缔组织生长因子(connective tissue growth factor,CTGF)基因启动子的作用及其分子机制。方法:利用CTGF基因启动子驱动的萤光素酶报告基因系统观察TGF-β_1和THD对HELF细胞CTGF基因启动子活性的影响;同时以带有生物素标记的CTGF基因启动子序列作为探针,采用DNA pull-down技术分析TGF-β_1和THD对CTGF基因启动子结合蛋白的影响。结果:TGF-β_1能显著增强HELF细胞中报告基因的活性(P<0.01),而THD以剂量依赖方式显著抑制TGF-β_1上调报告基因活性的效应(P<0.01)。同时,TGF-β_1引起的CTGF基因启动子结合蛋白变化也能被THD所抑制(P<0.05)。结论:CTGF基因启动子结合蛋白调节可能参与TGF-β_1对HELF细胞中CTGF基因启动子的激活过程,而THD能有效拮抗此过程。

大蒜新素对人巨细胞病毒感染的人胚肺成纤维细胞凋亡的影响

目的研究大蒜新素对人巨细胞病毒(HCMV)诱导感染的人胚肺成纤维细胞(HELF)凋亡的动态变化及凋亡调控基因bcl-2和fasmRNA表达的影响。方法用流式细胞术测定HELF在高、低感染复数(MOI分别为2.5、0.25)HCMV感染后1、12、24、36、48、72、96h凋亡细胞比率;大、中、小剂量大蒜新素(9、6和3μg/mL)处理正常的和感染的HELF细胞(MOI为2.5)后上述各时间点凋亡细胞比率。用原位杂交法检测大剂量大蒜新素处理感染细胞(MIO为0.25)72h后bcl-2和fasmRNA表达强度变化,并与正常细胞和感染细胞对比分析。结果正常细胞凋亡比率保持恒定低水平(凋亡率平均2.68%);低、高感染复数感染细胞随时间延长凋亡细胞逐渐增多,凋亡率峰值分别达8.85%(96h)和25.63%(72h);各剂量大蒜新素处理的正常细胞凋亡率增加,呈剂量依赖性,峰值分别为4.88%、6.47%和8.35%;但各剂量药物处理感染细胞后却使细胞凋亡比率下降,大剂量药物处理72h时效应最为明显,凋亡细胞比率由25.63%降至16.24%。正常细胞高表达bcl-2,低表达fas基因;感染HCMV后,bcl-2表达显著下调,fas表达明显增强;大蒜新素处理感染细胞后使bcl-2表达强度明显高于感染细胞,fas表达水平明显低于感染细胞,但仍未恢复到正常细胞水平。结论HCMV是HELF凋亡的强诱导剂;

纳米氧化锌对人胚肺成纤维细胞的生物毒性

【目的】研究化妆品添加剂-氧化锌纳米粒子对正常人胚肺成纤维细胞(HELF)的生物毒性。【方法】采用MTT法检测氧化锌纳米粒子对体细胞存活率的影响;利用光学显微镜评价细胞的形态学变化;电子显微镜观察细胞与纳米氧化锌作用前后表面微结构的变化。【结果】在测试的2.5～150mg·L-1浓度范围内,氧化锌纳米粒子对HELF细胞均有抑制作用,细胞毒性呈明显的剂量依赖效应关系。浓度在20mg·L-1以上时,氧化锌纳米粒子可致使细胞生存率低于10%。荧光显微镜可见典型的细胞凋亡改变。扫描电子显微镜观察到HELF细胞表面与高浓度纳米粒子作用后产生的纳米级孔。【结论】纳米氧化锌粒子由于小尺寸效应和Zn2+自身毒性的协同作用,高浓度时抑制细胞结活性,致使细胞死亡。在化妆品中添加氧化锌纳米粒子作为紫外屏蔽剂时,建议控制浓度为20mg·L-1以下。旨在对化妆品生产企业在功效添加方面起到警示作用,也为卫生监督提供理论依据。

青蒿琥酯对人胚肺成纤维细胞系HFL-I细胞增殖、凋亡的影响及机制

目的进一步探讨青蒿琥酯的抗纤维化作用及机制。方法取对数生长期人胚肺成纤维细胞（HELF）系HFL-I细胞株，随机分为观察1—4组及对照组，观察1-4组分别加入质量浓度为4、8、16、32mg／L的青蒿琥酯，对照组加入等体积培养液后继续培养。用CCK-8法检测细胞增殖情况（A值），流式细胞仪检测细胞周期及凋亡率，RT-PCR法测定Survivin mRNA表达。结果观察1-4组G0＋G1期细胞所占比例及细胞凋亡率均显著高于对照组，细胞A值及Survivin mRNA表达均显著低于对照组，且各观察组间亦有显著差异（P〈0．05）。结论青蒿琥酯具有抗肺纤维化作用，可能机制为通过下调Survivin mRNA表达抑制HFL-I细胞增殖、促进HFL-I细胞凋亡。

胰蛋白酶消化法和组织块法原代培养人包皮成纤维细胞的比较

小鼠胚胎成纤维细胞(MEFs)是目前国际上公认的人胚胎干细胞(hESCs)体外培养的饲养层细胞,但MEFs存在寿命短、动物源性污染等问题,需要探索适于hESCs体外培养且寿命长的人源性饲养层.采用胰蛋白酶消化法和组织块法分别原代培养人包皮成纤维细胞(hFFs),探索hFFs原代培养的最佳方法,为hFFs作为饲养层在hESCs研究中的应用提供可靠的科学依据;通过倒置显微镜下观察其生长状态和免疫细胞化学染色鉴定,结果显示两种原代培养方法获得的hFFs的形态及生物学特性均符合成纤维细胞;通过测定细胞生长曲线及MTT法检测,结果显示两种原代培养方法获得的不同代数的hFFs均具有较高的增殖活性,传代10余代仍能保持较好的细胞形态,可以制备成饲养层用于hESCs的研究.

小鼠胚胎干细胞体外分化为神经前体细胞的研究

目的 探索小鼠胚胎干细胞 (Embryonicstemcell ,EScell)体外分化为神经前体细胞 (Neuralprecursorcells ,NPC)的无血清培养条件 ,比较人胚胎成纤维细胞 (Humanembryonicfibroblasts ,HEF)与小鼠胚胎成纤维细胞 (Mouseembryonicfibroblasts ,MEF)对小鼠ES细胞生长的作用。方法 在MEF或HEF饲养层上培养ES细胞 ,培养液中含白血病抑制因子。采用无血清方法培养NPC ,免疫组化方法检测巢蛋白 (Nestin) ,用硝基四氮唑蓝 /5 溴 4 氯 3 吲哚基磷酸 (NBT/BCIP)显色检测碱性磷酸酶。结果 无血清培养可以获得 86 %的NPC。HEF与MEF一样能维持ES未分化状态。结论 无血清培养方法有利于ES细胞向NPC分化 ,HEF可用于小鼠ES细胞的培养 ,而且比MEF优越。