大鼠脂肪干细胞复合胶原-壳聚糖-硫酸软骨素三维支架构建组织工程软骨

Objective To evaluate the character of the collagen-chitosan-chondroitin sulfate scaffold seeded with rat adipose tissue-derived stromal cells. Methods A dipose tissue were harvested from 6 weeks old Wistar rats and the stromal cells were harvested by type Ⅰ collagenase and then cultured in vitro. Type Ⅰ collagen was fully mixed with chitosan, freeze-dried and cross-linked with chondroitin sulfate, then freeze-dried again and sterilized by ethylene oxide. The pore diameter, water content, porosity of the scaffold were tested. The adipose tissue-derived stromal cells were digested, seeded into the plates, scaffold, and cen-trifuged into pellet, and then induced into cartilage. MTT detection for cell proliferation was done. After 3 weeks, the cell morphology, and cell proliferation and adhesion were observed, and chondrngenic differenti-ation was also analyzed. Results The pore diameter, water content, porosity tested for the scaffold showed an appropriate form. Cell proliferation showed faster in the scaffold and pellet culture system after 5 day, there was still cell proliferation in the scaffold system after 14 days but no obvious changes in the pellet cul-ture system; ceils on the scaffold proliferated densely showed by histological staining, but there was a scaf-fold structure residues in the inner layer. The finding of type Ⅱ immunohistochemistry stain showed that cells express strong positive for type Ⅱ collagen in the scaffold and pellet culture system whereas it was weakly positive in the plate culture system; the specific mRNA for cartilage, type Ⅱ collagen, aggrecan and SOX-9 were expressed in all three systems showed by RT-PCR, but type X collagen was expressed continu-ously in the plate culture system and expressed after 21 days in the pellet culture system, whereas it was not detected in the collagen-chitosan-chondroitin sulfate scaffold system. Conclusion The parameters of the collagen-chitosan-chondroitin sulfate scaffold were suitable in our study. The results suggested that it can promote the adipose tissue-derived stromal cells proliferation and chondrogenic differentiation better than the plate and pellet culture systems and maintain the phenotype of chondrocytes well; it is the optimal choice for cartilage tissue engineering in the future.     

人骨髓间质干细胞体外扩增和向内皮细胞定向诱导分化的研究

目的：体外分离、扩增成人骨髓间质干细胞（MSCs）和向内皮细胞（ECs）定向诱导分化，开辟心血管组织工程种子细胞的新来源。 方法： 采用Percoll(1 073 g/L)从正常成人骨髓中分离出MSCs，纯化和扩增后流式细胞仪鉴定其纯度；用血管内皮生长因子(VEGF)诱导MSCs向ECs分化，Ⅷ因子(vWF)免疫组化和透射电镜(TEM)鉴定细胞性质。 结果： 5.0×105个MSCs在体外扩增15代后，获得8.0×1012个MSCs，扩增了约1.6×107倍；MSCs在加入VEGF诱导培养大约14-21 d，80%-90%的诱导细胞对Ⅷ因子相关抗原呈阳性反应；TEM可观察到胞浆内有Weible-palade小体，证实为ECs。 结论： 成人骨髓MSCs在体外具有定向诱导分化为ECs的潜能，这为心脏组织工程瓣体外构建, 尤其是在小儿先天性心脏病组织工程研究中种子细胞的来源提供了可能性。     

二氧化硅活化巨噬细胞中早期生长反应因子-1及其信号转导通路的研究

目的 探讨早期生长反应因子(Egr-1)及其信号转导在矽肺发生发展中的作用。方法用细胞免疫荧光、原位杂交方法检测二氧化硅(SiO2)刺激后Egr-1的表达定位,用报道质粒及EMSA检测其活性改变;用激酶活性分析法检测si0：刺激巨噬细胞后ERK1／2活性改变,进一步用激酶抑制剂初步探讨SiO2活化Egr-1的信号转导通路。结果SiO2刺激RAW264．7细胞短时间Egr-1核蛋白表达及转录因子明显增加;且在处理后30～60min,Egr-1核蛋白结合活性明显升高(为未处理组的20倍);在刺激后15min ERK1／2活性开始升高,30min达高峰(活性为对照组的29倍)而后渐降至基础水平;进一步用激酶阻断发现,Egr-1 mRNA及蛋白表达均减少。结论SiO2能激活巨噬细胞中Egr-1,且此过程可能由ERK1／2、p38介导,提示SiO2-ERK1／2、p38-Egr-1通路可能在矽肺发生发展过程中起重要作用。     

PD98059对人骨髓间质干细胞分化为成骨细胞的影响

目的:探讨胞外信号调节激酶(ERK)信号传导途径对骨髓间质干细胞(MSC)分化为成骨细胞的影响。方法:采用Ficoll-Paque淋巴细胞分离液分离成人MSC,体外扩增,应用地塞米松、β-甘油磷酸钠、vitaminC定向诱导MSC分化为成骨细胞。在成骨诱导液中加入不同剂量的PD98059,观察其对成骨细胞形成的影响。结果:MSC体外扩增15代可获得(3-4)×10¹²个细胞。在成骨诱导液作用下,MSC可在体外定向分化为成骨细胞。不同剂量的PD98059均可抑制MSC分化为成骨细胞,并有剂量依赖关系;同时促使部分细胞转化为脂肪细胞。结论:ERK信号传导途径可能在MSC分化为成骨细胞和脂肪细胞过程中起关键作用。     

兔髓核细胞诱导大鼠骨髓间充质干细胞分化为髓核细胞的研究

目的 研究体外新西兰大白兔髓核细胞(nucleus pulposus cells)与SD大鼠骨髓间充质干细胞(mes-enchymal stem cells,MSCs)共培养时,兔髓核细胞与大鼠MSCs直接和间接接触对MSCs分化为髓核细胞的影响.方法 DAPI (4‘,6-二咪基-2‘-苯吲哚盐酸)标记原代髓核细胞后,分别与第三代MSCs按接触组和非接触组(Transwell培养系统)共培养.每隔24小时应用免疫荧光观察MSCs的形态学变化,并用RT-PCR方法检测Ⅱ型胶原和可凝集蛋白多糖(Aggrecan)的表达.结果 直接接触培养组中可见分化的MSCs形态和功能接近髓核细胞;非直接接触组的MSCs未见变化.结论 髓核细胞与MSCs的直接接触,是诱导MSCs分化为髓核细胞的重要因素.     

人白细胞介素12在哺乳动物细胞中的稳定表达及其生物活性的研究

目的采用遗传基因工程方法获得具有生物活性的人白细胞介素12,探索其治疗肿瘤和慢性肝炎的可行性。方法采用已克隆的国人IL-12基因序列,利用内部核糖体切入位点(IRES)完成IL-12P35、P40双亚基共表达载体的构建,通过转染CHODHFR缺陷细胞,双抗夹心ELISA法筛选阳性克隆,MTX加压扩增,PCR检测其基因整合,T淋巴细胞增殖和诱生γ干扰素实验检测其生物活性。结果获得了稳定高效表达人IL-12的工程细胞系,表达产物为70×103左右的糖蛋白。结论本研究得到的基因重组人IL-12具有良好的生物活性,有强的诱导产生γ干扰素的能力和诱导活化T淋巴细胞增殖能力。     

川芎嗪诱导大鼠骨髓间质干细胞分化为神经元样细胞的研究

目的用川芎嗪(ligustrazin hydrochloride)在体外定向诱导SD青年鼠骨髓间质干细胞(mesenchymal stem cells，rMSCs)分化为神经元样细胞。方法用低糖DMEM冲洗骨髓腔，收集骨髓细胞悬液，接种在塑料培养瓶中。经体外扩增、纯化，选用第5代后的骨髓间质干细胞进行诱导分化。用10μg／LbFcF预诱导24h，更换成含川芎嗪的无血清培养基DMEM诱导间质干细胞分化为神经元样细胞。用免疫组织化学SABC法鉴定神经丝蛋白(NF—M)、神经元特异性烯醇化酶(NSE)、巢蛋白(nestin)、微管联合蛋白-2(MAP-2)、生长相关蛋白-43(GAP-43)、胶质纤维酸性蛋白(GFAP)的表达。结果第5代间质干细胞形态达到均一，呈梭形。用川芎嗪诱导15min到3h，间质干细胞胞体逐渐增大，并伸出细长突起形似神经元样细胞。免疫组织化学显示NF-M、NSE、nestin、MAP-2和GAP-43表达阳性，而GFAP阴性。对照组上述染色均为阴性。结论川芎嗪可诱导骨髓间质干细胞分化为神经元样细胞。     

Activation of MAP kinases,pp90rsk and pp70-S6 kinases in mouse mast cells by signaling through the c-kit receptor tyrosine kinase or FcϵRI: rapamycin inhibits activation of pp70-S6 kinase and proliferation in mouse mast cells

The high-affinity receptor for IgE, Fc_?RI, represents the major cell surface structure through which mast cells express immunologically specific secretory function. By contrast, the stem cell factor receptor (SCFR), which is encoded by c-kit, is essential for normal mast cell development. The signaling pathways initiated by the stimulation of mast cells through the Fc_?RI, which lacks intrinsic kinase activity, and the SCFR, a member of the receptor tyrosine kinase family, generally have been regarded to be distinct. We report here that mouse mast cells stimulated either with SCF or with IgE and specific antigen exhibit a remarkably similar pattern of activation of mitogen-activated protein kinases (MAPK), 90 kDa-S6 kinases (pp90^rsk), and pp70-S6 kinases (pp70-S6K). These results indicate that all three families of protein kinases are associated with the cell surface receptor-dependent activation of secretion, as well as proliferation, in mast cells. We also show that the immunosuppressant rapamycin, but not FK506, can inhibit both SCF-dependent pp70-S6 kinase activation and SCF-dependent proliferation in mouse mast cells, without suppressing IgE- and antigen-dependent mediator release. These findings suggest that the activation of pp70-S6 kinase represents an important link in the stimulation of cell proliferation by SCF. Our results also indicate that the intracellular signaling pathways initiated by stimulation of mast cells through the Fc_?RI or the SCFR exhibit more overlap than has previously been appreciated.     

氨氯地平抑制氧化型胆固醇诱导的血管内皮细胞凋亡

目的:研究氧化型胆固醇(Triol与25-OH)对人脐静脉内皮细胞凋亡的诱导作用,并观察氨氯地平对氧化型胆固醇诱导内皮细胞凋亡的影响。方法:体外培养人脐静脉内皮细胞,利用光镜、电镜、DNA电泳及流式细胞仪测定作为凋亡检测指标。结果:对照及胆固醇组未检测到细胞凋亡,Triol与25-OH处理组光镜、电镜下可见典型的细胞凋亡形态学改变,电泳示"DNAladder",流式细胞仪检测出现亚二倍体峰,凋亡率分别为32.25%与23.04%,而氨氯地平使其凋亡率分别下降至13.42%与11.77%。结论:氧化型胆固醇(Triol与25-OH)可以诱导人脐静脉内皮细胞发生凋亡,而氨氯地平抑制其凋亡诱导作用。     

中枢神经系统不同部位来源的神经干细胞在体外生长特性的比较

目的 比较相同发育阶段中枢神经系统不同部位来源的神经干细胞在体外的生长特性。方法 胚胎小鼠(E14)于无菌条件下分别分离并收集皮层、纹状体、间脑、中．后脑和脊髓，各部分制备成单细胞悬液，接种在添加有纤维细胞生长因子(FGF)的无血清培养液内，神经干细胞克隆生成后，经免疫细胞化学方法鉴定细胞特性，并在相同条件下进行传代，相差显微镜下观察克隆生成和细胞的迁移特性。结果 在添加有纤维细胞生长因子的无血清培养液中，少量接种的单个细胞会增殖并形成悬浮于细胞培养液中的细胞克隆。这些克隆具有生成新克隆并分化成神经元和胶质细胞的能力。在相同发育阶段，皮层、纹状体、间脑均可生成悬浮的克隆，其中皮层生成的速度最快，纹状体、间脑较慢，中．后脑、脊髓生成克隆的速度最慢；生成克隆后，皮层克隆的贴壁能力最差，贴壁的克隆少有细胞从其底部迁出，纹状体、间脑克隆较易贴壁，贴壁克隆底部有明显的细胞迁出，中．后脑、脊髓生成的克隆不易悬浮，很快贴壁，在贴壁克隆的底部有大量的细胞迁出。结论 在无血清培养液中，神经干细胞可在体外增殖、传代并分化生成神经元和胶质细胞，不同部位来源的神经干细胞在体外生成克隆的速度和细胞迁移性不同，这可能同体内特定部位细胞的发育特性有关。