低温冻存对脐血树突状细胞生物特性的影响

目的 :观察低温冻存对脐血来源的树突状细胞 (DCs)培养生物特性的影响 ,为DCs的应用提供冻存方法。方法 :设未冻存脐血细胞 (UFCB)经增殖培养后产生的DCs(UFDCs)为对照组 ,来源于经低温冻存的脐血 (CPCB)的DCs和经低温冻存的DCs(CPDCs)为实验组 ,比较实验组与对照组DCs生物特性 ,包括细胞增殖量 ,不染色和染色的细胞形态 ,台盼蓝拒染回收率 (TBR) ;细胞表面抗原 ;混合淋巴细胞培养剌激指数 (SI)、抗毒 杀灭效应处理率(ER)。结果 :CPCB与UFCB比 ,形成DCs的时间迟 ,细胞增殖量、树突状细胞量、CD1a、CD83、HLA DR表达、SI、ER均低。CPDCs与UFDCs比 ,形成贴壁树突状细胞迟 ,细胞增殖量、树突状细胞量、CD1a、CD83、HLA DR表达、SI、ER均低。CPCB的TBR为 95.8% ,CPDCs的TBR为 88.7%。结论 :脐血细胞和经增殖培养的脐血DCs ,经低温冻存后复温培养 ,DCs的生物特性有一定的损伤 ,但基本功能仍比较完整 ,回收率均 >85%。     

大鼠骨髓基质细胞的培养及生物学特性鉴定

目的:分离、培养大鼠MSCs,对其生物学特性进行鉴定.方法:取大鼠长骨中的骨髓组织,以贴壁法培养分离大鼠MSCs,经多次传代得到较纯的MSCs,倒置相差显微镜下观察细胞形态,应用免疫细胞化学方法对细胞的表面抗原标志进行检测.取3代MSCs,B-ME诱导6小时候后,倒置相差显微镜下观察细胞形态,应用免疫细胞化学方法鉴定诱导后细胞的表型特征.结果:倒置相差显微镜观察发现,接种后24h,细胞开始贴壁.培养3代以后,细胞呈梭形或多角形,折光性好,核为圆形、居中.免疫细胞化学检测细胞表面抗原显示:CD34-、CD45-、CD29+、CD44+、CD90+.诱导后细胞发出突起,逐渐生长延伸并彼此相连,形态学上具有神经细胞的明显特征.免疫细胞化学显示诱导后细胞NSE(神经元特异性烯醇化酶)阳性.结论:所采用的细胞分离培养方法简便可行,所获得的细胞其表型特征与文献报道一致,且具有向神经细胞分化的潜能.     

低温冻存对兔脂肪间充质干细胞部分生物学特性的影响

目的：研究低温冻存对兔脂肪间充质干细胞部分生物学特性的影响。方法采用组织块法分离培养兔脂肪间充质干细胞。用倒置显微镜观察原代细胞的细胞形态,流式细胞仪检测兔脂肪间充质干细胞的免疫表型。取第3代兔脂肪间充质干细胞置于-196℃液氮保存半年,37℃复苏并传至第7代。实验分为两组,实验组为冻存复苏后传至第7代的兔脂肪间充质干细胞,对照组为未冻存的第7代兔脂肪间充质干细胞,用MTT绘制其生长曲线;添加成脂、成骨诱导液进行诱导,油红O、茜素红染色和碱性磷酸酶活性检测分别进行鉴定。结果体外培养的兔脂肪间充质干细胞呈梭形纤维样细胞形态,生长力旺盛。流式细胞仪检测显示,第3代兔脂肪间充质干细胞强表达CD44、CD90,阴性表达造血细胞相关的表面标志CD45。两组细胞生长曲线呈典型的“S”形,无统计学差异（P＞0.05）;成脂诱导14 d后,油红O染色呈阳性;成骨诱导2周时茜素红染色阳性,ALP表达活性随成骨诱导时间延长不断增加且无统计学差异（ P＞0.05）。结论冻存后的兔脂肪间充质干细胞体外生长及多向分化潜能未发生显著变化。     

猪骨髓基质干细胞低温生物学渗透特性的研究

以猪为材料利用细胞计数仪法研究了骨髓基质干细胞的渗透特性,包括细胞的等渗体积、低渗或高渗溶液中细胞的平衡体积及细胞的不可渗体积.结果表明,在等渗条件下,骨髓基质干细胞的平均体积为5248.4μm~3,相当直径d为21.6μm;细胞体积随溶液渗透压的变化规律符合Boyle van’t Hoff关系式,据此得到猪骨髓基质干细胞的不可渗体积V_b=0.36Vi,为1902.5μm~3.     

杂交瘤单克隆抗体研制中细胞的冻存与复苏

细胞的冻存与复苏是杂交瘤单克隆抗体(MCAb)研制中的一个重要环节.如果这个问题不解决,不但融合得不到成功,而且得到有价值的杂交瘤也会丧失掉.一、细胞的冻存在液氮中冷冻是保存杂交瘤细胞(或骨髓瘤细胞)最好的方法.在MCAb的研制中,一旦测得较有价值的阳性孔,就要一面进行克隆化,一面扩大培养,并冻存起来,以防体     

利用流式细胞术评价长期冻存对PBMCs各亚型的影响

目的:利用流式细胞术,检测长期冻存后PBMCs总数及各亚型的变化,评价PBMCs的长期冻存效果。方法:收集志愿者外周血PBMCs,利用流式细胞术分析液氮冻存后PBMCs细胞总数及其亚型的变化。结果:长期冻存后,PBMCs总细胞量和细胞活力无显著改变(P=0.19, P=0.32);T细胞、NK细胞和NKT细胞比例无明显变化,但B细胞比例增多(P0.01),单核细胞比例显著减少(P0.001);低温保存影响活化的T细胞和Tregs细胞数量(P0.05, P0.05),其中初始Tregs和记忆Tregs显著减少(P0.05,P0.01)。结论:PBMCs长期冻存会影响B细胞,单核细胞、活化T细胞和Tregs细胞的活性。     

人参总皂甙应用及改善细胞冻存的研究进展

人参作为一种名贵的药材,具有多方面的作用,近年来关于人参的成分之一人参总皂甙的研究也越来越多。大量实验研究表明,人参总皂甙对改善细胞冻存方面也有很大的作用。组织细胞经深低温冷冻技术处理后其活性能获得有效的保存,在液氮(-196℃)温度下,细胞、组织内各种酶的活力及代谢很低,几乎为零,生命处于所谓的"停滞"状态,在该状态下细胞的活性能得到最大限度的保存。目前常用的冷冻剂有海藻糖、丙二醇、丙三醇以及二甲基亚砜等。但这些冷冻剂均属于化学药剂,在一定程度上会对纤维细胞造成损伤,从而影响细胞的活性。人参总皂甙是从人参中提取出来的有效成分,其具有增强人体表面细胞活性,延缓细胞衰老的作用,为此本文将对人参总皂甙用于细胞冻存的效果进行综述,旨在为细胞的冻存技术提供参考依据。     

软骨细胞上清液诱导冻存复苏后人骨髓间充质干细胞的研究

目的:探讨人软骨细胞培养上清诱导冻存人骨髓充质干细胞向软骨细胞分化的可行性.方法:取进行全髋关节置换术老年患者的骨髓和软骨组织,利用密度梯度离心法、全骨髓培养法分别培养骨髓间充质干细胞,冻存备用.培养软骨细胞,观察细胞生长,收集软骨细胞培养上清.复苏冻存的人骨髓间充质干细胞,观察复苏后细胞生长状态.利用收集的软骨细胞培养上清对复苏间充质干细胞进行定向诱导,诱导培养2周,观察细胞外观表型变化,Ⅱ型胶原免疫组化检测诱导后人骨髓间充质干细胞Ⅱ型胶原的表达.结果:密度梯度离心法与全骨髓培养法均可分离获得人骨髓间充质干细胞,原代生长前者优于后者.复苏细胞仍进行可传代,与正常生长骨髓间充质细胞无明显差异,均可传至第8代.软骨细胞培养上清诱导2周后,细胞形状向圆形,多角形转变,冻存骨髓间充质干细胞Ⅱ型胶原免疫组化检测Ⅱ型胶原表达阳性.结论:老年人骨髓间充质干细胞仍具有向软骨细胞转化的能力,冻存不影响其转化能力.     

壳聚糖及其改性材料对骨髓基质细胞的作用

壳聚糖是一种广泛应用的生物可降解材料,该论文研究了几种与壳聚糖相关的材料对骨髓基质细胞生长和分化的作用,主要实验方法是在材料表面培养骨髓基质细胞并对其进行诱导促使其向成骨细胞方向分化。通过对细胞生长和分化情况的观察和测定,对几种材料与骨髓基质细胞的亲和性作出了评价。另外,通过ELISA法测定了细胞外基质分子在材料上的吸附量,测量了各材料的表面接触角以研究细胞在材料表面的铺展和增殖。结果表明尽管壳聚糖本身与骨髓基质细胞并不具有很好的亲和性,但通过与明胶混合,壳聚糖的生物相容性得到了明显提高,是很有应用前景的骨修复材料。     

鮸鱼精子的生理特性及超低温冻存

通过测定精子的激活率、运动时间及寿命,研究了鮸鱼精子的生理特性,以0.5mL麦细管为冻存管、两步降温法超低温冻存鮸鱼精子。结果表明,鮸鱼精子激活与运动的适宜盐度为20~30、适宜pH值为5.5~9.0,适宜的KCl、NaCl、CaCl2溶液浓度分别为（500~600）mmol/L、（400~500）mmol/L、（300~400）mmol/L,适宜的葡萄糖溶液浓度为（800~900）mmol/L。无Ca2＋、Mg2＋及HCO3-的人工海水均能使鮸鱼精子激活,但运动时间及寿命有所下降。以Cortland溶液为稀释液,10%Gly、15%Gly、5%DMSO、10%DMSO、15%DMSO、10%EG、10%PG、15%PG及20%PG为抗冻剂,超低温冻存鮸鱼精子15d后,冻精的活力与鲜精相比无显著差异,其中,以10%Gly为抗冻剂冻存精子的效果最好,冻精的激活率、运动时间及寿命分别达（86.38±1.63）%、（8.24±1.37）min及（10.21±0.42）min。     

Adenovirus-mediated BMP2 expression in human bone marrow stromal cells

Recombinant adenoviral vectors have been shown to be potential new tools for a variety of musculoskeletal defects. Much emphasis in the field of orthopedic research has been placed on developing systems for the production of bone. This study aims to determine the necessary conditions for sustained production of high levels of active bone morphogenetic protein 2 (BMP2) using a recombinant adenovirus type 5 (Ad5BMP2) capable of eliciting BMP2 synthesis upon infection and to evaluate the consequences for osteoprogenitor cells. The results indicate that high levels (144 ng/ml) of BMP2 can be produced in non-osteoprogenitor cells (A549 cell line) by this method and the resultant protein appears to be three times more biologically active than the recombinant protein. Surprisingly, similar levels of BMP2 expression could not be achieved after transduction with Ad5BMP2 of either human bone marrow stromal cells or the mouse bone marrow stromal cell line W20-17. However, human bone marrow stromal cells cultured with 1 microM dexamethasone for four days, or further stimulated to become osteoblast-like cells with 50 microg/ml ascorbic acid, produced high levels of BMP2 upon Ad5BMP2 infection as compared to the undifferentiated cells. The increased production of BMP2 in adenovirus transduced cells following exposure to 1 microM dexamethasone was reduced if the cells were not given 50 microg/ml ascorbic acid. When bone marrow stromal cells were allowed to become confluent in culture prior to differentiation, BMP2 production in response to Ad5BMP2 infection was lost entirely. Furthermore, the increase in BMP2 synthesis seen during differentiation was greatly decreased when Ad5BMP2 was administered prior to dexamethasone treatment. In short, the efficiency of adenovirus mediated expression of BMP2 in bone marrow stromal cells appears to be dependent on the differentiation state of these cells.     

骨髓基质细胞的特征及其在细胞和基因治疗中的应用

骨髓基质细胞是一类独特的间质干细胞,可分化为多种非造血系的组织。骨髓基质细胞具有贴壁生长的特性,因而易于在体外分离和扩增;另外骨髓基质细胞可在体内外表达多种治疗性的外湖目的基因。因此,骨髓基质细胞被认为是一种理想的治疗性细胞的基因治疗中的靶细胞。本文对骨髓基质细胞的研究进展及其在细胞和基因治疗中的应用作一综述。     

Inflammatory T cells rapidly induce differentiation of human bone marrow stromal cells into mature osteoblasts

Activated T cells secrete multiple osteoclastogenic cytokines which play a major role in the bone destruction associated with rheumatoid arthritis. While the role of T cells in osteoclastogenesis has received much attention recently, the effect of T cells on osteoblast formation and activity is poorly defined. In this study, we investigated the hypothesis that in chronic inflammation activated T cells contribute to enhanced bone turnover by promoting osteoblastic differentiation. We show that T cells produce soluble factors that induce alkaline phosphatase activity in bone marrow stromal cells and elevated expression of mRNA for Runx2 and osteocalcin. This data indicate that T cell derived factors have the capacity to stimulate the differentiation of bone marrow stromal cells into the osteoblast phenotype. RANKL mRNA was undetectable under any conditions in highly purified bone marrow stromal cells. In contrast, RANKL was constitutively expressed in primary osteoblasts and only moderately up-regulated by activated T cell conditioned medium. Interestingly, both bone marrow stromal cells and osteoblasts expressed mRNA for RANK, which was strongly up-regulated in both cell types by activated T cell conditioned medium. Although, mRNA for the RANKL decoy receptor, osteoprotegerin, was also up-regulated by activated T cell conditioned medium, it's inhibitory effects may be mitigated by a simultaneous rise in the osteoprotegerin competitor TNF-related apoptosis-inducing ligand. Based on our data we propose that during chronic inflammation, T cells regulate bone loss by a dual mechanism involving both direct stimulation of osteoclastogenesis, by production of osteoclastogenic cytokines, and indirectly by induction of osteoblast differentiation and up-regulation of bone turnover via coupling.     

人骨髓基质细胞向成骨细胞分化过程中差异表达基因的筛选

为了探讨人骨髓基质细胞（bone marrow stromal cells,BMSCs）向成骨细胞分化过程中差异表达的基因,本实验采用体外培养人BMSCs,诱导向成骨细胞分化。分别选取培养12和21d的细胞作为驱动方（driver）和实验方（tester）,进行抑制消减杂交,构建cDNA消减文库,将挑选出的阳性克隆与GenBank人基因库中己公布的核酸序列进行同源性比较分析。结果表明,从培养21d的BMSCs中,筛查出5个差异基因,与人基因库中己知基因的同源性分别达到90％以上。有兴趣的是,核心蛋白聚糖和Bax inhibitorl在培养2ld的BMSCs中差异表达。RT-PCR检测显示,核心蛋白聚糖基因在培养21d的细胞中高表达,而在12d的细胞中未检测到表达;Bax inhibitorl基因在培养21d细胞中的表达明显高于12d的细胞。     

无巨核细胞条件下促血小板生成素对骨髓基质细胞纤维形成的影响

目的：观察无巨核细胞存在的条件下促血小板生成素能否刺激骨髓基质细胞纤维形成。方法：用改良Dexter培养法进行体外不同浓度促血小板生成素（TPO）作用下的基质细胞培养,在培养过程中检测基质细胞相对增殖指数,纤维连接蛋白、层粘素和Ⅳ型胶原的表达,以及Ⅲ型前胶原蛋白的合成。结果：TPO可刺激基质细胞增殖,相对增殖指数随TPO浓度增加而增强,但不随作用时间延长而增强;纤维连接素、层粘素和Ⅳ型胶原在对照组与实验组均有阳性表达,但实验组强于对照组,但阳性强度不随培养时间的延长而增强;标记的Ⅲ型前胶原蛋白平均荧光强度实验组高于对照组,差异明显,但这种作用的强弱与TPO浓度相关性不强。结论：无巨核细胞存在的条件下,TPO可直接刺激骨髓基质细胞产生细胞外基质和胶原,促进其纤维形成。     

Bone marrow stromal cells produce nerve growth factor and glial cell line-derived neurotrophic factors

Bone marrow stromal cells (BMSC) have attracted interest through their possible use for cell therapy in neurological diseases. Recent reports demonstrated that these cells are able to migrate and have potential for neuronal differentiation after transplantation into brain parenchyma. The objective of this work was determine whether rat BMSC express NGF and GDNF, in order to study its potential application for treatment of neurodegenerative diseases. BMSC were harvested from male rats and cultured in DMEM supplemented with 20% fetal bovine serum. At passage 6 the total RNA was isolated using TriZol reactive. RT-PCRs to evaluate the expression of NGF and GDNF using specific primers were carried out. Our results indicate that rat BMSC have potential to produce NGF and GDNF. We have not found any report in favor of GDNF or NGF production from rat BMSC.     

Differentiation capacity of stromal fibroblast-like cells from human bone marrow, adipose tissue, hair follicle dermal papilla and derma

We compared the morphology and differentiation capacity of human stromal cells derived from bone marrow (BMSC), adipose tissue (ATSC), hair follicle dermal papilla (DPC) and dermal fibroblasts (DFb). All cells have fibroblast-like morphology. ATSC and DPC cells expressed stem cell the surface markers CD105, CD49d, and STRO-1, which were revealed immunocytochemically. CD49d was not found on BMSC. The low expression of CD49d and STRO-1 was registered in the DFb population. ATSC, BMSC, and DPC have similar capacities for adipo- and osteogenic differentiation. These cells, cultured in appropriate induction media, alter the phenotype and synthesize specific proteins. However, the expression of differentiation in the DPC population is lower than in ATSC and BMSC cultures. We propose that these cell populations have primitive progenitor cells with properties of mesenchymal stem cells.     

Isolation and expansion of high yield of pure mesenchymal stromal cells from fresh and cryopreserved placental tissues

The injection of placental stromal cells isolated from fetal human tissues (f-hPSC) was reported to indirectly induce tissue regeneration in different animal models. A procedure of f-hPSC isolation from fragments of both selected fresh or cryopreserved bulk placental neonate tissues is proposed, based on their high migratory potential,. The fragments of the desired fetal placental tissues are adhered to a culture dish by traces of diluted fibrin and covered with culture medium. Spontaneous migration of pure f-hPSC from the tissue fragments to the cell culture dishes is followed by their rapid expansion by numerous passages. The isolated f-hPSC express typical mesenchymal surface antigens, including CD29, CD105, CD166 and CD146, with negative expression of white blood cell lineage and endothelial cells markers. Optimal yields of f-hPSC cultures can also be obtained from tissue samples cryopreserved in medium composed of 10% dimethyl sulfoxide (M₂SO) and 50% fetal calf serum. Slightly better yields are obtained with media supplemented with 1% human albumin. Medium with 5% M₂SO and/or 0.25 mg/ml PEG yielded inferior results. The f-hPSC from fresh or cryopreserved tissues express similar cell markers and growth kinetics. The proposed isolation protocol may also be applied for high yield isolation of stromal cells from fresh and cryopreserved tissue of other organs.