RANKL signaling in bone marrow mesenchymal stem cells negatively regulates osteoblastic bone formation

RANKL signaling is essential for osteoclastogenesis. Its role in osteoblastic differentiation and bone formation is unknown. Here we demonstrate that RANK is expressed at an early stage of bone marrow mesenchymal stem cells(BMSCs) during osteogenic differentiation in both mice and human and decreased rapidly. RANKL signaling inhibits osteogenesis by promoting β-catenin degradation and inhibiting its synthesis. In contrast, RANKL signaling has no significant effects on adipogenesis of BMSCs.Interestingly, conditional knockout of rank in BMSCs with Prx1-Cre mice leads to a higher bone mass and increased trabecular bone formation independent of osteoclasts. In addition, rank: Prx1-Cre mice show resistance to ovariectomy-(OVX) induced bone loss. Thus, our results reveal that RANKL signaling regulates both osteoclasts and osteoblasts by inhibition of osteogenic differentiation of BMSCs and promotion of osteoclastogenesis.

miR-23a/b regulates the balance between osteoblast and adipocyte differentiation in bone marrow mesenchymal stem cells

Age-related osteoporosis is associated with the reduced capacity of bone marrow mesenchymal stem cells （BMSCs） to differentiate into osteoblasts instead of adipocytes. However, the molecular mechanisms that decide the fate of BMSCs remain unclear. In our study, microRNA-23a, and microRNA-23b （miR-23a/b） were found to be markedly downregulated in BMSCs of aged mice and humans. The overexpression of miR-23a/b in BMSCs promoted osteogenic differentiation, whereas the inhibition of miR-23a/b increased adipogenic differentiation. Transmembrane protein 64 （Tmem64）, which has expression levels inversely related to those of miR-23a/b in aged and young mice, was identified as a major target of miR-23a/b during BMSC differentiation. In conclusion, our study suggests that miR-23a/b has a critical role in the regulation of mesenchymal lineage differentiation through the suppression of Tmem64.

Effects of Panax notoginseng saponins on apoptosis induced by hydrogen peroxide in cultured rabbit bone marrow stromal cells via altering the oxidative stress level and down-regulating caspase-3

Objective： To investigate the effects of Panax notoginseng saponins （PNS） on hydrogen peroxide （H2O2）-induced apoptosis in cultured rabbit bone marrow stromal cells （BMSCs）. Methods： The effects of different concentrations of PNS on proliferation and early osteoblast differentiation of BMSCs were determined by the MTT assay and an alkaline phosphatase （ALP） assay. An optimal effective concentration of PNS was determined and used in subsequent experiments. The cultured BMSCs were divided into three groups： untreated control, H2O2 treated, and PNS pretreatment of H2O2 treated. The oxidative stress level was assessed by superoxide dismutase （SOD） and malondialdehyde （MDA） assays. Flow cytometry was used to determine BMSC apoptosis by staining with annexinV-FITC/propidium iodide （PI）. The activity of caspase-3 enzyme was measured by spectrofluorometry. Results： PNS （0.1g/L） significantly increased both BMSC proliferation rate and ALP activity, while it decreased the indicators of oxidative stress, caspase-3 activity, and the apoptosis rate of BMSCs induced by H2O2.. Conclusion： PNS, acting as a biological antioxidant, had a protective effect on H2O2-induced apoptosis in cultured rabbit BMSCs by decreasing oxidative stress and down-regulating caspase-3.

Nanofibrous Scaffold Containing Osteoblast-Derived Extracellular Matrix for the Proliferation of Bone Marrow Mesenchymal Stem Cells

Extracellular matrix( ECM) plays a prominent role in establishing and maintaining an appropriate microenvironment for tissue regeneration. The aims of this study were to construct a tissue engineered scaffold by reconstituting osteoblast cell-derived ECM( O-ECM) on the electrospun nanofibrous scaffold,and further to evaluate its subsequent application for promoting the proliferation of bone marrow mesenchymal stem cells( BMSCs). To engineer a biomimetic scaffold, calvarial osteoblasts and electrospun poly-llactic acid( PLLA) nanofibers were prepared and subjected to decellularize for O-ECM deposition. To evaluate and characterize the O-ECM/PLLA scaffold, the morphology was examined and several specific mark proteins of osteoblasts matrix were evaluated.Furthermore,the cell counting kit-8( CCK-8) assay was used to detect the proliferation of the BMSCs cultivated on the O-ECM/PLLA scaffold. The results indicated O-ECM/PLLA scaffold was loaded with Collagen I, Fibronectin, and Laminin, as the composition of the marrow ECM. After decellularization,O-ECM deposition was observed in O-ECM/PLLA scaffold. Moreover,the O-ECM/PLLA scaffold could significantly enhance the proliferation of BMSCs,suggesting better cytocompatibility compared to the other groups tested. Taken together,a biomimetic scaffold based on the joint use of O-ECM and PLLA biomaterials,which represents a promising approach to bone tissue engineering, facilitates the expansion of BMSCs in vitro.

Synergistic effects of brain-derived neurotrophic factor and retinoic acid on inducing the differentiation of bone marrow stromal cells into neuron-like cells in adult rats in vitro

BACKGROUND： Under induction of retinoic acid （RA）, bone marrow stromal cells （BMSCs） can differentiate into nerve cells or neuron-like cells, which do not survive for a long time, so those are restricted to an application. Other neurotrophic factors can also differentiate into neuronal cells through inducing BMSCs; especially, brain-derived neurotrophic factor （BDNF） can delay natural death of neurons and play a key role in survival and growth of neurons. The combination of them is beneficial for differentiation of BMSCs. OBJECTIVE： To investigate the effects of BDNF combining with RA on inducing differentiation of BMSCs to nerve cells of adult rats and compare the results between common medium group and single BDNF group. DESIGN： Randomized controlled animal study SETTING： Department of Neurology, Affiliated Hospital of Xuzhou Medical College MATERIALS： The experiment was carried out in the Clinical Neurological Laboratory of Xuzhou Medical College from September 2003 to April 2005. A total of 24 SD rats, of either gender, 2 months old, weighing 130-150 g, were provided by Experimental Animal Center of Xuzhou Medical College [certification： SYXK （su） 2002-0038]. Materials and reagents： low-glucose DMEM medium, bovine serum, BDNF, RA, trypsin, separating medium of lymphocyte, monoclonal antibody of mouse-anti-nestin, neuro-specific enolase, glial fibrillary acidic protein （GFAP） antibody, SABC kit, and diaminobenzidine （DAB） color agent. All these mentioned above were mainly provided by SIGMA Company, GIBCO Company and Boshide Company. METHODS： Bone marrow of SD rats was selected for density gradient centrifugation. BMSCs were undertaken primary culture and subculture; and then, those cells were induced respectively in various mediums in total of 3 groups, including control group （primary culture）, BDNF group （20 μg/L BDNF） and BDNF＋RA group （20 μg/L BDNF plus 20 μg/L RA）. On the 3^rd and the 7^th days after induction, BMSCs were stained immunocytochemically with nestin （sign of nerve stem cells）, neuron-specific enolase （NSE, sign of diagnosing neurons） and GFAP （diagnosing astrocyte）, and evaluated cellular property. MAIN OUTCOME MEASURES ： Induction and differentiation in vitro of BMSCs in 3 groups RESULTS： （1） Induction and differentiation of BMSCs： Seven days after induction, cells having 2 or more apophyses were observed. Soma shaped like angle or erose form, which were similar to neurons and glial cells having strong refraction. （2） Results of immunocytochemical detection： Three days after induction, rate of positive cells in BDNF＋RA group was higher than that in BDNF group and control group [（86.15±4.58）%, （65.43±4.23）%, （4.18±1.09）%, P 〈 0.01]. Seven days after induction, rate of positive cells was lower in BDNF group and BDNF＋RA group than that in both groups at 3 days after induction [（31.12±3.18）%, （29.35±2.69）%, P 〈 0.01]; however, amounts of positive cells of NSE and GFAP were higher than those at 3 days after induction （P 〈 0.01）; meanwhile, the amount in BDNF＋RA group was remarkably higher than that in BDNF group （P 〈 0.01）. CONCLUSION： Combination of BDNF and RA can cooperate differentiation of BMSCs into neurons and astrocyte, and the effect is superior to single usage of BDNF.

The effect of neuropeptides on proliferation of rat bone marrow mesenchymal stem cells

Objective To investigate the effects and mechanism of calcitonin gene-related peptide(CGRP)and substance P (SP) on proliferation of rat bone marrow mesenchymal stem cells.Methods The rBMSCs were isolated using whole bone marrow

The future of bone marrow stromal cell transplantation for the treatment of spinal cord injury

Bone marrow stromal cell （BMSC） transplantation therapy is a promising approach for treating spinal cord injury （SCI）, based on a number of experimental and clinical reports （Wright et al., 2011）. BMSCs are a source of neuroregenerative somatic stem cells that are without the potential for tumorigenicity. Although clinical studies of autologous BMSC transplantation have been reported in Asia （fiang et al., 2013; Yoon et al., 2007）, in Japan, it is currently an uncommon procedure and highly controversial as well. This perspective paper provides an overview of the clinical effectiveness of BMSC trans- 191antation and a proposal to enhance its use as a viable therapy.

转染BMP-2基因的兔BMSCs种植PLA/PCL支架体外构建组织工程骨

目的 :用腺病毒载体将人骨形态发生蛋白 2 (BMP 2 )基因导入兔骨髓基质干细胞 (BMSCs) ,种植PLA/PCL (聚乳酸 /聚己内酯 )支架体外构建组织工程骨。方法 :蛋白印迹法检测转染后细胞BMP 2的表达 ,流式细胞仪和ALP活性检测分析基因转染对细胞增殖分化的影响。然后将转染后细胞接种到PLA/PCL支架上 ,扫描电镜观察细胞贴附、生长状况。结果 :转染后 ,BMSCs表达BMP 2 ,S期细胞比例和ALP活性明显增高。扫描电镜见转染细胞分布均匀 ,伸展良好。结论 :BMP 2基因转染BMSCs ,可促进细胞增殖分化。转染后细胞在PLA/PCL支架上生长良好 ,BMP 2基因治疗的组织工程骨构建成功。

BMPs信号通路在压力调控兔BMSCs成软骨响应中的作用

目的:探讨骨形态发生蛋白(bone morphogenetic protein,BMPs)信号通路在压力刺激兔骨髓间充质干细胞(bone marrow-derived mesenchymal stem cells,BMSCs)成软骨响应中的作用。方法:体外分离、培养兔BMSCs,经鉴定后随机分为4组:空白对照组、压力刺激组、BMPs拮抗剂Noggin刺激组、压力+BMPs拮抗剂Noggin刺激组,其中压力刺激组和压力联合Noggin刺激组置于静态液压细胞加载装置中培养,并给予120 kPa、每天1 h、连续4 d的力学刺激。Real-time PCR和Western Blot方法检测压力刺激前后细胞中BMPs信号相关分子BMP2、Smad1、Smad5表达的变化;Western Blot方法检测4个实验组中P-Smad1/Smad5和软骨特异性基因Col-II、Aggrecan的蛋白表达。结果:兔BMSCs传代后细胞生长状态稳定,细胞表面标记物CD29阳性率97.2%、CD44阳性率93.2%、CD45阳性率0.8%;成骨诱导3周后,茜素红染色可见矿化结节形成;成脂诱导2周后,油红O染色可见红色脂滴;压力刺激后BMP2、Smad1、Smad5的基因与蛋白表达均明显增加(P<0.05);Western Blot检测显示,压力加载方式作用于兔BMSCs后,软骨细胞特异性指标Col-Ⅱ、Aggrecan的表达明显上调(P<0.05);BMPs特异性拮抗剂Noggin能明显抑制压力刺激兔BMSCs中P-Smad1/Smad5、Col-Ⅱ、Aggrecan的蛋白表达。结论:BMP/Smad信号通路介导了压力刺激兔BMSCs成软骨响应的过程。

rhBMP-2体外诱导骨质疏松大鼠BMSCs成骨及VEGF表达的研究

目的 :观察骨形态发生蛋白-2对骨质疏松时骨髓基质干细胞(BMSCs)体外成骨及成骨因子VEGF表达的影响,为骨质疏松证的防治提供新的方法。方法:将20只6月龄,体重(300±20)g雌性SD大鼠双侧卵巢切除,术后3个月利用双能X线骨密度仪测量大鼠全身骨密度并与术前比较,确保造模成功,并运用全骨髓贴壁法培养骨质疏松大鼠BMSCs,倒置相差显微镜下观察BMSCs形态。随机把骨质疏松大鼠BMSCs第2代(p2)细胞分成实验组和对照组,分别加入完全培养基(含rh BMP-2)、成骨诱导液进行成骨诱导。2周后茜素红染色法检测各组细胞钙结节的形成,酶标仪测定碱性磷酸酶活性及RT-PCR法检测VEGF的表达量。结果:(1)大鼠全身骨密度:手术前后大鼠全身骨密度分别为(0.179±0.007),(0.158±0.006)g/cm2,差异有统计学意义(t=4.180,P<0.05)。(2)茜素红染色:BMSCs(P2)成骨诱导2周后实验组染色效果明显强与对照组。(3)碱性磷酸酶活性:BMSCs(P2)成骨诱导2周后碱性磷酸酶活性实验组明显高于对照组,分别为(15.62±1.27),(8.62±0.93)μg/prot,差异有统计学意义(t=7.709,P<0.01)。(4)BMSCs(P2)成骨诱导2周后VEGF表达:实验组明显高于对照组,分别为3.723±0.143,0.950±0.072,差异有统计学意义(t=29.462,P<0.01)。结论 :rh BMP-2能提高去卵巢骨质疏松大鼠BMSCs的体外成骨能力,可促进成骨因子VEGF的表达,调控VEGF的表达可能是骨形态发生蛋白-2参与骨代谢的机制之一。

BMSCs与PLGA支架构建组织工程化骨软骨复合组织

目的:探讨同种异体骨髓间充质干细胞(bone mesenchymal stem cells,BMSCs)体外分离培养后种植到孔径和孔隙率不同且复合不同胶原和生长因子的PLGA支架上再种植到大鼠肌袋内构建组织工程化骨软骨复合组织的可行性。方法:制作复合BMP-2和Ι型胶原PLGA支架与复合bFGF、TGF-β1和Ⅱ型胶原PLGA支架后把两者用生物蛋白胶粘合形成复合支架,把体外培养扩增的BMSCs种植到复合支架上,植入实验组A组、对照组B组、空白组C组SD大鼠肌袋内,于术后4、8、12周取材,分别行大体观察、HE染色、甲苯胺蓝染色、Ⅱ型胶原免疫组化、ALP染色、扫描电镜、透视电镜观察。结果:实验组大体标本成骨区呈白色类骨样组织,质硬,成软骨区呈乳白色类软骨样组织,质较硬,两区融合;扫描电镜观察可见成骨细胞、破骨细胞及软骨细胞,透视电镜尚可见细胞浆内有大量的线粒体和内质网,并见大量胶原分泌,与对照组、空白组有明显区别,组织学评分表明A组较B、C两组差异具有统计学意义(P<0.05)。结论:BMSCs体外分离扩增后种植到孔径和孔隙率不同且复合不同胶原和生长因子的PLGA支架上再植入动物肌袋可构建骨软骨复合组织。

hBMP-2基因修饰自体BMSCs移植促进兔下颌骨牵张成骨新骨形成的X线分析

目的:探讨hBMP-2基因修饰自体BMSCs移植对兔下颌骨牵张成骨新骨形成的促进作用。方法:取新西兰白兔36只随机分为3组,每组12只。建立牵张成骨动物模型,在固定期第2天,实验组于牵张间隙注射200μl的BMP-2基因修饰的自体BMSCs(2×105个细胞)悬液;对照组注射200μl的自体BMSCs(2×105个细胞)悬液;空白组注射200μl生理盐水。分别于固定2、6周摄X线片观察骨质愈合、改建情况。结果:通过X线观察并经过灰度值统计软件分析,在固定期2周及6周实验组牵张区骨密度明显高于对照组和空白组(P<0.01)。结论:BMP-2基因修饰的自体BMSCs移植能有效促进兔下颌骨牵张成骨新骨形成。

IFN-γ对犬BMSCs增殖及分泌多种免疫抑制因子的影响

目的:探讨IFN-γ对犬BMSCs增殖及分泌多种免疫抑制因子能力的影响。方法:从犬骨髓中分离培养BMSCs,通过免疫化学和诱导分化进行鉴定。利用梯度浓度IFN-γ刺激BMSCs,CCK-8检测细胞增殖情况;RT-qPCR检测BMSCs表面受体TLR3、TLR4的表达情况,免疫抑制基因IDO1、IDO2、COX2的表达情况;ELISA检测BMSCs分泌的IL-10、HGF、TGF-β、PGE2和犬尿氨酸的含量。结果:与对照组相比,经IFN-γ刺激后能有效促进BMSCs的增殖,差异有统计学意义(P<0.05);BMSCs表达TLR3、IDO1、COX2上调,差异有统计学意义(P<0.05),TLR4、IDO2的表达,差异有统计学意义(P>0.05);可溶性免疫抑制因子IL-10、HGF、犬尿氨酸的分泌增加,而PGE2和TGF-β的分泌降低,差异有统计学意义(P<0.05)。结论:IFN-γ促进犬BMSCs的增殖并且能够诱导BMSCs表达免疫抑制因子,提高其分泌可溶性抗炎因子的能力,提示IFN-γ在一定条件下可促进BMSCs的免疫抑制能力。

压力对骨髓间充质干细胞(BMSCs)膜片复合富血小板纤维蛋白(PRF)双膜结构中BMSCs成软骨能力的影响

目的:观察压力对骨髓间充质干细胞(Bone marrow mesenchymal stem cells,BMSCs)复合富血小板纤维蛋白(Platelet-rich Fibrin,PRF)(BMSCs/PRF)双膜结构中BMSCs的成软骨能力。方法:密度梯度离心法分离培养兔骨髓间充质干细胞,经表面标记分子检测及成骨、成脂能力鉴定后,制备细胞膜片。将取自同一个体的兔耳廓动脉全血通过离心获得PRF,将PRF压制成膜后与BMSCs细胞膜片复合并进行混合培养。培养2 d后按不同力值将复合膜随机分为0 kPa(对照)、90、120、150 kPa 4大组;每一大组再分为刺激1 h/d、6 h/d两组,然后置于加载装置中按分组分别施以不同静态压力。分别于加载第2、4、6天终止培养、取材;Real-time PCR法检测PCNA、SOX-9、Aggrecan、COL-ⅡmRNA表达水平。结果:实验所设定的各组压力刺激条件均可对双膜结构中的BMSCs产生显著的促增殖效应,其中以120 kPa/1 h持续4 d的压力条件下PCNA基因表达水平最高。2 d压力刺激明显上调Aggrecan水平,而对SOX-9与COL-Ⅱ的表达无显著作用;4 d压力刺激可同时促进Aggrecan、SOX-9及COL-Ⅱ mRNA的表达,其中以120 kPa/1 h/4 d的压力条件下的成软骨基因表达水平最高;6 d压力刺激下仅在90、120 kPa加压1 h时表现出对COL-Ⅱ mRNA的促进作用。结论:适当的压力刺激可明显促进BMSCs/PRF双膜结构中BMSCs的增殖与软骨向分化能力。

犬PRF复合BMSCs修复拔牙窝颊侧骨壁缺损的实验研究

目的:评价富血小板纤维蛋白(PRF)构建的组织工程骨,在颊侧骨壁缺损修复中的成骨作用。方法:体外将PRF作用于比格犬的骨髓间充质干细胞(BMSCs),第21天测定钙结节量;4、7、11 d时采用实时定量PCR法检测成骨相关基因。9只成年比格犬拔除上颌左右两侧的侧切牙,构建颊侧骨壁缺损的拔牙位点,并随机分为血凝块组、PRF组和组织工程骨组,在手术后即刻、6周及12周时评价各组的颊侧骨高度和拔牙窝的骨密度。结果:PRF在体外实验中能明显促进BMSCs的增殖,提高成骨分化以及钙化能力(P<0.05)。动物实验中,PRF表现出了促进早期伤口愈合的能力。在颊侧骨壁缺损的修复中,组织工程组在6周时骨高度和骨密度分别为(2.63±0.57)mm、(765.19±59.70)HU,较血凝块组[(5.65±2.91)mm、(599.08±53.88)HU]和PRF组[(4.14±1.16)mm、(644.76±65.39)HU]显著增高(P<0.05)。结论:PRF复合BMSCs构建的组织工程骨可以在早期有效地修复拔牙窝骨壁缺损。

BMSCs的分离培养、纯化与鉴定

目的建立一种持续、稳定的可多向分化的骨髓间充质干细胞(BMSCs)体外分离培养体系。方法运用密度梯度离心法从1月龄新西兰兔骨髓中分离培养BMSCs,利用相差显微镜观察其形态及生长情况,扫描电镜观察其细胞结构,运用流式细胞术分析分离细胞群所处细胞周期和细胞活力,用MTT比色法绘制细胞生长曲线,并用特定诱导液将分离的BMSCs向成骨细胞和成脂肪细胞定向诱导分化,利用ALP和油红O进行染色鉴定。结果所分离的BMSCs细胞在形态学观察与生长动力学上均符合BMSCs特征,分离培养的BMSCs细胞在第3天进入对数生长期,第10天进入平台期;在成骨、成脂肪的诱导培养条件下,分别出现成骨、成脂肪表型特征,可进一步定向分化,结论所收获的细胞具有BMSCs的特异性。

腺苷酸环化酶(AC)基因家族在小鼠骨髓间充质干细胞(BMSCs)中的表达

骨髓间充质干细胞(bone marrow stromal cells,BMSCs)是骨髓中具有多向分化潜能的干细胞,腺苷酸环化酶(adenylyl cyclase,AC)作为第二信使c AMP信号通路的重要组分,在BMSCs的成骨/成脂分化中具有重要作用,但BMSCs中AC亚型表达种类,尚待明了。通过对小鼠BMSCs原代培养条件优化,获得最适培养条件下生长良好的细胞,提取其总RNA并反转录;采用RT-PCR和序列比对分析,鉴定了小鼠BMSCs中AC亚型的表达种类。研究发现:1小鼠BMSCs原代培养:以4.0×106cell/m L的骨髓单核细胞浓度培养,并于4 d首次换液,增殖速度快,可以达到后续实验要求;2原代小鼠BMSCs中AC亚型表达种类分别为AC2、AC3、AC4、AC6、AC7和AC9。

腺病毒介导hBMP-2转染BMSCs复合DBM修复兔缺血性股骨头坏死的实验研究

目的评价人骨形态发生蛋白(h BMP)-2/骨髓间充质干细胞(BMSCs)/脱钙松质骨(DBM)对兔股骨头坏死的修复作用,探索临床治疗股骨头坏死的新途径。方法髓芯减压联合液氮冰冻法制备兔股骨头坏死模型。将造模成功兔随机分为A、B、C、D 4组(n=12),A组不植入材料,为对照组,B、C、D分别植入DBM、DBM/BMSCs、h BMP-2/BMSCs/DBM。术后4、8及12周各组分别处死4只,运用X线技术、大体标本观察、HE染色技术评判股骨头坏死修复情况。结果 X线示A组股骨头塌陷,无明显成骨;B、C、D组股骨头缺损区有骨再生现象,但D组再生情况明显优于B、C组。Lane-Sandhu X线评分A组<B、C组<D组(P<0.05),B和C组差异无统计学意义。大体观示A组股骨头塌陷,钻孔存在;B、C组股骨头未塌陷,钻孔存在;D组股骨头未塌陷,钻孔消失。HE染色示A组骨小梁坏死、碎裂,大量空骨陷窝;B、C组可见成骨细胞及新生幼稚骨小梁;D组大量骨细胞,新生骨小梁与正常骨小梁无异。空骨陷窝率A组>B、C组>D组(P<0.05),B和C组差异无统计学意义。结论 h BMP-2/BMSCs/DBM植入体内后能够诱导BMSCs向成骨方向分化,对兔股骨头坏死具有较好的修复效果。