AAV-mediated expression of p65shRNA and bone morphogenetic protein 4 synergistically enhances chondrocyte regeneration

BACKGROUND:Adeno-associated virus(AAV)gene therapy has been proven to be reliable and safe for the treatment of osteoarthritis in recent years.However,given the complexity of osteoarthritis pathogenesis,single gene manipulation for the treatment of osteoarthritis may not produce satisfactory results.Previous studies have shown that nuclear factorκB could promote the inflammatory pathway in osteoarthritic chondrocytes,and bone morphogenetic protein 4(BMP4)could promote cartilage regeneration.OBJECTIVE:To test whether combined application of AAV-p65shRNA and AAV-BMP4 will yield the synergistic effect on chondrocytes regeneration and osteoarthritis treatment.METHODS:Viral particles containing AAV-p65-shRNA and AAV-BMP4 were prepared.Their efficacy in inhibiting inflammation in chondrocytes and promoting chondrogenesis was assessed in vitro and in vivo by transfecting AAV-p65-shRNA or AAV-BMP4 into cells.The experiments were divided into five groups:PBS group;osteoarthritis group;AAV-BMP4 group;AAV-p65shRNA group;and BMP4-p65shRNA 1:1 group.Samples were collected at 4,12,and 24 weeks postoperatively.Tissue staining,including safranin O and Alcian blue,was applied after collecting articular tissue.Then,the optimal ratio between the two types of transfected viral particles was further investigated to improve the chondrogenic potential of mixed cells in vivo.RESULTS AND CONCLUSION:The combined application of AAV-p65shRNA and AAV-BMP4 together showed a synergistic effect on cartilage regeneration and osteoarthritis treatment.Mixed cells transfected with AAV-p65shRNA and AAV-BMP4 at a 1:1 ratio produced the most extracellular matrix synthesis(P<0.05).In vivo results also revealed that the combination of the two viruses had the highest regenerative potential for osteoarthritic cartilage(P<0.05).In the present study,we also discovered that the combined therapy had the maximum effect when the two viruses were administered in equal proportions.Decreasing either p65shRNA or BMP4 transfected cells resulted in less collagen II synthesis.This implies that inhibiting inflammation by p65shRNA and promoting regeneration by BMP4 are equally important for osteoarthritis treatment.These findings provide a new strategy for the treatment of early osteoarthritis by simultaneously inhibiting cartilage inflammation and promoting cartilage repair.

Construction of Adeno-associated Virus System for Human Bone Morphogenetic Protein 7 Gene

To construct the recombinant adeno-associated virus （rAAV） vector with human bone morphogenetic protein 7 （BMP7） and observe the BMP7 mRNA expression in vitro, BMP7 CDS sequence was cloned into expression plasmid pAAV-MCS of AAV Helper Free System. The recombinant plasmid was identified with enzyme digestion and sequencing. The recombinant plasmid, pAAV-RC, pHelper were co-transfected into AAV-293 cells according to the calcium phosphate-based protocol. The viral stock was collected by 4 rounds of freeze/thaw. After purified and concentrated, the recombinant virus titer was determined by dot-blot assay. HEK293 cells were transfected with the recombinant virus at different MOI, and the expression of BMP7 mRNA was detected by RT-PCR. The results showed rAAV-BMP7 was constructed and packaged successfully. The physical particle titer was 2.5×10^11 vector genomes/mL. There was different expression level of BMP7 mRNA after transfecton. These data suggested that recombinant AAV mediated a stable expression of hBMP7 mRNA in 293 cells. The AAV production method may pave the way of an effective strategy for the jaw bone defection around dental implants.

CO-TRANSFECTION OF RAT BONE MARROW MESENCHYMAL STEM CELLS WITH HUMAN BMP2 AND VEGF165 GENES

Objective To explore the feasibility and efficacy of lentivirus-mediated co-transfection of rat bone marrow mesenchymal stem cells （MSCs） with human vascular endothelial growth factor 165 （hVEGFI65） gene and human bone morphogenetic protein 2 （hBMP2） gene. Methods The hVEGF165 and hBMP2 cDNAs were obtained from human osteosarcoma cell line MG63 and cloned into lentiviral expression vectors designed to co-express the copepod green fluorescent protein （copGFP）. The expression lentivector and packaging Plasmid Mix were co-transferred to 293TN cells, which produced the lentivirus carrying hVEGF165 （Lv-VEGF） or hBMP2 （ Lv-BMP） , respectively. MSCs of Wistar rats were co-transfected with Lv-BMP and Lv-VEGF （BMP ＋ VEGF group）, or each alone （BMP group and VEGF group）, or with no virus （ Control group）. The mRNA and protein expressions of hVEGF165 and hBMP2 genes in each group were detected by real-time PCR and enzyme linked immunosorbent assay （ELISA）. Results Lentiviral expression vectors carrying hVEGF165 or hBMP2 were correctly constructed and confirmed by restriction endonucleses analysis and DNA sequencing analysis. A transfer efficiency up to 90% was archieved in all the transfected groups detected by the fraction of fluorescent cells using fluorescent microscopy. From the results generated by real-time PCR and ELISA, VEGF165 and BMP2 genes were co-expressed in BMP ＋ VEGF group. No significant difference of BMP2 expression was detected between BMP ＋ VEGF and BMP groups （ P 〉 0. 05）. Similarly, there was no significant difference of VEGF165 expression between BMP ＋ VEGF and VEGF groups （ P 〉 0. 05）. Conclusion VEGF165 and BMP2 genes were successfully co-expressed in MSCs by lentivirus-mediated co-transfection, which provided a further foundation for the combined gene therapy of bone regeneration.

人骨形态发生蛋白12基因重组腺病毒载体的构建

目的:构建及制备人骨形态发生蛋白12(BMP12)基因重组腺病毒,证明其可感染脂肪组织来源干细胞并表达蛋白。方法:将包含有BMP12cDNA全长序列的BMP12-pED6质粒用限制性内切酶EcoRI进行酶切,得到一个1260bp大小的含有BMP12cDNA的目的基因片段。将目的基因片段插入质粒pcDNA3.1后,用KpnI和PmeI进行双酶切,插入pAdtrack-CMV。插入目的基因片段的穿梭质粒pAdtrack-CMV-BMP12用PmeI进行酶切线性化后与腺病毒骨架载体pAdEasy-1一起电转化入感受态BJ5183菌株。用PCR及多种酶切方法鉴定重组体。最终将线性化的重组质粒利用脂质体转入293A细胞中进行病毒包装。BMP12基因随着重组腺病毒在感染的293A细胞中扩增而得到复制,并通过CsCl梯度离心法得以纯化。Elisa法检测Ad-BMP12感染脂肪组织来源干细胞后BMP12的蛋白表达。结果:pAdtrack-CMV-BMP12经酶切证实有1260bp的插入片段。酶切及PCR鉴定证实BMP12基因重组腺病毒载体构建成功。GFP(green fluorescent protein)表明重组腺病毒扩增成功并制备出高滴度重组病毒。该重组病毒可成功感染脂肪来源组织干细胞并表达BMP12蛋白。结论:BMP12基因能够重组于腺病毒载体,可以进行有效扩增,产生高浓度的重组腺病毒,从而用于BMP12基因治疗的研究。

双基因rhBMP-4/VEGF_(121)在治疗兔桡骨缺损中的作用

目的研究双基因rhBMP-4/VEGF121混悬液在骨缺损修复中的作用。方法新西兰成年兔20只,制作40侧桡骨中段15mm骨缺损实验模型,随机分为A、B、C、D组。A组植入rhBMP-4+VEGF121+明胶海绵,B组植入rhBMP-4+明胶海绵,C组植入VEGF121+明胶海绵,D组只植入明胶海绵。并于术后4、8、12周对骨缺损区进行大体、X线片、组织形态学观察,图像分析新生骨小梁的面积。结果A组在12周内骨缺损完全修复,髓腔再通,且同时期内新生骨的数量和质量显著优于其他组;B、C组骨缺损为未完全成熟的板层骨修复,髓腔部分再通,B组骨愈合成熟度较C组佳;D组缺损主要由纤维结缔组织填充。结论双基因rhBMP-4/VEGF121治疗骨缺损比单基因具有更好的促进骨修复再生能力。

BMP12诱导恒河猴骨髓间充质干细胞定向分化为腱细胞

目的:研究骨髓间充质干细胞定向分化为腱细胞的可能性。方法:通过电穿孔法将外源基因BMP12导入骨髓间充质干细胞中,诱导骨髓间充质干细胞定向分化为腱细胞;在形态学和分子生物学水平上对诱导后的细胞加以鉴定。结果:光镜下,诱导后的细胞形态发生明显改变;RT-PCR结果表明,诱导后的细胞有BMP12和CollagenⅠ的mRNA的表达,而没有CollagenⅢ的mRNA表达;诱导后细胞呈CD44+为98.39%,HLA-DR-。结论:BMP12能够诱导骨髓间充质干细胞定向分化为腱细胞,间充质干细胞有可能成为肌腱组织工程种子细胞来源之一。

二种不同病毒基因表达调节元件对骨多形性蛋白12基因在COS细胞中的表达影响

目的 比较巨细胞病毒的早期启动子和腺病毒主要晚期启动子(MPL)、三联前导序列(TPL)和插入序列 (IVS)组合对BMP12在COS细胞中表达的影响。方法 BMP12cDNA分别克隆在pED载体中的腺病毒主要晚期 启动子(MPL)、三联前导序列(TPL)和插入序列(IVS)组合下游,构建了表达质粒BMP12/pED。及克隆在AD1- 1载体中巨细胞病毒的早期启动子下游,构建了表达质粒BMP12/AD1 1。采用脂质体法将二个表达质粒分别转 染入COS细胞。40h及60h后,分别取100μl培养上清进行Western印迹,检测所表达的BMP12蛋白。结果 Western印迹结果显示:转染40hr后,只在BMP12/pED转染的COS细胞培养液检测出2个BMP12特异表达产 物,大小约为50kD和44kD(较弱)。转染60h后,BMP12/Ad1 1转染的COS细胞培养液有3个BMP12特异表达 产物,大小约为:50kD、40kD、15kD;BMP12/pED转染细胞培养液有4个BMP12特异表达产物,大小约为:50kD、 48kD、44kD、15kD。结论 腺病毒主要晚期启动子(MPL)、三联前导序列(TPL)和插入序列(IVS)组合的基因表 达调节元件驱动的BMP12表达量高于巨细胞病毒的早期启动子;二种病毒基因表达调节元件驱动的BMP12表达 产物的种类与大小均有差异。

Osteogenic potential of the human bone morphogenetic protein 2 gene activated nanobone putty

Background Nanobone putty is an injectable and bioresorbable bone substitute. The neutral-pH putty resembles hard bone tissue, does not contain polymers or plasticizers, and is self-setting and nearly isothermic, properties which are helpful for the adhesion, proliferation, and function of bone cells. The aim of this study was to investigate the osteogenic potential of human bone morphogenetic protein 2 （hBMP2） gene activated nanobone putty in inducing ectopic bone formation, and the effects of the hBMP2 gene activated nanobone putty on repairing bone defects. Methods Twenty four Kunming mice were randomly divided into two groups. The nanobone putty ＋ hBMP2 plasmid was injected into the right thigh muscle pouches of the mice （experiment side）. The nanobone putty ＋ blank plasmid or nanobone putty was injected into the left thigh muscle pouches of the group 1 （control side 1） or group 2 （control side 2）, respectively. The effects of ectopic bone formation were evaluated by radiography, histology, and molecular biology analysis at 2 and 4 weeks after operation. Bilateral 15 mm radial defects were made in forty-eight rabbits. These rabbits were randomly divided into three groups： Group A, nanobone putty ＋ hBMP2 plasmid; Group B, putty ＋ blank plasmid; Group C, nanobone putty only. Six rabbits with left radial defects served as blank controls. The effect of bone repairing was evaluated by radiography, histology, molecular biology, and biomechanical analysis at 4, 8, and 12 weeks after operation. Results The tissue from the experimental side of the mice expressed hBMP2. Obvious cartilage and island-distributed immature bone formation in implants of the experiment side were observed at 2 weeks after operation, and massive mature bone observed at 4 weeks. No bone formation was observed in the control side of the mice. The ALP activity in the experiment side of the mice was higher than that in the control side. The tissue of Group A rabbits expressed hBMP2 protein and higher ALP level. The new bone formation rate and antibending strength of group A was significantly higher than those of group B and C. The defects in blank control were not healed. Conclusions The hBMP2 gene activated nanobone putty exhibited osteoinductive ability, and had a better bone defect repair capabilitv than that of nanobone putty only.

Ectopic bone formation of human bone morphogenetic protein-2 gene transfected goat bone marrow-derived mesenchymal stem cells in nude mice

Objective: To evaluate the osteogenic potential of bone morphogenetic protein (BMP)-2 gene transfected goat bone marrow-derived mesenchymal stem cells (MSCs). Methods: Goat bone marrow- derived MSCs were transfected by Adv-human bone morphogenetic protein (hBMP)-2 gene(Group 1), Adv-beta gal transfected MSCs (Group 2)and uninfected MSCs(Group 3). Western blot analysis, alkaline phosphatase staining, Von Kossa staining and transmission electron microscopy were adopted to determine the phenotype of MSCs. Then the cells were injected into thigh muscles of the nude mice. Radiographical and histological evaluations were performed at different intervals. Results: Only Adv-hBMP-2 transfected MSCs produced hBMP-2. These cells were positive for alkaline phosphatase staining at the 12th day and were positive for Von Kossa staining at the 16th day after gene transfer. Electron microscopic observation showed that there were more rough endoplasmic reticulum, mitochondria and lysosomes in Adv-hBMP-2 transfected MSCs compared to MSCs of other two groups. At the 3rd and 6th weeks after cell injection, ectopic bones were observed in muscles of nude mice of Group 1. Only fibrous tissue or a little bone was found in other two groups. Conclusions: BMP-2 gene transfected MSCs can differentiate into osteoblasts in vitro and induce bone formation in vivo.

BMP12诱导恒河猴骨髓间充质干细胞定向分化为腱细胞(英文)

目的 研究骨髓间充质干细胞定向分化为腱细胞的可能性。方法 通过电穿孔法将外源基因BMP12导入骨髓间充质干细胞中 ,诱导骨髓间充质干细胞定向分化为腱细胞 ;在形态学和分子生物学水平上对诱导后的细胞加以鉴定。结果 光镜下 ,诱导后的细胞形态发生明显改变 ;RT PCR结果表明 ,诱导后的细胞有BMP12和CollagenⅠ的mRNA表达 ,而没有CollagenⅢ的mRNA表达 ;诱导后98 39%的细胞呈CD4 4 + 、HLA DR-。结论 BMP12能够诱导骨髓间充质干细胞定向分化为腱细胞 ,间充质干细胞有可能成为肌腱组织工程种子细胞来源之一。

骨形成蛋白-2基因转染人骨髓间质干细胞诱导异位成骨的实验研究

目的 评价腺病毒介导的人骨形成蛋白 - 2基因 (Adv- h BMP- 2 )转染人骨髓间质干细胞 (MSCs)的诱导成骨能力。方法 从人骨髓中分离培养获取 MSCs,分为三组 :1Adv- h BMP- 2转染细胞组 ;2 Adv- βgal转染细胞组 ;3未转染细胞组。分别于体外行 Western immunoblot试验、碱性磷酸酶 (AL P)和 Von Kossa染色、AL P定量测定 ,以及裸鼠肌内诱导成骨试验。共 9只裸鼠 ,双侧股后肌群内注射 ,每组 6侧。结果 Adv- h BMP- 2组 MSCs可分泌 BMP- 2蛋白 ;转染后第 9天 AL P染色多数细胞为阳性 ,其它两组 AL P染色阳性细胞少见 ;AL P活性第 3天开始升高 ,12天达高峰为 14 .76单位 ,与其它两组比较有统计学意义 (P<0 .0 5 ) ;于第 2 1天后出现钙结节 ,而其它两组未见。裸鼠肌内注射后 4周 Adv- h BMP- 2组 X线片均有异位成骨 ,Adv- βgal转染细胞组未见明显成骨 ,未转染细胞组仅有少量骨形成。组织学检查发现 :Adv- h BMP- 2组也可见典型的板层骨和骨髓腔形成 ,Adv- βgal组主要为纤维组织 ,未转染组也可见散在骨小梁形成。结论 Adv- h BMP- 2基因转染可诱导人骨髓间质干细胞成骨。

基因修饰的生物可降解人工骨修复骨缺损的血管化研究

目的评价转染骨形成蛋白2(bonemorphogeneticprotein2,BMP-2)基因的骨髓间充质干细胞(marrowmesenchymalstemcells,MSCs)复合生物可降解人工骨修复兔桡骨缺损的血管化过程,观察BMP-2基因对促进移植骨血管化的影响。方法利用携带BMP-2基因的腺病毒载体(adenoviruscarryingBMP-2gene,Ad-BMP-2)转染MSCs及复合人工骨制备。取新西兰大耳白兔60只制成双侧桡骨中段1.5cm骨缺损模型,随机分为4组,每组15只(30侧)。各组采用不同材料植入缺损,A组Ad-BMP-2转染MSCs+聚乳酸/聚己内酯(polylacticacid/polycaprolactone,PLA/PCL);B组β-半乳糖酐酶基因的重组腺病毒转染MSCs+PLA/PCL;C组未转染MSCs+PLA/PCL;D组单纯PLA/PCL。分别于术后4、8和12周各组处死5只动物,行X线片、微血管分布、组织学、透射电镜观察,并行血管内皮生长因子(vascularendothelialgrowthfactor,VEGF)表达检测及微血管计数。结果A组4周时见移植骨内片状成骨影,有较多新生血管长入,支架孔隙内充满软骨痂,功能活跃的成骨细胞围绕微血管生长,VEGF表达及微血管数均明显高于其它各组,且差异有统计学意义(P<0.01);8周时移植骨内成骨逐渐增多,微血管迂曲扩张并相互连接,软骨痂转变为小梁骨;12周时皮质骨连续,髓腔再通,微血管呈规则地纵向排列。B、C组成骨能力较弱,血管再生缓慢,12周时骨缺损得到初步修复,微血管沿新生骨小梁孔隙分布。D组各时间点新生血管少见,12周时骨端硬化,缺损区被纤维组织填充。结论BMP-2基因转染可通过上调VEGF表达,间接诱导移植骨血管化,促进种子细胞成活,加速新骨形成。

骨形态发生蛋白2基因治疗与缓释载体修复骨缺损的比较研究

[目的]比较骨形态发生蛋白2(BMP-2)基因治疗与生长因子缓释方法修复节段性骨缺损效果。[方法]于兔双侧桡骨中段造成1·5cm骨缺损,采用4种方法修复:A组植入转基因骨髓间质干细胞(MSCs)与PLA/PCL(聚乳酸/聚己内酯)支架的复合物;B组植入单纯MSCs与含重组BMP-2的PLA/PCL缓释载体的复合物;C组植入单纯MSCs与PLA/PCL复合物;D组植入单纯PLA/PCL。术后4、8、12周行X线、组织学、生物力学和骨密度等检测。[结果]A组体内植入4周后,成骨细胞和间质细胞呈BMP-2强阳性表达;其成骨速度及成骨质量均明显优于B组,12周时骨缺损完全修复。C组成骨能力较弱,而D组则无新骨形成,残留骨缺损。[结论]BMP-2基因治疗是修复节段性骨缺损的好方法。

骨形成蛋白-2基因促进犬牙周组织再生的体内研究

目的:观察重组入骨形成蛋白-2(rhBMP-2)质粒对犬牙周骨缺损再生作用的影响。方法:选用6只成年bea犬,将其下颌两侧的第2、3、4前磨牙(P2、P3、P4)作为实验牙。在每颗实验牙的近中根颊侧制作“U”型骨缺损,并随设计为3组,即pIRES-rhBMP-2组、rhBMP-2组(阳性对照组)和PBS组(空白对照组)。术后第4与第8周分别处动物。光镜下观察组织学变化,采用Image-Pro-Express系统测量新生牙槽骨和牙骨质的高度、新生结缔组织的附量。测量结果以SAS 6．12软件包进行Newman-Keuls q检验。结果:实验第8周时,组织学观察可见2个实验组新牙槽骨接近于正常骨结构,新生牙周纤维稠密,富含血管;空白对照组胶原纤维稀疏,排列不规则。新生组织测量果显示:2个实验组新生牙槽骨和牙骨质的高度、新生结缔组织的附着量较空白对照组显著增加(P<0．05,P<0．01) 2个实验组间相比无显著性差异(P>0．05)。结论:pIRES-rhBMP-2有较强的骨诱导活性,能有效促进犬牙周骨缺的组织再生。

BMP-7基因促进大鼠下颌牵张成骨的研究

目的:探讨骨形成蛋白-7(BMP-7)基因修饰的自体骨髓间充质干细胞(MSCs)促进大鼠下颌牵张骨痂形成的可行性。方法:选用48只雄性SD大鼠,随机分为实验和对照2组。建立大鼠下颌DO模型;于牵张结束最后1d,实验组大鼠牵张间隙内注射转染重组质粒pEGFP-BMP7的自体骨髓MSCs;而对照组大鼠注射转染pEGFP-N1空质粒的MSCs。分别于固定期第2、4、8周分3批处死大鼠,进行放射学、组织学观察,并进行骨组织形态计量学分析。结果:实验组牵张间隙内新骨形成和骨痂密度均明显高于对照组;计量学分析也显示各时间点实验组新生骨量(NBV1和NBV2)和新生骨小梁宽度(TNT)均显著高于对照组(P<0.01)。结论:基于MSCs的BMP-7exvivo基因治疗可有效促进DO新骨形成,从而缩短固定期,为临床颅颌面骨缺损的重建提供了一个极具价值的修复策略。

BMP-4基因在成纤维细胞内的表达

目的 :构建mBMP 4真核表达载体并转染成纤维细胞 ,观测外源基因在靶细胞内的表达及对细胞表现型的影响。方法 :利用基因重组技术构建mBMP 4基因真核表达载体 pCR 3 .1uni mBMP 4;利用基因转染技术体外转染mBMP 4基因至成纤维细胞NIH 3T3 ,转染的细胞用G418筛选 ,利用斑点杂交和免疫组化检测转染 4周后外源基因表达的情况。结果 :琼脂糖电泳证明mBMP 4真核表达载体 pCR 3 .1uni mBMP 4构建成功。细胞转染后第 4周 ,斑点杂交和免疫组化均显示为阳性 ,阳性细胞碱性磷酸酶表达升高。结论 :外源BMP 4基因可在成纤维细胞内获得表达并可影响靶细胞的表现型。

hBMP-4瞬时转染对兔骨髓基质干细胞生物学行为的影响

目的应用兔骨髓基质干细胞(bonemarrowstromalcells,MSCs)作为基因治疗的靶细胞,体外转染人骨形成蛋白4(humanbonemorphogeneticprotein-4,hBMP-4)基因,观察瞬时转染对兔MSCs生物学行为的影响。方法贴壁法培养兔MSCs,分别在体外转染pEGFP-hBMP-4和pEGFP基因并留置空白对照。检测转染效率及目的基因的转录和表达,观察细胞形态及生长情况,检测碱性磷酸酶、钙结节及骨钙素等成骨细胞表型。结果基因转染效率达到20%～30%,RT-PCR显示MSCs本身有目的基因的少量转录,转染pEGFP-hBMP-4后转录增强。目的基因转染后细胞形态略有变化,生长曲线与对照组相似,碱性磷酸酶阳性染色面积增加(P=0.0016),钙结节增多(P=0.0001),骨钙素表达增强(P=0.03)。结论优化的条件下取得了较高的转染效率,hBMP-4基因转染可以增强目的基因的转录,加速MSCs向成骨细胞表型转化。hBMP-4转染的MSCs可望成为组织工程化骨理想的种子细胞。

腺病毒介导的BMP-2基因转染兔骨髓基质干细胞及对其增殖、成骨分化的影响

目的:用骨形态发生蛋白-2(BMP-2)腺病毒表达载体(Ad-BMP-2)转染兔骨髓基质干细胞(BMSCs),研究转染对其增殖、成骨分化的影响。方法:用Ad-BMP-2转染兔BMSCs,利用免疫细胞化学法、原位杂交染色和蛋白印迹法检测转染后细胞BMP-2的表达。流式细胞仪观察细胞周期的变化,分析转染对BMSCs增殖的影响。酶标法检测ALP活性;免疫荧光检测骨钙素(OCN)、Ⅰ型胶原表达,分析转染对BMSCs成骨分化的影响。结果:BMP-2基因在转染细胞内mRNA水平和蛋白水平均有较高表达,蛋白印迹法检测到培养液中有BMP-2蛋白阳性表达。流式细胞仪检测G1期、S期细胞比例与空白对照组无差异。ALP活性明显增高,骨钙素、Ⅰ型胶原免疫荧光检测,见胞浆内有大量显绿色荧光的阳性物质。结论:在腺病毒载体介导下BMP-2基因成功导入BMSCs,细胞增殖未因转染而受影响,并可持续表达基因产物,向成骨细胞分化。

人转化生长因子β_1及骨形成蛋白7基因共表达载体的构建及对骨髓基质干细胞的定向诱导作用

目的构建人转化生长因子1β(transform ing grow th factor1β,TGF-1β)及骨形成蛋白7(bonem orphogenetic prote in 7,BM P-7)基因共表达腺病毒真核表达载体,并观察感染骨髓基质干细胞(m arrow strom a l stemce lls,M SC s)后目的基因的表达和对细胞生物学行为的影响。方法以复制缺陷的腺病毒A dE asy为基因载体,制备携带TGF-1β及BM P-7基因的高滴度腺病毒液感染人M SC s,通过免疫细胞化学、原位杂交、RT-PCR及己糖醛酸水平检测等方法鉴定外源基因的表达,分析外源性基因共表达对M SC s定向软骨分化的调控机制。结果腺病毒感染72 h后,TGF-1β和BM P-7免疫细胞化学染色可见大部份M SC s胞浆内均出现棕黄色粗颗粒,通过原位杂交检测出Ⅱ型胶原蛋白基因mRNA,感染10 d后细胞培养液中己糖醛酸含量为68.03±3.34μg/m l与感染前的53.20±3.70μg/m l明显升高有统计学意义(P<0.01)。结论成功构建了人TGF-1β及BM P-7共表达基因腺病毒表达载体,证实其在M SC s中的表达和具有向软骨细胞定向分化的诱导作用,为软骨缺损修复的局部基因治疗奠定实验基础。

人骨形成蛋白4基因修饰的兔骨髓基质细胞异位成骨试验

目的:通过人骨形成蛋白4(bonemorphogeneticprotein,BMP4)基因修饰的兔骨髓基质细胞(bonemarrowStromalcells,bMSCs)与天然型无机骨(naturalnon鄄organicbone,NNB)支架复合,进行自体皮下异位成骨试验,探索BMP4基因治疗与组织工程技术相结合的可行性。方法:贴壁法培养兔bMSCs,体外应用脂质体介导转染pEGFP鄄hBMP4及pEGFP真核表达质粒。将转染基因的细胞和未转染基因的对照组细胞,分别以5×107/ml的浓度,与NNB支架复合,构建组织工程化骨,植入6只新西兰兔自体皮下,每组6例,4周后取材,组织学观察,并进行新骨成骨面积分析。结果:空白对照NNB孔隙内无新骨形成,转染pEGFP基因组及对照细胞组,支架网孔内均有新生骨及软骨样组织形成,而pEGFP鄄hBMP4实验组形成的新生骨及软骨样组织面积更大(P<0.05)。结论:应用hBMP4基因修饰的bMSCs作为骨组织工程的种子细胞,可望取得更强的成骨能力。