组织工程骨-软骨复合支架的构建与优化

背景：制备具有细胞识别信号的细胞外基质替代材料及仿生支架是目前组织工程支架材料研究的重点和热点。 目的：制备并筛选出能够满足构建骨-软骨复合组织要求的多孔三维支架,并评价其生物学性能。 方法：制备胶原-壳聚糖、明胶-硫酸软骨素-透明质酸钠、胶原-陶瓷化骨、明胶-陶瓷化骨支架材料,以新鲜关节为对照组。 结果与结论：胶原-壳聚糖支架孔径50-200 μm,孔隙率(90.5±2.1)%;明胶-硫酸软骨素-透明质酸钠支架孔径100- 150 μm,孔隙率(78.0±1.1)%;胶原-陶瓷化骨支架孔径400-500 μm,孔隙率(67.5±2.1)%;明胶-陶瓷化骨支架孔径300-400 μm,孔隙率(65.9±1.2)%。明胶-硫酸软骨素-透明质酸钠与明胶-陶瓷化骨支架基本符合实验要求,其结构与生物化学成分近似于自然细胞外基质,能够模拟细胞外微环境。说明明胶-硫酸软骨素-透明质酸钠与明胶-陶瓷化骨支架可作为复合组织的支架。     

聚磷酸钙纤维/羟基磷灰石/明胶软骨组织工程支架材料的制备及性能

背景：目前明胶基组织工程支架材料存在力学性能低、生物相容性差、降解速率难以控制等缺陷。 目的：通过添加聚磷酸钙纤维和羟基磷灰石改善明胶支架材料的性能。 方法：以自制聚磷酸钙纤维和羟基磷灰石为添加材料,明胶为基体材料,以戊二醛为交联剂,采用溶媒浇铸/粒子滤取技术制备配比为50/10/40的聚磷酸钙纤维/羟基磷灰石/明胶软骨组织工程支架复合材料。测试支架材料的物理力学性能,并观察其微观结构。 结果与结论：采用溶胶凝胶法制得的羟基磷灰石粉末结晶程度较差,经900 ℃下煅烧0.5 h后,可制得结晶程度较高的羟基磷灰石粉末。聚磷酸钙纤维/羟基磷灰石/明胶软骨组织工程支架材料具有三维、连通、微孔网状空间结构,孔隙率在65%-90%之间,满足软骨组织工程对其支架材料孔隙的要求。戊二醛的交联作用和聚磷酸钙纤维的增强作用,克服了明胶在制备多孔支架时容易收缩的缺点,制得高孔隙率三维连通的支架材料。     

皮肤组织工程-细胞支架的构筑及其生物相容性评价

皮肤组织工程的发展提供了一种无损伤修复创伤和功能重建的皮肤治疗模式.作为组织工程的三要素之一,细胞支架发挥着重要的作用.为满足组织工程中对细胞支架在力学性能、物理结构及生物相容性等方面的要求,我们首先制备了聚乳酸(PDLLA)、聚乳酸-己内酯(PLACL)多孔支架,并以生物相容性较好的猪的无细胞真皮(acellular dermis matrix,ADM)为参比,分别把三种材料植入大鼠背部肌层,术后定期取大鼠皮下埋藏组织进行组织学检测.结果发现PDLLA与PLACL多孔支架的降解周期、力学性能、孔隙率及其孔径都可以根据皮肤组织工程中的要求进行调控.组织学检查,移植物内无明显炎性细胞,21天后,均完全血管化且分布较均匀.说明PDLLA与PLACL的生物相容性较ADM差,但并未出现明显的异物排斥反应,两者的生物相容性基本上可以满足组织工程中对支架的要求,这为聚乳酸类人工皮肤的进一步研究提供了有意义的实验依据.     

碳纤维-聚乳酸-聚乙二醇复合支架的制备及性能检测

背景：长期实验发现聚乳酸-聚乙二醇支架的力学性能及细胞相容性能较差,因此多数研究向支架中加入其他材料,以提高其生物活性及力学性能。 目的：制备改性碳纤维-聚乳酸-聚乙二醇支架,并检测其性能。 方法：采用溶液潘注/粒子沥滤法制备改性碳纤维-聚乳酸-聚乙二醇复合支架。对比改性碳纤维-聚乳酸-聚乙二醇复合支架与聚乳酸-聚乙二醇支架的超微结构、孔隙率、吸水性、降解率及力学性能。将改性碳纤维-聚乳酸-聚乙二醇复合支架与聚乳酸-聚乙二醇支架分别与SD大鼠成骨细胞共培养,12 h后采用沉淀法检测细胞黏附率;培养1,3,5,7,9 d后,采用 MTT 法检测细胞增殖。 结果与结论：聚乳酸-聚乙二醇支架材料表面孔结构分布均匀,孔径为(404.0±10.5) µm;改性碳纤维-聚乳酸-聚乙二醇支架碳纤维表面见大量纵向沟槽,表面孔结构分布均匀,孔径为(433.0±3.0) µm,两组支架孔径比较差异有显著性意义(P < 0.05)。改性碳纤维-聚乳酸-聚乙二醇支架的孔隙率、吸水性、弹性模量和抗压强度、降解率、细胞黏附率与增殖率均高于聚乳酸-聚乙二醇支架(P < 0.05)。表明改性碳纤维的加入改善了聚乳酸-聚乙二醇复合支架的力学性能及细胞相容性。中国组织工程研究杂志出版内容重点：生物材料;骨生物材料; 口腔生物材料; 纳米材料; 缓释材料; 材料相容性;组织工程     

壳聚糖/磷酸三钙复合组织工程支架材料的制备及其性能*

背景：通过适当的工艺混合、加工来制备复合支架材料,可以弥补单一材料的不足,最大限度地满足组织工程的需要。 目的：制备壳聚糖/磷酸三钙复合支架,探讨其作为牙髓组织工程支架材料的可行性。 方法：壳聚糖粉末溶于微量冰醋酸溶液中,搅拌均匀,静置脱泡,预冷冻,交联,再次冷冻制成海绵状多孔壳聚糖/磷酸三钙支架。 结果与结论：冻干法制备的壳聚糖/磷酸三钙多孔支架平均孔隙率达85.78%,最高孔隙率达90%以上,孔径在100~300 μm,复合后的支架材料具有良好的韧性,当轴向压缩变形量超过5 mm时,材料仍然没有发生破坏。材料浸提液与牙髓细胞复合培养后,细胞毒性均为0级,由此可见壳聚糖/磷酸三钙复合材料具有良好的生物相容性、细胞亲和性和一定的力学性能,满足生物材料基本要求。     

一种可注射体内成孔的磷酸钙骨水泥

背景：磷酸钙骨水泥存在脆性大、抗水溶性(血溶性)差、力学性能不足、降解缓慢等缺点,其临床应用受到一定限制,故需要对其进行改性研究。 目的：制备一种具有一定强度、孔隙率、适合骨生长的多孔磷酸钙骨水泥生物支架材料。 方法：以磷酸钙骨水泥为基本体系,液相采用壳聚糖的弱酸溶液,以提高磷酸钙骨水泥的可塑性和黏弹性,使骨水泥具有可注射性,显著提升骨水泥的应用范围及应用舒适度。固相为双相磷酸钙(磷酸四钙+磷酸氢钙)粉体,并在固相中添加一定量的甘露醇及聚乳酸-乙醇酸共聚物作为造孔剂,制备磷酸钙支架材料。 结果与结论：此材料孔径可达到10~300 μm。添加60%致孔剂时,磷酸钙骨水泥固化体孔隙率可达到(68.3±1.5)%。磷酸钙骨水泥孔隙率的增加使材料的力学性能下降,其抗压强度从最初不含致孔剂时的(53.0±1.4) MPa下降到含60%致孔剂的(2.5±0.2) MPa。实验制备的此种多孔磷酸钙骨水泥材料,是具有一定抗压强度、较好的孔隙率,并能体内降解的可注射生物支架材料。     

三维打印双相磁性纳米复合支架材料的性能测定

目的研究制备出一种新型双相磁性纳米复合支架材料(PLGA/Col-I-PLGA/n-HA/Fe_2O_3),通过各项生物学性能检测,评价并探讨其作为骨组织工程支架的可行性。方法通过低温快速成型方法制备双相磁性纳米复合支架材料(PLGA/Col-I-PLGA/n-HA/Fe_2O_3),采用电子试验机检测支架材料的抗弯,抗压,弹性模量评价其力学性能,通过电镜观察支架材料超微结构;以介质(乙醇)浸泡法测定支架材料的孔隙率,将支架材料与骨髓间充质干细胞复合共培养,检测其生物相容性。结果双相磁性纳米复合支架材料力学检测结果显示其具有良好的力学性能,电镜观察结果显示上下两层孔径均匀分布,上层软骨相孔径较小,中间连续相良好融合,孔径及孔隙率检测结果显示软骨层支架的孔径为189um,孔隙率86.5%。骨层支架的孔径为364um,孔隙率77.1%,符合双层支架材料的设计要求。双相磁性纳米复合支架材料与骨髓间充质干细胞共培养,结果显示骨髓间充质干细胞的增殖效果很好,能更好的促进分化为目的细胞,说明双相磁性纳米复合支架材料具有良好的生物相容性。结论双相磁性纳米复合支架材料(PLGA/Col-I-PLGA/n-HA/Fe_2O_3)有很好的力学性能和生物相容性,孔径及孔隙率达到细胞粘附生长的要求,与正常的关节软骨及软骨下骨生理结构更加接近,有望可以更好的修复骨关节炎或者外伤等疾病带来的软骨和软骨下骨损伤。     

聚乳酸/壳聚糖纳米纤维/纳米羟基磷灰石支架与兔软骨细胞的相容性

背景：传统的支架材料存在疏水性强,材料表面缺乏细胞表面受体特异结合的生物活性分子,材料的酸性降解产物易引发无菌性炎性反应等不足。根据仿生原理及软骨真实结构和构成来选择和制备组织工程软骨支架能够获得理想效果。 目的：制备聚乳酸/壳聚糖纳米纤维/纳米羟基磷灰石支架,评价其与兔膝关节软骨细胞的生物相容性,探讨其应用于关节软骨组织工程的可行性。 方法：采用二次相分离技术制备聚乳酸/壳聚糖纳米纤维/纳米羟基磷灰石复合支架,将第3代新西兰兔软骨细胞接种至复合支架材料上复合培养,倒置相差显微镜下观察细胞生长情况。细胞-支架复合物在24孔板中培养5 d以后,将其植入裸鼠皮下8周。 结果与结论：聚乳酸/壳聚糖纳米纤维/纳米羟基磷灰石支架材料经化学合成后,具有合适的三维多孔结构,孔隙率为90%,孔径300~450 μm;植入裸鼠皮下8周后Ⅱ型胶原免疫组织化学染色和甲苯胺蓝染色显示细胞-支架复合物中的软骨细胞可以像天然软骨一样分泌黏多糖和Ⅱ型胶原。提示生物材料聚乳酸/壳聚糖纳米纤维/纳米羟基磷灰石对于兔软骨细胞有良好的生物相容性,可作为生物组织工程支架。     

低温快速成型亲水改性复合人工骨支架的性能测定

背景：低温快速成型技术具有支架成型可控性、保持材料生物学活性和易于实现支架材料的三维多孔立体结构等优势,被迅速用于骨组织工程支架的制备。 目的：采用低温快速成型制备聚乙二醇改性聚乳酸-乙醇酸/纳米羟基磷灰石复合支架,并检测其性能。 方法：采用低温快速成型设备分别制备聚乙二醇改性聚乳酸-乙醇酸/纳米羟基磷灰石与聚乳酸-乙醇酸/纳米羟基磷灰石复合支架,通过电镜观察支架超微结构,以介质(乙醇)浸泡法测定支架孔隙率,采用电子试验机检测支架力学性能;将两种支架材料分别与大鼠成骨细胞共培养,培养12 h采用沉淀法检测细胞黏附率,培养1,3,5,7,9,12 d采用CCK-8法检测细胞增殖。 结果与结论：两组支架孔径均在理想范围内并具有较高孔隙率,但聚乙二醇改性聚乳酸-乙醇酸/纳米羟基磷灰石支架的孔径波动范围大,孔径均值较聚乳酸-乙醇酸/纳米羟基磷灰石支架小且部分有闭塞现象。聚乙二醇改性聚乳酸-乙醇酸/纳米羟基磷灰石支架的细胞黏附率及表面细胞增殖活性高于聚乳酸-乙醇酸/纳米羟基磷灰石支架(P < 0.05),力学性能低于聚乳酸-乙醇酸/纳米羟基磷灰石支架(P < 0.05)。表明聚乙二醇改性聚乳酸-乙醇酸/纳米羟基磷灰石复合支架具有良好的细胞相容性。中国组织工程研究杂志出版内容重点：生物材料;骨生物材料; 口腔生物材料; 纳米材料; 缓释材料; 材料相容性;组织工程全文链接：     

兔肋软骨脱细胞基质的制备

背景：研究表明新西兰兔软骨组织可作为组织工程支架材料,其中关节软骨及耳软骨的脱细胞基质的研究较多,但采用肋软骨作为组织工程软骨支架的研究较少。 目的：制备新西兰兔肋软骨脱细胞基质,探讨天然软骨支架作为组织工程支架的可行性。 方法：用联合去垢剂-酶法获得软骨支架,根据脱细胞过程中Triton X-100第2次处理时间0,24,48,96 h分为4组。脱细胞完毕后各组支架固定行扫描电镜采集图像观察计算支架孔隙率、孔径长度,并对支架进行苏木精-伊红染色、甲苯胺蓝及Ⅱ型胶原免疫组织化学染色,并将脱细胞支架植入异体新西兰兔皮下观察其相容性。 结果与结论：兔肋软骨脱细胞基质呈乳白色,大小均一,染色示支架结构完整,仍保存大量酸性黏多糖及Ⅱ型胶原成分,扫描电镜观察经一定时间的脱细胞处理后可得到结构完整,孔隙均匀的天然软骨支架,其孔隙率为(61.31±8.45) %;孔径长度为(32.80±5.15) μm,符合正态性分布,各组脱细胞支架植入异体新西兰兔皮下7 d后生物相容性良好,周围软组织无明显充血、化脓等炎症排斥反应出现。结果显示,兔肋软骨脱细胞支架具有良好的基质组成,有较完整、均匀的孔隙结构及孔径分布,可作为组织工程支架材料。     

Fabrication and characterization of gelatin-based biocompatible porous composite scaffold for bone tissue engineering

In this study, composite scaffolds were prepared with polyethylene oxide (PEO)-linked gelatin and tricalcium phosphate (TCP). Chitosan, a positively charged polysaccharide, was introduced into the scaffolds to improve the properties of the artificial bone matrix. The chemical and thermal properties of composite scaffolds were investigated by Fourier transform infrared spectroscopy, thermogravimetric analyzer, differential thermal analyzer. In vitro cytotoxicity of the composite scaffold was also evaluated and the sample showed no cytotoxic effect. The morphology was studied by SEM and light microscopy. It was observed that the prepared scaffold had an open interconnected porous structure with pore size of 230-354 μm, which is suitable for osteoblast cell proliferation. The mechanical properties were assessed and it was found that the composite had compressive modulus of 1200 MPa with a strength of 5.2 MPa and bending modulus of 250 MPa having strength of 12.3 MPa. The porosity and apparent density were calculated and it was found that the incorporation of TCP can reduce the porosity and water absorption. It was revealed from the study that the composite had a 3D porous microstructure and TCP particles were dispersed evenly among the crosslinked gelatin/chitosan scaffold. ? 2012 Wiley Periodicals, Inc. J Biomed Mater Res Part A: 100A:3020-3028, 2012.     

基于丝素/胶原/羟基磷灰石仿生骨材料的多维结构及其性能

目的 体外构建丝素蛋白（silk fibroin,SF）、I型胶原(type I collagen,Col-I)和羟基磷灰石(hydroxyapatite, HA)共混体系制备二维复合膜和三维仿生支架,研究其理化性质和生物相容性,探讨其在组织工程支架材料中应用的可行性。方法 通过在细胞培养小室底部共混SF/Col-I/HA以及低温3D打印结合真空冷冻干燥法制备二维复合膜及三维支架。通过机械性能测试、电子显微镜和Micro-CT检测材料的理化性质,检测细胞的增殖评估其生物相容性。结果 通过共混和低温3D打印获得稳定的二维复合膜及三维多孔结构支架;力学性能具有较好的一致性,孔径、吸水率、孔隙率和弹性模量均符合构建组织工程骨的要求;支架为网格状的白色立方体,内部孔隙连通性较好; HA均匀分布在复合膜中,细胞黏附在复合膜上,呈扁平状;细胞分布在支架孔壁周围,呈梭形状,生长及增殖良好。结论 利用SF/Col-I/HA共混体系成功制备复合膜及三维支架,具有较好的孔连通性与孔结构,有利于细胞和组织的生长以及营养输送,其理化性能以及生物相容性符合骨组织工程生物材料的要求。     

Preparation and characterization of gelatin-bioactive glass ceramic scaffolds for bone tissue engineering

Macroporous composite scaffolds comprising of gelatin and glass ceramic has been fabricated and characterized for bone tissue engineering applications. Gelatin scaffold with varying glass-ceramic content was fabricated using lyophilization technique. The microstructure, compressive strength, bioactivity, biodegradation and biocompatibility of the fabricated scaffolds were evaluated. The scaffolds presented macroporous pore size with porosity varying from 79 to 84%. The compressive strength was enhanced by glass ceramic addition and the scaffolds exhibited strength in the range of 1.9 to 5.7?MPa. The obtained strength and porosity was in the range of cancellous bone. The dissolution of gelatin scaffolds was optimized by an additional in situ glutaraldehyde crosslinking step and further by glass-ceramic addition. The composite scaffolds showed good apatite-forming ability in vitro. Biocompatibility and osteogenic ability of the scaffolds were analyzed in vitro by cell adhesion study, alkaline phosphatase activity and Alizarin S staining. The obtained results revealed the composite scaffolds possessed enhanced osteogenic ability and good cell adhesion properties. The developed scaffold is a prospective candidate as a biomaterial for bone tissue engineering.     

Development of gelatin-chitosan-hydroxyapatite based bioactive bone scaffold with controlled pore size and mechanical strength

Hydroxyapatite–chitosan/gelatin (HA:Chi:Gel) nanocomposite scaffold has potential to serve as a template matrix to regenerate extra cellular matrix of human bone. Scaffolds with varying composition of hydroxyapatite, chitosan, and gelatin were prepared using lyophilization technique where glutaraldehyde (GTA) acted as a cross-linking agent for biopolymers. First, phase pure hydroxyapatite–chitosan nanocrystals were in situ synthesized by coprecipitation method using a solution of 2% acetic acid dissolved chitosan and aqueous solution of calcium nitrate tetrahydrate [Ca(NO₃)₂,4H₂O] and diammonium hydrogen phosphate [(NH₄)₂H PO₄]. Keeping solid loading constant at 30 wt% and changing the composition of the original slurry of gelatin, HA–chitosan allowed control of the pore size, its distribution, and mechanical properties of the scaffolds. Microstructural investigation by scanning electron microscopy revealed the formation of a well interconnected porous scaffold with a pore size in the range of 35–150 μm. The HA granules were uniformly dispersed in the gelatin–chitosan network. An optimal composition in terms of pore size and mechanical properties was obtained from the scaffold with an HA:Chi:Gel ratio of 21:49:30. The composite scaffold having 70% porosity with pore size distribution of 35–150 μm exhibited a compressive strength of 3.3–3.5 MPa, which is within the range of that exhibited by cancellous bone. The bioactivity of the scaffold was evaluated after conducting mesenchymal stem cell (MSC) – materials interaction and MTT (3-[4,5-dimethylthiazol-2-yl]-2,5-diphenyltetrazolium bromide) assay using MSCs. The scaffold found to be conducive to MSC’s adhesion as evident from lamellipodia, filopodia extensions from cell cytoskeleton, proliferation, and differentiation up to 14 days of cell culture.     

Preparation,characterization and bioactivities of nano anhydrous calcium phosphate added gelatin–chitosan scaffolds for bone tissue engineering

Abstract

Gelatin, chitosan and nano calcium phosphate based composite scaffold with tailored architectures and properties has great potential for bone regeneration. Herein, we aimed to improve the physico chemical, mechanical and osteogenic properties of 3D porous scaffold by incorporation of dihydrogen calcium phosphate anhydrous (DCPA) nanoparticles into biopolymer matrix with variation in composition in the prepared scaffolds. Scaffolds were prepared from the slurry containing gelatin, chitosan and synthesized nano DCPA particle using lyophilization technique. DCPA nano particles were synthesized using calcium carbonate and phosphoric acid in water–ethanol medium. XRD pattern showed phase pure DCPA in synthesized nanopowder. Scaffolds were prepared by addition of DCPA nanoparticles to the extent of 5–10?wt% of total polymer into gelatin–chitosan solution with solid loading varying between 2.5 and 2.75?wt%. The prepared scaffold showed interconnected porosity with pore size varying between 110 and 200 micrometer. With addition of DCPA nanoparticles, average pore size of the prepared scaffolds decreased. With increase in nano ceramic phase content from 5?wt% to 10?wt% of total polymer, the compressive strength of the scaffold increased. Scaffold containing 10?wt% DCPA showed the highest average compressive strength of 2.2?MPa. Higher cellular activities were observed in DCPA containing scaffolds as compared to pure gelatin chitosan scaffold suggesting the fact that nano DCPA addition into the scaffold promoted better osteoblast adhesion and proliferation as evident from MTT assay and scanning electron microscopic (SEM) investigation of osteoblast cultured scaffolds. A higher degree of lamellopodia and filopodia extensions and better spreading behavior of osteoblasts were observed in FESEM micrographs of MG 63 cultured DCPA containing scaffold. The results demonstrated that both mechanical strength and osteogenic properties of gelatin–chitosan scaffold could be improved by addition of anhydrous dihydrogen calcium phosphate nanoparticles into it.     

聚乳酸-羟基乙酸共聚物/硅酸钙三维多孔骨组织工程支架的构建与性能

BACKGROUND: Some disadvantages exsist in commonly used poly(lactic-co-glycolic acid) (PLGA) scaffolds, including acidic degradation products, suboptimal mechanical properties, low pore size, poor porosity and pore connectivity rate and uncontrollable shape. OBJECTIVE: To construct a scaffold with three-dimensional (3D) pores by adding calcium silicate to improve the properties of PLGA, and then detect its degradability, mechanical properties and biocompatibility. METHODS: PLGA/calcium silicate porous composite microspheres were prepared by the emulsion-solvent evaporation method, and PLGA 3D porous scaffold was established by 3D-Bioplotter, and then PLGA/calcium silicate composite porous scaffolds were constructed by combining the microspheres with the scaffold using low temperature fusion technology. The compositions, morphology and degradability of the PLGA/calcium silicate porous composite microspheres and PLGA microspheres, as well as the morphology, pore properties and compression strength of the PLGA 3D scaffolds and PLGA/calcium silicate composite porous scaffolds were measured, respectively. Mouse bone marrow mesenchymal stem cells were respectively cultivated in the extracts of PLGA/calcium silicate porous composite microspheres and PLGA microspheres, and then were respectively seeded onto the PLGA 3D scaffolds and PLGA/calcium silicate composite porous scaffolds. Thereafter, the cell proliferation activity was detected at 1, 3 and 5 days. RESULTS AND CONCLUSION: Regular pores on the PLGA microspheres and internal cavities were formed, and the PH values of the degradation products were improved after adding calcium silicate. The fiber diameter, pore, porosity and average pore size of the composite porous scaffolds were all smaller than those of the PLGA scaffolds. The compression strength and elasticity modulus of the composite porous scaffolds were both higher than those of the PLGA scaffolds (P < 0.05). Bone marrow mesenchymal stem cells grew well in above microsphere extracts and scaffolds. These results indicate that PLGA/calcium silicate composite porous scaffolds exhibit good degradability in vitro, mechanical properties and biocompatibility.     

生物活性玻璃与壳聚糖复合的骨修复材料

背景：生物活性玻璃是一种多相复合材料,具有良好的生物活性、骨传导性及生物相容性,但作为骨修复材料仍然存在不能完全降解、机械强度较低等不足。 目的：设计生物活性玻璃/壳聚糖复合材料骨组织工程支架,并检测其理化性能。 方法：将2.0%壳聚糖盐酸溶液与β-甘油磷酸钠以7∶1的体积比混合制备壳聚糖溶液。称取0.5,1.0,1.5 g生物活性玻璃分别加入上述壳聚糖溶液中,使得壳聚糖与生物活性玻璃的质量比为2∶1,1∶1及1∶1.5。将复合材料浸泡于模拟生理体液中7 d进行体外矿化。 结果与结论：扫描电镜见复合支架具有相互贯通的多孔结构,孔隙率最高可达89%,孔径大小合适,为100-  300 µm,生物活性玻璃以针状形式分散在壳聚糖支架之间,均匀排列,被壳聚糖支架充分包裹结合紧密。随生物活性玻璃含量的增加,复合材料的孔隙率逐渐下降,断裂强度逐渐升高,他们之间呈正相关性。X射线衍射图及傅里叶变换红外光谱证实复合支架中的单一材料未发生性质改变,示差扫描量热法分析显示正常体温情况下材料无质量丢失。矿化3 d后材料表面形成的羟基磷灰石逐渐长大为绒毛状,数量也明显增多;矿化7 d后绒毛状的羟基磷灰石长成为针状,数量进一步增多,且众多的矿化物结成球状。中国组织工程研究杂志出版内容重点：生物材料;骨生物材料; 口腔生物材料; 纳米材料; 缓释材料; 材料相容性;组织工程全文链接：