羟基磷灰石/明胶支架复合骨髓间充质干细胞和脐静脉内皮细胞修复兔颅骨缺损

背景:羟基磷灰石/明胶复合材料具有良好的生物相容性及骨诱导性,可作为组织工程支架用于修复骨缺损。目的:观察3D打印羟基磷灰石/明胶支架复合骨髓间充质干细胞和脐静脉内皮细胞修复兔颅骨缺损的效果。方法:取9只雄性新西兰白兔,建立直径约0.8 cm的颅骨缺损模型,分3组处理:空白组不做处理,对照组植入3D打印羟基磷灰石/明胶支架,实验组植入3D打印羟基磷灰石/明胶支架与骨髓间充质干细胞和脐静脉内皮细胞复合物,每组3只。术后第8周,对各组白兔进行颅骨锥形束CT扫描与颅骨缺损部位组织学观察。动物实验获得济宁医学院伦理委员会批准。结果与结论:①锥形束CT扫描:空白组可见明显的骨缺损,缺损区域与周围正常骨组织边缘有点状不透射影;对照组可见有部分新生骨形成,呈不连续状,与周围骨组织亦不连贯;实验组可见新生骨组织呈线性连续,厚度较薄,缺损区域与邻近骨组织边缘融合;②组织学观察:苏木精-伊红染色与Masson三色显示,空白组缺损区见纤维结缔组织生成及少量游离骨细胞;对照组可见少量成骨,材料边缘可见有骨基质沉积,取代材料形成骨小梁;实验组材料空间逐渐被新生骨代替,新生骨和骨小梁结构样组织充填于缺损区域;③结果表明,3D仿生打印羟基磷灰石/明胶支架复合骨髓间充质干细胞和脐静脉内皮细胞可有效促进骨组织的生长,加快骨缺损修复。

3D打印羟基磷灰石-明胶支架联合BMSCs和HUVECs修复兔颅骨缺损的组织学评价

目的通过组织病理学方法评价3D打印技术制备的羟基磷灰石-明胶(HAP-GEL)支架联合骨髓间充质干细胞(BMSCs)和脐静脉内皮细胞(HUVECs)修复兔颅骨缺损的效果。方法将3D打印HAP-GEL支架与BMSCs和HUVECs细胞联合培养,构建组织工程骨。24只新西兰大白兔随机分为空白对照组、阳性对照组、HAP-GEL材料组及BMSCs+HUVECs+HAP-GEL支架共培养组,每组6只,于缺损区随机植入3D打印HAP-GEL支架、HAP-GEL支架+BMSCs和HUVECs细胞,自体颅骨设为阳性对照组,空白缺损设为空白对照组。分别于模型复制后4周和12周通过组织学观察骨愈合情况。结果镜下各组均未见急慢性炎症细胞浸润。术后4周,HE染色显示空白对照组仅有少量纤维结缔组织生成;HAP-GEL材料组有少量新骨生成;BMSCs+HUVECs+HAP-GEL支架共培养组可见部分新骨开始彼此融合,新生骨量与阳性对照组相似;术后12周,HE染色显示空白对照组新生骨量少;HAP-GEL材料组新生骨呈较大面积的板层状;BMSCs+HUVECs+HAP-GEL支架共培养组缺损区几乎全部被新生骨充填,新生骨量较前两组明显增多,且与阳性对照组相似。术后4周,Masson染色显示空白对照组仅有少量纤维组织;HAP-GEL材料组内有蓝染新骨、少量红染成熟骨形成,但着色均较浅;BMSCs+HUVECs+HAP-GEL支架共培养组红染成熟骨面积较HAP-GEL材料组大,修复效果与阳性对照组相似。术后12周,Masson染色显示空白对照组出现蓝染新骨;HAP-GEL材料组成熟骨面积进一步扩大,支架被分割包裹、吸收;BMSCs+HUVECs+HAP-GEL支架共培养组可见大片红染成熟骨生成,夹杂少量蓝染新生骨,支架残存少量,成骨效果与阳性对照组相似,优于HAP-GEL材料组与空白对照组。结论3D打印HAP-GEL支架联合BMSCs和HUVECs对兔颅骨缺损有较好的修复效果。

关于牙科学中的一类最优化问题的解

针对求解过程中遇到的非线性方程组以及强烈依赖于初始值的局部解,提出用线性方程组来代替非线性方程组,然后通过矩阵代数运算找到最优化问题的拟整体解.理论和数值实验结果令人满意.

Dopaminergic effects on in vitro osteogenesis

Multiple growth factors（e.g., BMP2, TGF-b1, FGF2） and isolated genes have been shown to improve osteoblastic proliferation and mineralization, advancing bone tissue engineering. Among these factors, both polydopamine（PDA） and dopamine（DA） monomer have recently been reported to increase osteoblast proliferation and mineralization in vitro. Although a well-characterized neurotransmitter, DA＇s role in the bone is unknown. We hypothesize that DA can directly act on osteoblasts, and examined whether osteoblasts express DA receptors that respond to exogenous DA. m RNAs and protein cell lysates were obtained from MC3T3-E1 cells during osteogenic differentiation phase. Reverse transcription polymerase chain reaction and western blot analysis were used to examine the expression of DA receptors, D1–D5. Dose-response effect and time course of DA treatment on cell proliferation, mineralization, and osteogenic differentiation were investigated at pre-determined days. Real-time PCR was performed to investigate whether DA affects osteogenic gene expression（ALP, BSP, OC, OSX, RUNX2, and Collagen1a2） with or without receptor antagonists（SCH233390 and GR103691）. Two-way ANOVA was used for statistical analysis. All five DA receptors（D1, D2, D3, D4, and D5） m RNAs and proteins were expressed in MC3T3-E1 cells. DA treatment increased cell proliferation for up to 7 days（P, 0.05）. Osteogenic mineralization was significantly greater in the DA-treated group than control group（P, 0.05）. Finally, expression of all the osteogenic genes was inhibited by DA receptor antagonists for D1, D3, and D5. Our findings suggest that MC3T3-E1 osteoblasts express functional DA receptors that enhance proliferation and mineralization. PDA is not biologically inert and has important implications in orthopedic applications. Furthermore, osteoblast differentiation might be regulated by the nervous system, presumably during bone development, remodeling, or repair.

羟基磷灰石-凝胶支架复合成骨细胞修复兔颅骨缺损的影像学评价

目的:探索羟基磷灰石/凝胶支架(HAP-GEL)复合成骨细胞在兔颅骨缺损中的修复效果。方法:将HAP-GEL复合物与成骨细胞联合培养,制备兔颅顶骨骨缺损模型,根据植入材料分为3组,分别为HAP-GEL复合成骨细胞、HAP-GEL支架与空白对照。于术后12周通过大体标本观察、X线与CT分析骨缺损修复情况。结果:术后12周影像学评估,空白对照组骨缺损均为明显透射影;HAP-GEL支架复合成骨细胞与HAP-GEL支架组均为低密度影,缺损的边缘略显模糊。结论:HAP-GEL复合成骨细胞修复兔颅骨缺损,可取得较好的修复效果。

甲状旁腺激素对大鼠牵张成骨过程中ONC、OPN、C-FOS、COL1、VEGF、RUNX2、ALP基因表达的影响

目的探讨甲状旁腺激素(PTH)对大鼠牵张成骨(DO)过程中ONC、OPN、C-FOS、COL1、VEGF、RUNX2、ALP基因表达的影响。方法 30只雄性大鼠制备大鼠下颌骨DO模型。随机分5组,每组6只。第1组(只有牵张无PTH),术后8周取材,应用HE染色及微CT检测,以确定成骨情况。第2组(有牵张无PTH),第3组(有牵张有PTH),第4组(无牵张有PTH),第5组(对照组:无牵张无PTH)。2、3、4组及对照组术后1周取材,RT-PCR测定ONC、OPN、C-FOS、COL1、VEGF、RUNX2、ALP基因的表达。结果第1组,新骨形成,骨质充满牵张区,骨质连续,大鼠建模成功。RT-PCR检测结果显示,2、3、4组与对照组比较,OPN、COL1、RUNX2、ALP基因表达有明显提高(P<0.05),其中第3组最为明显。ONC、C-FOS、VEGF基因2、3、4组与对照组比较差异无统计学意义(P>0.05)。结论 PTH在DO过程中,间歇性给以PTH的作用只有在牵张期发挥作用,其对OPN、COL1、RUNX2、ALP基因表达能够获得理想的协同作用。