Zeng Bai Jin, Yu Ri Yue, Zhou Yong Sheng, Xu Jun, Ni Yong Wei, Liu Yun Song, Xu Yong Wei
Department of Prosthodontics, Peking University School and Hospital of Stomatology, Beijing 100081, China.
Beijing Da Xue Xue Bao Yi Xue Ban. 2009 Oct 18;41(5):565-70.
To investigate the proliferation and the secretion of vascular endothelial growth factor(VEGF), fibroblast growth factor-2(FGF-2) and insulin-like growth factor-1(IGF-1) of human adipose tissue-derived stromal cells(hADSCs) before and after osteogenic differentiation under the stimuli of recombinant human tumor necrosis factor alpha (rhTNF-alpha).
hADSCs were obtained from human lipoaspirates. All the cells used were at passage four. The proliferation of hADSCs was measured with MTT assays 48, 72, 96 hours after being treated with 0, 1, 5, 10, 50 or 100 microg/L rhTNF-alpha respectively. The secretion of VEGF, FGF-2 and IGF-1 of the undifferentiated hADSCs under stimuli of rhTNF-alpha with the above 5 concentration grades was observed and the secretion of these 3 growth factors of hADSCs at different stages of osteogenic differentiation under stimuli of 10 microg/L rhTNF-alpha was also observed. All the supernatants were harvested for measuring after 24 hours' incubation with rhTNF-alpha. The secretion of VEGF, FGF-2 and IGF-1 was measured with ELISA, and the values were normalized to the cell number of the corresponding wells.
The effect of rhTNF-alpha on the proliferation of hADSCs varied with the concentration and time. Compared with the control(0 microg/L), 10 microg/L rhTNF-alpha showed no suppression or acceleration on proliferation of hADSCs at hour 48, but significantly promoted the proliferation at hour 96 (0.903+/-0.042 vs 0.810+/-0.011, P<0.01), 100 microg/L rhTNF-alpha seemed to suppress the proliferation at hour 48 (0.317+/-0.024 vs 0.458+/-0.046, P<0.01), but appeared to promote it (0.956+/-0.030 vs 0.810+/-0.011, P<0.01) at hour 96. rhTNF-alpha(1, 5, 10, 50 and 100 microg/L) significantly increased VEGF, FGF-2 and IGF-1 production of hADSCs versus the control (0 microg/L) (P<0.01). After osteogenic differention, the secretion of the three growth factors of hADSCs (without rhTNF-alpha treated) was elevated with the days increasing. Under the stimulus of 10 microg/L rhTNF-alpha, the hADSCs after 1 day of osteogenic differentiation significantly increased the secretion of VEGF (P<0.01) compared with the group without rhTNF-alpha treated; after 3 and 7 days of osteogenic differentiation, the hADSCs significantly increased the secretion of VEGF (P<0.01), FGF-2 (P<0.05)and IGF-1 (P<0.05). However, after 14 days of osteogenic differentiation, 10 microg/L rhTNF-alpha appeared to suppress the production of VEGF (P<0.01), FGF-2 (P<0.05) and IGF-1 (P<0.05) of the differentiated hADSCs.
Within certain concentration range, rhTNF-alpha can promote the proliferation of hADSCs and the production of VEGF, FGF-2 and IGF-1. The effect of 10 microg/L rhTNF-alpha on the production of VEGF, FGF-2 and IGF-1 of the differentiated hADSCs varied at different stages of osteogenic differentiation.
研究重组人肿瘤坏死因子α(rhTNF-α)刺激下人脂肪组织来源的基质细胞(hADSCs)成骨分化前后的增殖情况以及血管内皮生长因子(VEGF)、成纤维细胞生长因子-2(FGF-2)和胰岛素样生长因子-1(IGF-1)的分泌情况。
从人抽脂物中获取hADSCs。所有使用的细胞均为第4代。分别用0、1、5、10、50或100μg/L rhTNF-α处理hADSCs后,在48、72、96小时用MTT法检测hADSCs的增殖情况。观察上述5个浓度梯度的rhTNF-α刺激下未分化hADSCs的VEGF、FGF-2和IGF-1分泌情况,同时观察10μg/L rhTNF-α刺激下hADSCs成骨分化不同阶段这3种生长因子的分泌情况。与rhTNF-α孵育24小时后收集所有上清液进行检测。用ELISA法检测VEGF、FGF-2和IGF-1的分泌情况,并将数值标准化为相应孔中的细胞数量。
rhTNF-α对hADSCs增殖的影响随浓度和时间而变化。与对照组(0μg/L)相比,10μg/L rhTNF-α在48小时时对hADSCs的增殖无抑制或促进作用,但在96小时时显著促进增殖(0.903±0.042对0.810±0.011,P<0.01);100μg/L rhTNF-α在48小时时似乎抑制增殖(0.317±0.024对0.458±0.046,P<0.01),但在96小时时似乎促进增殖(0.956±0.030对0.810±0.011,P<0.01)。与对照组(0μg/L)相比,rhTNF-α(1、5、10、50和100μg/L)显著增加hADSCs的VEGF、FGF-2和IGF-1分泌(P<0.01)。成骨分化后,hADSCs(未用rhTNF-α处理)的这3种生长因子分泌随天数增加而升高。在10μg/L rhTNF-α刺激下,成骨分化1天后的hADSCs与未用rhTNF-α处理的组相比,VEGF分泌显著增加(P<0.01);成骨分化3天和7天后,hADSCs的VEGF(P<0.01)、FGF-2(P<0.05)和IGF-1(P<0.05)分泌显著增加。然而,成骨分化14天后,10μg/L rhTNF-α似乎抑制分化后hADSCs的VEGF(P<0.01)、FGF-2(P<0.05)和IGF-1(P<0.05)分泌。
在一定浓度范围内,rhTNF-α可促进hADSCs的增殖以及VEGF、FGF-2和IGF-1的分泌。10μg/L rhTNF-α对分化后hADSCs的VEGF、FGF-2和IGF-1分泌在成骨分化的不同阶段有不同影响。
