Moioli Eduardo K, Hong Liu, Guardado Jesse, Clark Paul A, Mao Jeremy J
Tissue Engineering Laboratory, University of Illinois at Chicago, Illinois, USA.
Tissue Eng. 2006 Mar;12(3):537-46. doi: 10.1089/ten.2006.12.537.
Despite the widespread role of transforming growth factor-beta3 (TGFbeta3) in wound healing and tissue regeneration, its long-term controlled release has not been demonstrated. Here, we report microencapsulation of TGFbeta3 in poly-d-l-lactic-co-glycolic acid (PLGA) microspheres and determine its bioactivity. The release profiles of PLGA-encapsulated TGFbeta3 with 50:50 and 75:25 PLA:PGA ratios differed throughout the experimental period. To compare sterilization modalities of microspheres, bFGF was encapsulated in 50:50 PLGA microspheres and subjected to ethylene oxide (EO) gas, radio-frequency glow discharge (RFGD), or ultraviolet (UV) light. The release of bFGF was significantly attenuated by UV light, but not significantly altered by either EO or RFGD. To verify its bioactivity, TGFbeta3 (1.35 ng/mL) was control-released to the culture of human mesenchymal stem cells (hMSC) under induced osteogenic differentiation. Alkaline phosphatase staining intensity was markedly reduced 1 week after exposing hMSC-derived osteogenic cells to TGFbeta3. This was confirmed by lower alkaline phosphatase activity (2.25 +/- 0.57 mU/mL/ng DNA) than controls (TGFbeta3- free) at 5.8 +/- 0.9 mU/mL/ng DNA (p < 0.05). Control-released TGFbeta3 bioactivity was further confirmed by lack of significant differences in alkaline phosphatase upon direct addition of 1.35 ng/mL TGFbeta3 to cell culture (p > 0.05). These findings provide baseline data for potential uses of microencapsulated TGFbeta3 in wound healing and tissue-engineering applications.
尽管转化生长因子β3(TGFβ3)在伤口愈合和组织再生中具有广泛作用,但其长期控释尚未得到证实。在此,我们报道了TGFβ3在聚-d-丙交酯-乙交酯共聚物(PLGA)微球中的微囊化,并测定了其生物活性。在整个实验期间,具有50:50和75:25 PLA:PGA比例的PLGA包封的TGFβ3的释放曲线有所不同。为了比较微球的灭菌方式,将碱性成纤维细胞生长因子(bFGF)包封在50:50的PLGA微球中,并进行环氧乙烷(EO)气体、射频辉光放电(RFGD)或紫外线(UV)照射处理。UV光显著减弱了bFGF的释放,但EO或RFGD处理对其释放没有显著影响。为了验证其生物活性,将TGFβ3(1.35 ng/mL)在诱导成骨分化条件下对人间充质干细胞(hMSC)进行控释培养。将hMSC来源的成骨细胞暴露于TGFβ3 1周后,碱性磷酸酶染色强度明显降低。这通过碱性磷酸酶活性(2.25±0.57 mU/mL/ng DNA)低于对照组(无TGFβ3)的5.8±0.9 mU/mL/ng DNA得到证实(p<0.05)。在细胞培养中直接添加1.35 ng/mL TGFβ3后碱性磷酸酶无显著差异(p>0.05),进一步证实了控释TGFβ3的生物活性。这些发现为微囊化TGFβ3在伤口愈合和组织工程应用中的潜在用途提供了基线数据。