Abraham Leah C, Vorrasi John, Kaplan David L
Departments of Chemical and Biological Engineering and Biomedical Engineering; and Bioengineering Center, Tufts University, Medford, Massachusetts 02155, USA.
J Biomed Mater Res A. 2004 Jul 1;70(1):39-48. doi: 10.1002/jbm.a.30057.
Biodegradation of collagen biomaterial matrices and the deposition of new collagen extracellular matrix (ECM) are critical to the integration of in vitro bioengineered materials and tissues in vivo. In previous studies, we observed significant impact of collagen matrix structure on primary lung fibroblast behavior in vitro. In the present work, to begin to understand the mechanistic basis for our previous observation, the response of human fibroblasts (IMR-90) to the structural state of collagen matrices was studied with respect to cell proliferation, cell morphology, beta-galactosidase level, and transcript content for collagen (Col-1), matrix metalloproteinases (MMP-1, MMP-2), tissue inhibitors of matrix metalloproteinase (TIMP-1 and TIMP-2). Collagen digestion was assessed quantitatively by uptake of collagen-coated fluorescent beads incorporated in the preformed collagen matrix. Transcript levels related to the deposition of new ECM proteins varied as a function of the structure of the collagen matrix presented to the cells. Col-1 expression was 2-fold higher and expression for MMP-1, MMP-2, TIMP-1, and TIMP-2 increased for cells when grown on 156 microg/cm2 denatured collagen compared with cells grown on tissue culture (TC) plastic. On 156 microg/cm2 nondenatured (native) collagen, Col-1 expression was decreased by half and MMP-2 was increased by 2.5-fold compared with cells grown on TC plastic. On 78 microg/cm2 denatured collagen, Col-1 expression was 80% whereas the MMPs and TIMPs were increased by 1.25- to 2-fold compared with cells grown on TC plastic. On 78 microg/cm2 nondenatured collagen expression of all 5 transcripts was reduced 60-90% of the levels determined for the cells grown on TC plastic. Cell viability, based on cell morphology and beta-galactosidase activity, was improved on the denatured collagen. A higher level of collagen matrix incorporation was observed for cells grown on denatured collagen than on nondenatured collagen or TC plastic. These data suggest that tissue engineering matrices incorporating denatured collagen may promote more active remodeling toward new ECM in comparison to cells grown on nondenatured collagen or cells grown on TC plastic.
胶原蛋白生物材料基质的生物降解以及新的胶原蛋白细胞外基质(ECM)的沉积对于体外生物工程材料和组织在体内的整合至关重要。在先前的研究中,我们观察到胶原蛋白基质结构对体外原代肺成纤维细胞行为有显著影响。在本研究中,为了开始理解我们先前观察结果的机制基础,研究了人成纤维细胞(IMR-90)对胶原蛋白基质结构状态在细胞增殖、细胞形态、β-半乳糖苷酶水平以及胶原蛋白(Col-1)、基质金属蛋白酶(MMP-1、MMP-2)、基质金属蛋白酶组织抑制剂(TIMP-1和TIMP-2)转录本含量方面的反应。通过摄取预先形成的胶原蛋白基质中掺入的胶原蛋白包被荧光珠来定量评估胶原蛋白消化情况。与新ECM蛋白沉积相关的转录本水平随呈现给细胞的胶原蛋白基质结构而变化。与在组织培养(TC)塑料上生长的细胞相比,当细胞在156μg/cm²变性胶原蛋白上生长时,Col-1表达高出2倍,MMP-1、MMP-2、TIMP-1和TIMP-2的表达增加。与在TC塑料上生长的细胞相比,在156μg/cm²非变性(天然)胶原蛋白上,Col-1表达降低一半,MMP-2增加2.5倍。与在TC塑料上生长的细胞相比,在78μg/cm²变性胶原蛋白上,Col-1表达为80%,而MMP和TIMP增加1.25至2倍。在78μg/cm²非变性胶原蛋白上,所有5种转录本的表达降低至在TC塑料上生长的细胞所确定水平的60 - 90%。基于细胞形态和β-半乳糖苷酶活性的细胞活力在变性胶原蛋白上有所改善。与在非变性胶原蛋白或TC塑料上生长的细胞相比,在变性胶原蛋白上生长的细胞观察到更高水平的胶原蛋白基质掺入。这些数据表明,与在非变性胶原蛋白上生长的细胞或在TC塑料上生长的细胞相比,包含变性胶原蛋白的组织工程基质可能促进向新ECM的更活跃重塑。
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