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可生物降解聚合物在人关节软骨细胞软骨形成中的作用

Biodegradable polymers in chondrogenesis of human articular chondrocytes.

作者信息

Banu Nasreen, Banu Yasmin, Sakai Masamune, Mashino Tadahiko, Tsuchiya Toshie

机构信息

Division of Medical Devices, National Institute of Health Sciences, 1-18-1 Kamiyoga, Setagaya-ku, Tokyo, 158-8501, Japan.

出版信息

J Artif Organs. 2005;8(3):184-91. doi: 10.1007/s10047-005-0302-3.

Abstract

The aim of this study was to evaluate the potential role of polyglycolic acid (PGA), poly(glycolic acid-epsilon-caprolactone) (PGCL), poly(L-lactic acid-glycolic acid) (PLGA), poly(L-lactic acid-epsilon-caprolactone, 75:25 (w/w)) [P(LA-CL)25], poly-epsilon-caprolactone (tetrabutoxy titanium) [PCL(Ti)], and fullerene C-60 dimalonic acid (DMA) in cartilage transplants. After 4 weeks of culture of human articular cartilage, the levels of cell proliferation and differentiation and the expression of cartilage-specific matrix genes were estimated. The relationship between cell differentiation and gap junction protein connexin 43 (Cx43) was also evaluated. All materials except PCL(Ti) retained cell proliferation activities similar to the controls. Cell differentiation levels from the highest to the lowest were in the following order: PGA >> PLGA > PGCL > Control = DMSO > P(LA-CL)25 = PCL(Ti) >> fullerene C-60 DMA. Expression of the collagen type II gene was selectively upregulated for PGA, PGCL, and PLGA and slightly increased for P(LA-CL)25 polymers but was downregulated for fullerene C-60 DMA. Aggrecan gene expression was strongest with PGA and was consistently expressed with other matrices, especially with PGCL and PLGA. However, the expression patterns of the connexin 43 gene were different from the former two genes. Multiple regression analysis revealed a high correlation between cartilage proteoglycans production and expression levels of these three genes.

摘要

本研究的目的是评估聚乙醇酸(PGA)、聚(乙醇酸-ε-己内酯)(PGCL)、聚(L-乳酸-乙醇酸)(PLGA)、聚(L-乳酸-ε-己内酯,75:25(w/w))[P(LA-CL)25]、聚-ε-己内酯(四丁氧基钛)[PCL(Ti)]和富勒烯C-60二丙二酸(DMA)在软骨移植中的潜在作用。在对人关节软骨进行4周培养后,评估细胞增殖和分化水平以及软骨特异性基质基因的表达。还评估了细胞分化与间隙连接蛋白连接蛋白43(Cx43)之间的关系。除PCL(Ti)外,所有材料均保持与对照相似的细胞增殖活性。细胞分化水平从高到低依次为:PGA >> PLGA > PGCL >对照 = 二甲基亚砜 > P(LA-CL)25 = PCL(Ti) >> 富勒烯C-60 DMA。II型胶原基因的表达在PGA、PGCL和PLGA中被选择性上调,在P(LA-CL)25聚合物中略有增加,但在富勒烯C-60 DMA中被下调。聚集蛋白聚糖基因表达在PGA中最强,在其他基质中持续表达,尤其是在PGCL和PLGA中。然而,连接蛋白43基因的表达模式与前两个基因不同。多元回归分析显示软骨蛋白聚糖产生与这三个基因的表达水平之间存在高度相关性。

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