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酶消化对组织工程中膝关节半月板细胞产量和表型的区域性影响。

Regional effects of enzymatic digestion on knee meniscus cell yield and phenotype for tissue engineering.

机构信息

Department of Bioengineering, Rice University, Houston, TX, USA.

出版信息

Tissue Eng Part C Methods. 2012 Mar;18(3):235-43. doi: 10.1089/ten.TEC.2011.0383. Epub 2011 Dec 2.

Abstract

An abundant cell source is the cornerstone of most tissue engineering strategies, but extracting cells from the knee meniscus is hindered by its dense fibrocartilaginous matrix. Identifying a method to efficiently isolate meniscus cells is important, as it can reduce the cost and effort required to perform meniscus engineering research. In this study, six enzymatic digestion regimens used for cartilaginous cell isolation were used to isolate cells from the outer, middle, and inner regions of the bovine knee meniscus. Each regimen in each region was assessed in terms of cell yield, impact on cell phenotype, and cytotoxicity. All digestion regimens caused an overall upregulation of cartilage-specific genes Sox9, collagen type I (Col 1), collagen type II (Col 2), cartilage oligomeric matrix protein, and aggrecan (AGC) in cells from all meniscus regions, but was highest for cells isolated using 1075 U/mL of collagenase for 3 h (high collagenase). In response to isolation, outer meniscus cells showed highest upregulation of Sox9 and Col 1 genes, whereas greatest upregulation for middle meniscus cells was seen in Col 1 expression, and Col 2 expression for inner cells. Cell yield was highest in all regions when subjected to 45 min of 61 U/mL pronase followed by 3 h of 1075 U/mL collagenase (pronase/collagenase [P/C]) digestion regimen (outer: 6.57±0.37, middle: 12.77±1.41, inner: 22.17±1.47×10(6) cells/g tissue). The second highest cell yield was achieved using the low collagenase (LC) digestion regimen that applied 433 U/mL of collagenase for 18 h (outer: 1.95±0.54, middle: 3.3±4.4, inner: 6.06±2.44×10(6) cells/g tissue). Cytotoxicity analysis showed higher cell death in the LC group compared with the P/C group. Self-assembled constructs formed from LC-isolated cells were less dense than constructs formed from P/C-isolated cells, and P/C constructs showed higher glycosaminoglycan content and compressive moduli than LC constructs. All isolation methods tested resulted in similar phenotypic changes in meniscus cells from each region. These results indicate that, compared with other common isolation protocols, the P/C isolation method is able to more efficiently isolate meniscus cells from all regions that can produce tissue engineered constructs.

摘要

一种丰富的细胞来源是大多数组织工程策略的基石,但从膝关节半月板中提取细胞受到其致密的纤维软骨基质的阻碍。鉴定一种有效分离半月板细胞的方法很重要,因为它可以降低进行半月板工程研究所需的成本和工作量。在这项研究中,使用了六种用于软骨细胞分离的酶消化方案来分离牛膝关节半月板的外、中、内区域的细胞。在每个区域的每个方案中,都根据细胞产量、对细胞表型的影响和细胞毒性进行了评估。所有消化方案均导致所有半月板区域的细胞中软骨特异性基因 Sox9、I 型胶原(Col 1)、II 型胶原(Col 2)、软骨寡聚基质蛋白和聚集蛋白聚糖(AGC)的整体上调,但用 1075U/mL 胶原酶处理 3 小时(高胶原酶)的细胞上调最为明显。在对外、中、内半月板细胞进行分离时,细胞对外半月板细胞 Sox9 和 Col 1 基因的上调作用最高,而中半月板细胞的 Col 1 表达上调最大,内半月板细胞的 Col 2 表达上调最大。在用 61U/mL 蛋白酶处理 45 分钟,然后用 1075U/mL 胶原酶处理 3 小时的(蛋白酶/胶原酶[P/C])消化方案中,所有区域的细胞产量均最高(外:6.57±0.37,中:12.77±1.41,内:22.17±1.47×10(6)个细胞/g 组织)。第二个最高的细胞产量是用低胶原酶(LC)消化方案获得的,该方案应用 433U/mL 胶原酶 18 小时(外:1.95±0.54,中:3.3±4.4,内:6.06±2.44×10(6)个细胞/g 组织)。细胞毒性分析表明,LC 组的细胞死亡率高于 P/C 组。与 P/C 分离细胞形成的自组装结构相比,LC 分离细胞形成的结构密度较低,并且 P/C 结构的糖胺聚糖含量和压缩模量均高于 LC 结构。测试的所有分离方法均导致每个区域的半月板细胞发生相似的表型变化。这些结果表明,与其他常见的分离方案相比,P/C 分离方法能够更有效地从所有区域分离半月板细胞,从而产生组织工程构建体。

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