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从接受全关节置换术的老年患者软骨中建立原代软骨细胞培养时胶原酶不足。

Insufficiency of collagenases in establishment of primary chondrocyte culture from cartilage of elderly patients receiving total joint replacement.

作者信息

Mao Jiamin, Huang Lexi, Ding Yiyang, Ma Xiaoyu, Wang Quanming, Ding Lei

机构信息

Department of Basic Medical Sciences, Jiangnan University Wuxi College of Medicine, 1800 Lihu Avenue, Wuxi, 214122, Jiangsu, China.

Department of Orthopaedic Surgery, Jiangnan University Affiliated Hospital, Wuxi, Jiangsu, China.

出版信息

Cell Tissue Bank. 2023 Dec;24(4):759-768. doi: 10.1007/s10561-023-10094-0. Epub 2023 May 3.

Abstract

Background Collagenases are frequently used in chondrocyte isolation from articular cartilage. However, the sufficiency of this enzyme in establishing primary human chondrocyte culture remains unknown. Methods Cartilage slices shaved from femoral head or tibial plateau of patients receiving total joint replacement surgery (16 hips, 8 knees) were subjected to 0.02% collagenase IA digestion for 16 h with (N = 19) or without (N = 5) the pre-treatment of 0.4% pronase E for 1.5 h. Chondrocyte yield and viability were compared between two groups. Chondrocyte phenotype was determined by the expression ratio of collagen type II to I. The morphology of cultured chondrocytes was monitored with a light microscope.Results Cartilage with pronase E pre-treatment yielded significantly higher chondrocytes than that without the pre-treatment (3,399 ± 1,637 cells/mg wet cartilage vs. 1,895 ± 688 cells/mg wet cartilage; P = 0.0067). Cell viability in the former group was also significantly higher than that in the latter (94% ± 2% vs. 86% ± 6%; P = 0.03). When cultured in monolayers, cells from cartilage with pronase E pre-treatment grew in a single plane showing rounded shape while cells from the other group grew in multi-planes and exhibited irregular shape. The mRNA expression ratio of collagen type II to I was 13.2 ± 7.5 in cells isolated from cartilage pre-treated with pronase E, indicating a typical chondrocyte phenotype. Conclusions Collagenase IA was not sufficient in establishing primary human chondrocyte culture. Cartilage must be treated with pronase E prior to collagenase IA application.

摘要

背景 胶原酶常用于从关节软骨中分离软骨细胞。然而,这种酶在建立原代人软骨细胞培养方面的充分性尚不清楚。方法 从接受全关节置换手术的患者的股骨头或胫骨平台上刮下的软骨切片(16例髋关节,8例膝关节),用0.02% 胶原酶IA消化16小时,其中19例进行了1.5小时的0.4%链霉蛋白酶E预处理,5例未进行预处理。比较两组软骨细胞的产量和活力。通过II型与I型胶原的表达比来确定软骨细胞表型。用光学显微镜监测培养的软骨细胞的形态。结果 经链霉蛋白酶E预处理的软骨产生的软骨细胞明显高于未预处理的软骨(3399±1637个细胞/毫克湿软骨对1895±688个细胞/毫克湿软骨;P = 0.0067)。前一组的细胞活力也明显高于后一组(94%±2%对86%±6%;P = 0.03)。当单层培养时,经链霉蛋白酶E预处理的软骨细胞在单一平面上生长,呈圆形,而另一组的细胞在多个平面上生长,呈不规则形状。从经链霉蛋白酶E预处理的软骨中分离出的细胞中,II型与I型胶原的mRNA表达比为13.2±7.5,表明具有典型的软骨细胞表型。结论 胶原酶IA在建立原代人软骨细胞培养方面是不充分的。在应用胶原酶IA之前,软骨必须先用链霉蛋白酶E处理。

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