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在骨关节炎三维培养模型中,卡洛芬和地塞米松对犬软骨细胞的影响。

Effects of carprofen and dexamethasone on canine chondrocytes in a three-dimensional culture model of osteoarthritis.

作者信息

Dvorak Laura D, Cook James L, Kreeger John M, Kuroki Keiichi, Tomlinson James L

机构信息

Department of Veterinary Medicine and Surgery, College of Veterinary Medicine, University of Missouri, Columbia 65211, USA.

出版信息

Am J Vet Res. 2002 Oct;63(10):1363-9. doi: 10.2460/ajvr.2002.63.1363.

Abstract

OBJECTIVE

To determine effects of carprofen and dexamethasone on chondrocytes in a culture model of osteoarthritis (OA).

SAMPLE POPULATION

Chondrocytes isolated from articular cartilage of the humeral head of 5 adult dogs.

PROCEDURE

Chondrocytes were harvested, cultured and subcultured in monolayer, and then cultured in a 3-dimensional (3-D) medium. Cells from each dog were distributed into 6 groups with differing content of liquid medium for each 3-D construct (agarose [AG], AG plus interleukin [IL]-1beta, AG plus carprofen [4 microg/mL], AG plus dexamethasone [1 mg/mL], AG plus IL-1beta [20 ng/mL] plus carprofen [4 microg/mL], and AG plus IL-1beta (20 ng/mL) plus dexamethasone (1 mg/mL). On days 3, 6, 12, and 20 of culture, samples from all groups were collected. Liquid media were assayed for glycosaminoglycan, prostaglandin (PG)E2, matrix metalloprotease (MMP)-3, and MMP-13 concentrations. All 3-D constructs were evaluated for viability, cell morphology, proteoglycan staining, and collagen type-II concentration. Total glycosaminoglycan content in each 3-D construct was quantitated by spectrophotometric assay.

RESULTS

Addition of IL-1beta caused a significant loss of cell viability and matrix production. Addition of carprofen or dexamethasone caused significant decreases in PGE2 in the liquid media, and each was minimally effective in protecting chondrocytes against negative effects of IL-1beta.

CONCLUSIONS AND CLINICAL RELEVANCE

Human recombinant IL-1beta resulted in loss of cell viability, alterations in extracellular matrix components, and production of PG and MMP Carprofen and dexamethasone had little effect on cell and matrix variables but did decrease PGE2 concentrations and primarily affected the inflammatory pathway of osteoarthritis.

摘要

目的

在骨关节炎(OA)培养模型中确定卡洛芬和地塞米松对软骨细胞的影响。

样本群体

从5只成年犬肱骨头关节软骨分离出的软骨细胞。

程序

收获软骨细胞,在单层中培养和传代培养,然后在三维(3-D)培养基中培养。将每只犬的细胞分配到6组,每组3-D构建体(琼脂糖[AG]、AG加白细胞介素[IL]-1β、AG加卡洛芬[4微克/毫升]、AG加地塞米松[1毫克/毫升]、AG加IL-1β[20纳克/毫升]加卡洛芬[4微克/毫升]、AG加IL-1β[20纳克/毫升]加地塞米松[1毫克/毫升])的液体培养基含量不同。在培养的第3、6、12和20天,收集所有组的样本。检测液体培养基中的糖胺聚糖、前列腺素(PG)E2、基质金属蛋白酶(MMP)-3和MMP-13浓度。对所有3-D构建体进行活力、细胞形态、蛋白聚糖染色和II型胶原浓度评估。通过分光光度法测定每个3-D构建体中的总糖胺聚糖含量。

结果

添加IL-1β导致细胞活力和基质产生显著丧失。添加卡洛芬或地塞米松导致液体培养基中PGE2显著降低,且二者在保护软骨细胞免受IL-1β负面影响方面效果甚微。

结论及临床意义

人重组IL-1β导致细胞活力丧失、细胞外基质成分改变以及PG和MMP产生。卡洛芬和地塞米松对细胞和基质变量影响较小,但确实降低了PGE2浓度,且主要影响骨关节炎的炎症途径。

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