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Effect of the disruption of three cytoskeleton components on chondrocyte metabolism in rabbit knee cartilage

         

摘要

Background Chondrocytes' phenotype and biosynthesis of matrix are dependent on having an intact cytoskeletal structure.Microfilaments,microtubules,and intermediate filaments are three important components of the cytoskeletal structure of chondrocytes.The aims of this study were to determine and compare the effects of the disruption of these three cytoskeletal elements on the apoptosis and matrix synthesis by rabbit knee chondrocytes in vitro.Methods Chondrocytes were isolated from full-thickness knee cartilage of two-month-old rabbits using enzymatic methods (n=24).The isolated cells were stabilized for three days and then exposed to low,medium,and high doses of chemical agents that disrupt the three principal cytoskeletal elements of interest:colchicine for microtubules,acrylamide for intermediate filaments,and cytochalasin D for actin microfilaments.A group of control cells were treated with carrier.Early apoptosis was assessed using the Annexin-FITC binding assay by flow cytometry on days 1 and 2 after exposure to the disrupting chemical agents.The components and distribution of the cytoskeleton within the cells were analyzed by laser scanning confocal microscopy (LSCM) with immunofluorescence staining on day 3.The mRNA levels of aggrecan (AGG) and type Ⅱ collagen (Col-2) and their levels in culture medium were analyzed using real-time PCR and enzymelinked immunosorbent serologic assay (ELISA) on days 3,6,and 9.Results In the initial drug-dose-response study,there was no significant difference in the vitality of cells treated with 0.1 μmol/L colchicine,2.5 mmol/L acrylamide,and 10 μg/L cytochalasin D for two days when compared with the control group of cells.The concentrations of colchicine and acrylamide treatment selected above significantly decreased the number of viable cells over the nine-day culture and disrupted significantly more cell nuclei.Real-time PCR and ELISA results showed that the mRNA levels and medium concentrations of AGG and Col-2 were significantly decreased for cultures treated with colchicine and acrylamide when compared with untreated cells at three,six,and nine days,and this inhibition was correlated with higher matrix metalloprotease-13 expression in these cells.Cellular proliferation,monolayer morphology,and matrix metabolism were unaffected in cytochalasin D-treated cells when compared with control cells over the nine-day culture period.Conclusions The disruption of the microtubulin and intermediate filaments induced chondrocyte apoptosis,increased matrix metalloprotease expression,and decreased AGG and Col-2 expression in rabbit knee chondrocyte cultures.Our findings suggest that microtubulin and intermediate filaments play a critical role in the synthesis of cartilage matrix by rabbit knee chondrocytes.

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  • 来源
    《中华医学杂志(英文版)》 |2014年第21期|3764-3770|共7页
  • 作者单位

    Department of Orthopaedics, Second Hospital of Shanxi Medical University;

    Shanxi Key Lab of Bone and Soft Tissue Injury Repair, Taiyuan, Shanxi 030001, China;

    Department of Orthopaedics, The Warren Alpert Medical School of Brown University/Rhode Island Hospital, Providence RI 02903, USA;

    Department of Orthopaedics, Second Hospital of Shanxi Medical University;

    Shanxi Key Lab of Bone and Soft Tissue Injury Repair, Taiyuan, Shanxi 030001, China;

    Department of Orthopaedics, Second Hospital of Shanxi Medical University;

    Shanxi Key Lab of Bone and Soft Tissue Injury Repair, Taiyuan, Shanxi 030001, China;

    Department of Orthopaedics, Second Hospital of Shanxi Medical University;

    Shanxi Key Lab of Bone and Soft Tissue Injury Repair, Taiyuan, Shanxi 030001, China;

    Department of Orthopaedics, Second Hospital of Shanxi Medical University;

    Shanxi Key Lab of Bone and Soft Tissue Injury Repair, Taiyuan, Shanxi 030001, China;

    Department of Orthopaedics, Second Hospital of Shanxi Medical University;

    Shanxi Key Lab of Bone and Soft Tissue Injury Repair, Taiyuan, Shanxi 030001, China;

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