Iopromide- and gadopentetic acid-derived preparates used in MR arthrography may be harmful to chondrocytes
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info:eu-repo/semantics/openAccessCC0 1.0 Universalhttps://creativecommons.org/publicdomain/zero/1.0/Tarih
2017Yazar
Öznam, KadirŞirin, Duygu Yaşar
Yılmaz, İbrahim
Kaya, Yasin Emre
İşyar, Mehmet
Gümüştaş, Seyit Ali
Özbek, Hanefi
Akkaya, Semih
Kayhan, Arda
Mahiroğulları, Mahir
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Öznam, K., Şirin, D. Y., Yılmaz, İ., Kaya, Y. E., İşyar, M., Gümüştaş, S. A. ... Mahiroğulları, M. (2017). Iopromide- and gadopentetic acid-derived preparates used in MR arthrography may be harmful to chondrocytes. Journal of Orthopaedic Surgery and Research, 12. https://dx.doi.org/10.1186/s13018-017-0600-5Özet
Background: Magnetic resonance arthrography, a procedure through which contrast agents containing gadolinium and/or iopromide are administered intra-articularly, has become a useful tool in musculoskeletal diagnosis. Nevertheless, despite being considered safe for systemic use, certain tissue toxicities have been identified for both drugs. In this study, the effects of short-term exposure of human primary chondrocyte cell cultures to gadolinium and/or iopromide contrast agents were examined by assaying for stage-specific embryonic antigen-1 (SSEA-1) protein expression (a chondrogenic differentiation marker), cell viability, toxicity, and proliferation. Methods: Human articular chondrocytes were grown in monolayer culture and were exposed to iopromide and/or gadolinium diethylenetriamine-pentaacetate (Gd-DPT) for 2 and 6 h. Cell cultures with no drug exposure were used as the control group. Cell differentiation status was assessed according to SSEA-1 protein expression. Contrast agent effects on cell viability and proliferation were analyzed using MTT analysis. Further, changes in cell morphology in relation to the control group were evaluated using inverted light microscopy, environmental scanning electron microscopy (ESEM), and 3-tesla magnetic resonance imaging. The obtained data were statistically compared. Results: When compared with the control group, both SSEA-1 protein expression and cell proliferation were lowest in the Gd-DPT group (P = 0.000). There was a statistically significant correlation between SSEA-1 expression and MTT results (rho = 0.351; P = 0.003). Conclusions: Nevertheless, the data obtained from in vitro experiments may not directly correspond to clinical applications. However, the mere fact that a drug used solely for diagnostic purposes may repress chondrocyte cell proliferation should be carefully considered by clinicians.
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Journal of Orthopaedic Surgery and ResearchCilt
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