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Herniated Intervertebral Disk Induces Hypertrophy and Ossification of Ligamentum Flavum

Authors
Kang, Young-MiSuk, Kyung-SooLee, Byung HoKim, Hak-SunLee, Kwang-IlPark, Si-YoungLee, Hwan-MoMoon, Seong-Hwan
Issue Date
Oct-2014
Publisher
LIPPINCOTT WILLIAMS & WILKINS
Keywords
ligamentum flavum; intervertebral disk; degeneration; hypertrophy; ossification
Citation
JOURNAL OF SPINAL DISORDERS & TECHNIQUES, v.27, no.7, pp.382 - 389
Indexed
SCIE
SCOPUS
Journal Title
JOURNAL OF SPINAL DISORDERS & TECHNIQUES
Volume
27
Number
7
Start Page
382
End Page
389
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/97283
ISSN
1536-0652
Abstract
Study Design: In vitro experiment using degenerated human ligamentum flavum (LF) and herniated intervertebral disk (IVD). Objectives: To investigate the role and effect of degenerated and herniated IVDs on LF hypertrophy and ossification. Summary of Background Data: Spinal stenosis is caused, in part, by hypertrophy and ossification of the LF, which are induced by aging and degenerative process. It is well known that degenerated IVDs spontaneously produce inflammatory cytokines. Therefore, we hypothesized that degenerated IVD may affect adjacent LF through secreted inflammatory cytokines. Methods: LF and herniated lumbar IVD tissues were obtained during surgical spinal procedures. LF fibroblasts were isolated by enzymatic digestion of LF tissue. LF cell cultures were treated with disk supernatant from herniated IVDs. Secreted cytokines from IVD tissue culture were detected by enzyme-linked immunosorbent assay. After analysis of cytotoxicity, DNA synthesis was measured. Reverse transcription-polymerase chain reaction for mRNA expressions of types I, II, III, V, and XI collagen and osteocalcin, and histochemical stains were performed. Results: Supernatant from tissue culture of herniated IVD showed increased production of interleukin-1 alpha, interleukin-6, tumor necrosis factor-a, prostaglandin E-2, and nitric oxide compared with disk tissue culture from traumatic condition. There was no cytotoxicity in LF cells treated with disk supernatant from herniated IVDs. There was significant increase in DNA synthesis, upregulation in mRNA expression of types III, XI collagen and osteocalcin, whereas variable expression pattern of type I and V, and strong positive stains for Von Kossa and alkaline phosphatase in LF cultures with disk supernatant. Conclusions: Degenerated and herniated IVDs provide an important pathomechanism in hypertrophy and ossification of the LF through inflammatory cytokines.
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