Abstract
BackgroundThe lifetime prevalence of degenerative disc disease is dramatically high. Numerous investigations on disc degeneration have been performed on cells from annulus fibrosus (AF) and nucleus pulposus (NP) of the intervertebral disc (IVD) in cell culture experiments utilising a broad variety of basal culture media. Although the basal media differ in nutrient formulation, it is not known whether the choice of the basal media itself has an impact on the cell’s behaviour in vitro. In this study, we evaluated the most common media used for monolayer expansion of AF and NP cells to set standards for disc cell culture.MethodsHuman AF and NP cells were isolated from cervical discs. Cells were expanded in monolayer until passage P2 using six different common culture media containing alpha-Minimal Essential Medium (alpha-MEM), Dulbecco’s Modified Eagle’s Medium (DMEM) or Ham’s F-12 medium (Ham’s F-12) as single medium or in a mixture of two media (alpha/F-12, DMEM/alpha, DMEM/F-12). Cell morphology, cell growth, glycosaminoglycan production and quantitative gene expression of cartilage- and IVD-related markers aggrecan, collagen type II, forkhead box F1 and keratin 18 were analysed. Statistical analysis was performed with two-way ANOVA testing and Bonferroni compensation.ResultsAF and NP cells were expandable in all tested media. Both cell types showed similar cell morphology and characteristics of dedifferentiation known for cultured disc cells independently from the media. However, proceeding culture in Ham’s F-12 impeded cell growth of both AF and NP cells. Furthermore, the keratin 18 gene expression profile of NP cells was changed in alpha-MEM and Ham’s F-12.ConclusionThe impact of the different media itself on disc cell’s behaviour in vitro was low. However, AF and NP cells were only robust, when DMEM was used as single medium or in a mixture (DMEM/alpha, DMEM/F-12). Therefore, we recommend using these media as standard medium for disc cell culture. Our findings are valuable for the harmonisation of preclinical study results and thereby push the development of cell therapies for clinical treatment of disc degeneration.
Highlights
The lifetime prevalence of degenerative disc disease is dramatically high
The successful separation of annulus fibrosus (AF) from nucleus pulposus (NP) was confirmed by histological evaluation
In Ham’s Ham’s F-12 medium (F-12) NP cells did not reach same confluency compared to the other media at both AF and NP cells were expandable in all tested media
Summary
The lifetime prevalence of degenerative disc disease is dramatically high. Numerous investigations on disc degeneration have been performed on cells from annulus fibrosus (AF) and nucleus pulposus (NP) of the intervertebral disc (IVD) in cell culture experiments utilising a broad variety of basal culture media. The lifetime prevalence of degenerative disc disease (DDD) is very high. The IVD is a cartilage-like tissue and consists of two compartments, the inner nucleus pulposus (NP) and the surrounding annulus fibrosus (AF). Both contain specific cells that maintain the extracellular matrix (ECM) through synthesis and degradation of ECM proteins. Disc cells are adapted to the limited nutrient supply, an imbalance in the ECM maintenance occurs with age. Cell expansion is necessary to obtain a sufficient cell number for implantation These strategies aim to slow down the degeneration process and are predominantly tested in preclinical studies using cell culture experiments [5]
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