Response of human peripheral blood monocyte-derived macrophages (PBMM) to demineralized and decellularized bovine bone graft substitutes.
K G Aghila RaniAhmed M Al-RawiAli Al QabbaniSausan AlKawasMohammad G MohammadA B Rani SamsudinPublished in: PloS one (2024)
The performance of apparently biocompatible implanted bovine bone grafts may be compromised by unresolved chronic inflammation, and poor graft incorporation leading to implant failure. Monitoring the intensity and duration of the inflammatory response caused by implanted bone grafts is crucial. In this study, the ability of demineralized (DMB) and decellularized (DCC) bovine bone substitutes in initiating inflammatory responses to peripheral blood monocyte-derived macrophages (PBMMs) was investigated. The response of PBMMs to bone substitutes was evaluated by using both direct and indirect cell culture, reactive oxygen species (ROS) generation, apoptosis, immunophenotyping, and cytokine production. Analysis of DMB and DCC substitutes using scanning electron microscope (SEM) showed a roughened surface with a size ranging between 500 and 750 μm. PBMMs treated with DMB demonstrated cell aggregation and clumping mimicking lipopolysaccharide (LPS) treated PBMMs and a higher proliferation ability (166.93%) compared to control (100%) and DCC treatments (115.64%; p<0.001) at 24h. This was associated with a significantly increased production of intracellular ROS in PBMMs exposed to DMB substitutes than control (3158.5 vs 1715.5; p<0.001) and DCC treatment (2117.5). The bone substitute exposure also caused an increase in percentage apoptosis which was significantly (p<0.0001) higher in both DMB (27.85) and DCC (29.2) treatment than control (19.383). A significant increase in proinflammatory cytokine expression (TNF-α: 3.4 folds; p<0.05) was observed in DMB substitute-treated PBMMs compared to control. Notably, IL-1β mRNA was significantly higher in DMB (21.75 folds; p<0.0001) than control and DCC (5.01 folds). In contrast, DCC substitutes exhibited immunoregulatory effects on PBMMs, as indicated by the expression for CD86, CD206, and HLDR surface markers mimicking IL-4 treatments. In conclusion, DMB excites a higher immunological response compared to DCC suggesting decellularization process of tissues dampen down inflammatory reactions when exposed to PBMM.
Keyphrases
- peripheral blood
- bone mineral density
- inflammatory response
- reactive oxygen species
- soft tissue
- oxidative stress
- bone loss
- cell death
- endothelial cells
- bone regeneration
- poor prognosis
- dna damage
- postmenopausal women
- endoplasmic reticulum stress
- magnetic resonance
- gene expression
- stem cells
- signaling pathway
- computed tomography
- long non coding rna
- immune response
- magnetic resonance imaging
- high intensity
- cell cycle arrest
- mesenchymal stem cells
- body composition
- high resolution
- combination therapy
- lipopolysaccharide induced
- single cell
- drug induced
- anti inflammatory
- pi k akt
- induced pluripotent stem cells
- contrast enhanced
- solar cells