Abstract
BackgroundNeuroinflammation accompanies neural trauma and most neurological diseases. Axotomy in the peripheral nervous system (PNS) leads to dramatic changes in the injured neuron: the cell body expresses a distinct set of genes known as regeneration-associated genes, the distal axonal segment degenerates and its debris is cleared, and the axons in the proximal segment form growth cones and extend neurites. These processes are orchestrated in part by immune and other non-neuronal cells. Macrophages in ganglia play an integral role in supporting regeneration. Here, we explore further the molecular and cellular components of the injury-induced immune response within peripheral ganglia.MethodsAdult male wild-type (WT) and Ccr2−/− mice were subjected to a unilateral transection of the sciatic nerve and axotomy of the superior cervical ganglion (SCG). Antibody arrays were used to determine the expression of chemokines and cytokines in the dorsal root ganglion (DRG) and SCG. Flow cytometry and immunohistochemistry were utilized to identify the cellular composition of the injury-induced immune response within ganglia.ResultsChemokine expression in the ganglia differed 48 h after nerve injury with a large increase in macrophage inflammatory protein-1γ in the SCG but not in the DRG, while C-C class chemokine ligand 2 was highly expressed in both ganglia. Differences between WT and Ccr2−/− mice were also observed with increased C-C class chemokine ligand 6/C10 expression in the WT DRG compared to C-C class chemokine receptor 2 (CCR2)−/− DRG and increased CXCL5 expression in CCR2−/− SCG compared to WT. Diminished macrophage accumulation in the DRG and SCG of Ccr2−/− mice was found compared to WT ganglia 7 days after nerve injury. Interestingly, neutrophils were found in the SCG but not in the DRG. Cytokine expression, measured 7 days after injury, differed between ganglion type and genotype. Macrophage activation was assayed by colabeling ganglia with the anti-inflammatory marker CD206 and the macrophage marker CD68, and an almost complete colocalization of the two markers was found in both ganglia.ConclusionsThis study demonstrates both molecular and cellular differences in the nerve injury-induced immune response between DRG and SCG and between WT and Ccr2−/− mice.
Highlights
Neuroinflammation accompanies neural trauma and most neurological diseases
By inhibiting macrophage accumulation within the superior cervical ganglion (SCG) and dorsal root ganglion (DRG) following axotomy using a global knockout of the chemokine receptor Ccr2 (Ccr2−/−), we showed that in vitro axonal regeneration is significantly reduced when the injury-induced immune response in ganglia is impaired [14]
Robust expression of both Macrophage inflammatory protein-1 gamma (MIP-1γ) and C motif chemokine ligand 2 (CCL2) in the SCG could explain the early and significant accumulation of macrophages that we observed in the axotomized sympathetic ganglia at 1 day post injury, compared to the typical increase in the macrophage response observed in the injured DRG after 3 days [11, 12]
Summary
Axotomy in the peripheral nervous system (PNS) leads to dramatic changes in the injured neuron: the cell body expresses a distinct set of genes known as regeneration-associated genes, the distal axonal segment degenerates and its debris is cleared, and the axons in the proximal segment form growth cones and extend neurites. These processes are orchestrated in part by immune and other non-neuronal cells. Macrophage responses to a peripheral axonal injury occur in two distinct compartments: the nerve distal to the injury site and the axotomized ganglion. Macrophage numbers remain elevated in the nerve for at least 30 days after injury [6]
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