What question did this study set out to answer?

Investigate the effects of co-culturing human stem cell-derived neural stem cells with chick embryonic dorsal root ganglia on sensory neuron maturation.

March 28, 2026Open Access

Functional sensory neurons derived from human stem cells from apical papilla

Key Points

Investigate the effects of co-culturing human stem cell-derived neural stem cells with chick embryonic dorsal root ganglia on sensory neuron maturation.
Isolated human stem cells from apical papilla of third molars
Induced stem cells into neural stem cells using 3D-neurosphere formation
Co-cultured neural stem cells with chick dorsal root ganglia under three conditions for 7 days
Evaluated neuronal differentiation using staining and calcium oscillation assays
Human stem cells successfully differentiated into neural stem cells under 3D conditions
Co-culture significantly increased differentiation into functional sensory neurons
Pseudounipolar sensory neurons exhibited positive staining for neuronal markers
Calcium oscillation activity indicated maturity of newly-formed neurons
The co-culture arrangement produced the highest proportion of sensory neurons compared to control conditions

Abstract

Objectives: This study aimed to investigate the sensory maturation–enhancing effects of co-culturing human stem cells from apical papilla (hSCAPs)-derived neural stem cells (NSCs) with chick embryonic dorsal root ganglia (DRG) under three-dimensional (3D) neurosphere conditions. The ultimate goal was to assess whether this co-culture approach promotes the generation of functional sensory neurons suitable for future sensory neuropathy transplantation applications. Methods: hSCAPs were isolated from the apical papilla of impacted third molars obtained from healthy Thai donors (n = 3; ages 18–21). The isolated hSCAPs were expanded and characterized for mesenchymal stem cell markers and multipotency. These cells were induced into NSCs via 3D-neurosphere formation. Embryonic chick DRG (E9) were dissected and co-cultured with NSCs under three experimental conditions: Co-culture, NeuroMat, and Control, for 7 days. Neuronal differentiation and maturation were evaluated by Cresyl violet staining, immunofluorescence staining for neuronal and glial markers, and intracellular calcium oscillation assays to assess functional activity. Results: hSCAPs exhibited MSC-like characteristics and successfully differentiated into NSCs under 3D-neurosphere conditions, expressing Nissl substance and early neurogenic markers (Nestin, SOX2). Co-culture with chick embryonic DRG significantly enhanced the differentiation of NSCs into functional sensory neurons. These neurons expressed neuronal-associated proteins including βIII-tubulin, MAP2, GFAP, and Brn3a, and demonstrated calcium oscillation activity indicative of mature, functional neurons. On day 7, the co-culture group exhibited the highest proportion of pseudounipolar sensory neurons (Cresyl violet positive), confirming the sensory maturation–enhancing effect of DRG co-culture on hSCAP-derived NSCs. Conclusions: Co-culture with embryonic DRG promotes the sensory neurogenic maturation of NSCs derived from hSCAPs, yielding functional pseudounipolar neurons. This model highlights the potential of hSCAPs as a promising stem cell source for neural regeneration and sensory neuropathy treatment.

Functional sensory neurons derived from human stem cells from apical papilla

Key Points

Abstract

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