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Merck
CN

Energy Metabolism During Osteogenic Differentiation: The Role of Akt.

Stem cells and development (2020-12-15)
Charles Owen Smith, Roman A Eliseev
摘要

Osteogenic differentiation, the process by which bone marrow mesenchymal stem/stromal (a.k.a. skeletal stem) cells and osteoprogenitors form osteoblasts, is a critical event for bone formation during development, fracture repair, and tissue maintenance. Extra cellular and intracellular signaling pathways triggering osteogenic differentiation are relatively well known; however, the ensuing change in cell energy metabolism is less clearly defined. We and others have previously reported activation of mitochondria during osteogenic differentiation. To further elucidate the involved bioenergetic mechanisms and triggers, we tested the effect of osteogenic media containing ascorbate and β-glycerol phosphate, or various osteogenic hormones and growth factors on energy metabolism in long bone (ST2)- and calvarial bone (MC3T3-E1)-derived osteoprogenitors. We show that osteogenic media and differentiation factors, Wnt3a and BMP2, stimulate mitochondrial oxidative phosphorylation (OxPhos) with little effect on glycolysis. The activation of OxPhos occurs acutely, suggesting a metabolic signaling change rather than protein expression change. To this end, we found that the observed mitochondrial activation is Akt dependent. Akt is activated by osteogenic media, Wnt3a, and BMP2, leading to increased phosphorylation of various mitochondrial Akt targets, a phenomenon known to stimulate OxPhos. In sum, our data provide comprehensive analysis of cellular bioenergetics during osteoinduction in cells of two different origins (mesenchyme vs neural crest) and identify Wnt3a and BMP2 as physiological stimulators of mitochondrial respiration through Akt activation.

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Sigma-Aldrich
D -(+)-葡萄糖, ≥99.5% (GC)
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羰基氰化物 4-(三氟甲氧基)苯腙, ≥98% (TLC), powder
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鱼藤酮, ≥95%
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L -抗坏血酸, suitable for cell culture, suitable for plant cell culture, ≥98%
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杜氏改良 Eagle 培养基-低葡萄糖, Without glucose, L-glutamine, phenol red, sodium pyruvate and sodium bicarbonate, powder, suitable for cell culture
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Akt1/2激酶抑制剂, ≥98% (HPLC)
Supelco
雷复尼特, PESTANAL®, analytical standard