转分化和葡萄糖阻断培养鸡胚神经视网膜细胞中的葡萄糖代谢:糖原和δ-结晶蛋白积累之间的反比关系

Saleh A.M. Karim, Michel Flor-Henry, David I. de Pomerai
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引用次数: 4

摘要

鸡胚神经视网膜(NR)细胞在低糖(FH)培养基中培养数周后可广泛转分化为晶状体,但在高水平补充葡萄糖(FHG)培养基中则不能。我们在这里表明,在高糖培养中,葡萄糖代谢的大多数方面都得到了促进,包括乳酸脱氢酶(LDH)和葡萄糖-6-磷酸脱氢酶(G-6-PDH)活性、2-脱氧葡萄糖摄取、戊糖分流活性和乳酸生成。持续补充低水平瓦阿因(FHGO)的高糖培养物可显著降低2-脱氧葡萄糖的摄取,从FHG水平下降到FH水平,特别是在NR培养的早期阶段。很久以后,在这些FHGO培养物中发生了广泛的转分化为透镜状体(伴随δ-结晶蛋白积累),因此类似于FHG而不是FHG对照。另一个受环境葡萄糖水平强烈影响的参数是糖原的积累。糖原本身和糖原合成酶活性在FHG培养中稳定增加,但在FH条件下略有下降。FHG培养中的糖原积累主要局限于神经胶质样细胞,特别是那些潜在的神经元簇。其他研究表明,与视网膜神经元的组织型相互作用促进了体外胶质细胞的分化。因此,高葡萄糖可能与神经元影响协同作用,刺激或稳定视网膜胶质细胞的正常分化,其体内特征包括糖原合成和储存。此外,我们发现,在高糖培养物中添加福斯克林或二丁基环AMP(两者都能促进糖原分解)会导致糖原积累速度减慢,并增强向晶状体的转分化。在这两个方面,补充福斯克林和二丁基camp的FHG培养介于FHG和FHG对照之间。因此,高葡萄糖增强NR培养的正常胶质细胞分化可能抑制或阻止随后向晶状体的转分化。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Glucose metabolism in transdifferentiating and glucose-blocked cultures of chick embryo neuroretinal cells: an inverse relationship between glycogen and δ-crystallin accumulation

Chick embryo neuroretinal (NR) cells transdifferentiate extensively into lens when cultured for several weeks in low-glucose (FH) medium, but fail to do so when high levels of supplementary glucose (FHG) are present. We show here that most aspects of glucose metabolism are promoted in high-glucose cultures, including lactate dehydrogenase (LDH) and glucose-6-phosphate dehydrogenase (G-6-PDH) activities, 2-deoxyglucose uptake, pentose shunt activity and lactate production. Continuous supplementation of high-glucose cultures with low levels of ouabain (FHGO) significantly lowers 2-deoxyglucose uptake, from FHG levels down towards FH levels, especially during the early stages of NR culture. Much later, extensive transdifferentiation into lentoids (with concomitant δ-crystallin accumulation) occurs in these FHGO cultures, which thus resemble FH rather than FHG controls. Another parameter strongly affected by ambient glucose levels is the accumulation of glycogen. Both glycogen itself and glycogen synthetase activity increase steadily in FHG cultures, but decrease slightly under FH conditions. Glycogen accumulation in FHG cultures is largely confined to glial-like cells, particularly those underlying clusters of neurones. Other studies have shown that glial differentiation in vitro is promoted by histotypic interactions with retinal neurones. Thus high glucose may act in concert with neuronal influences to stimulate or stabilize the normal differentiation of retinal glial cells, whose characteristic features in vivo include glycogen synthesis and storage. Furthermore, we show that supplementation of high-glucose cultures with forskolin or dibutyryl cyclic AMP (both of which promote glycogenolysis) results in a slower rate of glycogen accumulation and in enhanced transdifferentiation into lens. In both respects, the forskolin- and dibutyryl cAMP-supplemented FHG cultures are intermediate between FH and FHG controls. Thus the enhancement of normal glial differentiation in NR cultures by high glucose may inhibit or preclude subsequent transdifferentiation into lens.

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