The kinetics and voltage dependence of asparagine (Asn)-induced depolarization in endoderm cells from Xenopus laevis embryos were analysed using current-clamp techniques. The depolarization is assumed to reflect the activation of an amino acid membrane carrier; it is accompanied by a slight increase in membrane resistance and cannot be explained by only the electrogenic character of the Asn carrier. It is proposed that the Asn depolarization arises, at least in part, from the decrease of the permeability ratio PK/PNa indirectly associated with the Na-coupled amino acid uptake. At room temperature (20-23 degrees C) the Asn response develops according to a single exponential function whose time constant is correlated with the final level of depolarization. Both amplitude and rise time of the depolarization are sensitive to variations of membrane potential and changes in Asn or Na external concentrations. Lowering the temperature decreases the amplitude of the Asn depolarization and increases its rise time with a Q10 factor of two; the kinetics remain of the Michaelis-Menten type, with a marked decrease in delta Emax and no change in Km. When the holding potential is altered by depolarizing and hyperpolarizing currents, the Asn response varies according to a bell-shaped characteristic presenting an optimum near the normal resting level. Membrane depolarizations induced by Na/K-pump inhibitors or high external K concentrations reduce the size of the Asn response; repolarizing the cell by current injection does not reverse the inhibitory effect of external K ions. Hyperpolarizing the membrane with a K-free Ringer solution increases the amplitude of the Asn response. In all these cases a decrease in delta Emax accounts for the apparent voltage sensitivity of the carrier mechanism. When induced by alterations of [K]o, an additional change in Km is observed, suggesting a K/Na-competitive inhibition of the Asn carrier. The results are discussed in terms of the amino acid carrier and passive membrane properties. It is suggested that the outward K-electrochemical gradient contributes an additional source of energy to the Na-dependent Asn uptake.
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机译:使用电流钳技术分析了非洲爪蟾胚胎内胚层细胞中天冬酰胺(Asn)诱导的去极化的动力学和电压依赖性。假定去极化反应反映了氨基酸膜载体的活化。它伴随着膜电阻的轻微增加,不能仅用Asn载体的电学特性来解释。提出Asn去极化至少部分是由于与Na偶联的氨基酸摄取间接相关的渗透率PK / PNa的降低引起的。在室温(20-23摄氏度)下,Asn反应根据单个指数函数发展,其时间常数与去极化的最终水平相关。去极化的幅度和上升时间均对膜电位的变化以及Asn或Na外部浓度的变化敏感。降低温度会降低Asn去极化的幅度,并增加Q10因子为2的上升时间。动力学仍然是Michaelis-Menten类型的,其Emax最大值明显降低,Km不变。当通过去极化和超极化电流改变保持电位时,Asn响应会根据钟形特征而变化,该钟形特征在正常静息水平附近表现出最佳状态。 Na / K-泵抑制剂或高外部K浓度引起的膜去极化减少了Asn反应的大小;通过电流注入使细胞复极化不会逆转外部K离子的抑制作用。用无K的林格溶液对膜进行超极化可增加Asn响应的幅度。在所有这些情况下,ΔEmax的减小说明了载体机构的表观电压敏感性。当由[K] o的变化诱导时,观察到Km的其他变化,表明对Asn载体的K / Na竞争性抑制。根据氨基酸载体和被动膜性质讨论了结果。建议向外的K电化学梯度为依赖于Na的Asn吸收贡献额外的能量来源。
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