胰岛素刺激小鼠远曲小管细胞对Mg2+的摄取。

L J Dai, G Ritchie, B W Bapty, D Kerstan, G A Quamme
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引用次数: 35

摘要

胰岛素已被证明是一种保护镁的激素,其作用部分是通过刺激粗升肢内的镁吸收。尽管远曲小管拥有最多的胰岛素受体,但目前尚不清楚胰岛素在远曲小管中有什么作用。用放射免疫法测定小鼠远曲小管(MDCT)细胞cAMP的形成,用荧光法测定Mg2+的摄取,研究胰岛素对永生化小鼠远曲小管(MDCT)细胞的影响。为了评估Mg2+的摄取情况,我们先将MDCT细胞在无Mg2+的培养基中培养16 h,将Mg(2+)耗尽至0.22 +/- 0.01 mM,然后将其置于1.5 mM的MgCl2中,用微荧光检测细胞内Mg2+浓度([Mg2+]i)的变化。[Mg2+]i恢复到基础水平0.53 +/- 0.02 mM,平均再灌注速率d([Mg2+]i)/dt为164 +/- 5 nM/s。胰岛素以浓度依赖的方式刺激Mg2+进入,最大反应为214 +/- 12 nM/s,比对照组的平均摄取速率增加了30 +/- 5%。这与胰岛素介导的cAMP生成增加2.5倍(52 +/- 3 pmol)有关。毫克的蛋白质(1)。5分钟(1))。染料木黄酮,一种酪氨酸激酶抑制剂,减少胰岛素刺激的Mg2+摄取(169 +/- 11 nM/s),但不改变胰岛素介导的cAMP形成(47 +/- 5 pmol)。毫克的蛋白质(1)。5分钟(1))。PTH刺激Mg2+进入,部分是通过增加cAMP的形成。胰岛素和甲状旁腺激素增加Mg2+的摄取在一个附加的方式。总之,胰岛素介导Mg2+的进入,部分是通过染料木黄酮敏感机制和调节激素响应运输。这些研究表明,胰岛素刺激MDCT细胞对Mg2+的摄取,并提示胰岛素与其他肽和类固醇激素协同作用,控制远曲小管中镁的保存。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Insulin stimulates Mg2+ uptake in mouse distal convoluted tubule cells.

Insulin has been shown to be a magnesium-conserving hormone acting, in part, through stimulation of magnesium absorption within the thick ascending limb. Although the distal convoluted tubule possesses the most insulin receptors, it is unclear what, if any, actions insulin has in the distal tubule. The effects of insulin were studied on immortalized mouse distal convoluted tubule (MDCT) cells by measuring cellular cAMP formation with radioimmunoassays and Mg2+ uptake with fluorescence techniques using mag-fura 2. To assess Mg2+ uptake, MDCT cells were first Mg(2+) depleted to 0.22 +/- 0.01 mM by culturing in Mg2+-free media for 16 h and then placed in 1.5 mM MgCl2, and the changes in intracellular Mg2+ concentration ([Mg2+]i) were measured with microfluorescence. [Mg2+]i returned to basal levels, 0.53 +/- 0.02 mM, with a mean refill rate, d([Mg2+]i)/dt, of 164 +/- 5 nM/s. Insulin stimulated Mg2+ entry in a concentration-dependent manner with maximal response of 214 +/- 12 nM/s, which represented a 30 +/- 5% increase in the mean uptake rate above control values. This was associated with a 2.5-fold increase in insulin-mediated cAMP generation (52 +/- 3 pmol. mg protein(-1). 5 min(-1)). Genistein, a tyrosine kinase inhibitor, diminished insulin-stimulated Mg2+ uptake (169 +/- 11 nM/s), but did not change insulin-mediated cAMP formation (47 +/- 5 pmol. mg protein(-1). 5 min(-1)). PTH stimulates Mg2+ entry, in part, through increases in cAMP formation. Insulin and PTH increase Mg2+ uptake in an additive fashion. In conclusion, insulin mediates Mg2+ entry, in part, by a genistein-sensitive mechanism and by modifying hormone-responsive transport. These studies demonstrate that insulin stimulates Mg2+ uptake in MDCT cells and suggest that insulin acts in concert with other peptide and steroid hormones to control magnesium conservation in the distal convoluted tubule.

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