[An enzymatic method for the isolation of tubules and cells from human kidney cortex].

H Bojar, K Balzer, F Boeminghaus, W Staib
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Abstract

The isolation of tubules and cells from human kidney cortex was realized by an enzymatic method. Tubules and cells were released from slices of kidney cortex by collagenase. The yield amounted to 80 % of the wet weight of incubated cortex slices. Thus numerous experiments with isolated tubules from one organ could be performed. Glucose production from different substrates was measured in order to test the biochemical integrity of the isolated cells. The highest rates of glucose formation were obtained with fructose as precursor. Glucose production was higher from lactate than from pyruvate. With proline and glutamine as substrates only small amounts of glucose were produced. Glucose formation from 10 mmol/1 pyruvate was linear with time up to 80 minutes. Ado-3':5'-P stimulated glucose formation at 10 mumolar concentration and inhibited gluconeogenesis at 1 mmolar, 0.1 mmolar and 1 mumolar concentrations.

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[从人肾皮质中分离小管和细胞的酶法]。
采用酶法分离人肾皮质小管和细胞。在胶原酶作用下,肾皮质切片释放小管和细胞。产率为培养的皮质片湿重的80%。因此,从一个器官中分离的小管可以进行许多实验。测量了不同底物的葡萄糖产量,以测试分离细胞的生化完整性。以果糖为前体的葡萄糖生成率最高。乳酸的葡萄糖产量高于丙酮酸。以脯氨酸和谷氨酰胺为底物,只产生少量葡萄糖。10 mmol/1丙酮酸的葡萄糖生成与时间呈线性关系,时间最长可达80分钟。Ado-3':5'-P在10摩尔浓度下刺激葡萄糖形成,在1、0.1和1摩尔浓度下抑制糖异生。
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