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大鼠肝脏中糖原合成与葡萄糖合成的区域化,但糖酵解不存在区域化。

Zonation of glycogen and glucose syntheses, but not glycolysis, in rat liver.

作者信息

Chen K S, Katz J

机构信息

Cedars-Sinai Medical Center, Los Angeles, CA 90048.

出版信息

Biochem J. 1988 Oct 1;255(1):99-104. doi: 10.1042/bj2550099.

Abstract

We have investigated the cause of defective glycogen synthesis in hepatocyte preparations enriched with cells from the periportal or perivenous zones obtained by the methods of Lindros & Penttila [Biochem. J. (1985) 228, 757-760] and of Quistorff [Biochem. J. (1985) 229, 221-226]. A modified procedure which yields hepatocytes capable of consistent rates of glycogen synthesis is described, and the rates of glucose and glycogen syntheses and of glycolysis in hepatocytes from the two zones are compared. Glycogen synthesis in cells was greatly impaired by very low concentrations (0.01-0.05 mg/ml) of digitonin, which had little effect on glucose and protein syntheses and Trypan Blue exclusion. Cells exposed to such low concentrations of digitonin lose all their synthetic capacity and ability to exclude Trypan Blue when incubated with EGTA, which does not affect cells not exposed to digitonin. With a modified procedure based on this phenomenon, our study reveals that hepatocyte preparations enriched with cells from the periportal zone synthesized glucose from lactate and alanine at rates twice those by cells from the perivenous zone, whereas the rate of glycogen synthesis from C3 precursors in periportal cells was 4 times that in the perivenous preparations. With substrates entering the pathway at the triose phosphate level, gluconeogenesis in periportal-cell preparations was 20% higher, and glycogen synthesis was twice that in perivenous preparations. Glycolysis was studied by the formation of 3HOH from [2-3H]glucose, the yield of lactate, and the conversion of [14C]glucose into [14C]lactate. In cell preparations from both zones glycolysis by all criteria was negligible at 10 mM-glucose, but was substantial at higher concentrations. However, there was no difference between the zones. We confirm that the capacities for glucose and glycogen syntheses in periportal cells are higher than in perivenous cells, but that at physiological glucose concentrations there is negligible glycolysis in liver parenchyma in both zones. The metabolic pattern in the perivenous cells is not glycolytic.

摘要

我们研究了通过Lindros和Penttila [《生物化学杂志》(1985年)228卷,757 - 760页]以及Quistorff [《生物化学杂志》(1985年)229卷,221 - 226页]的方法获得的富含门静脉周围或肝静脉周围区域细胞的肝细胞制剂中糖原合成缺陷的原因。描述了一种改进的方法,该方法可产生能够保持一致糖原合成速率的肝细胞,并比较了来自这两个区域的肝细胞中葡萄糖和糖原的合成速率以及糖酵解速率。细胞中的糖原合成受到极低浓度(0.01 - 0.05 mg/ml)的洋地黄皂苷的极大损害,而洋地黄皂苷对葡萄糖和蛋白质合成以及台盼蓝排斥几乎没有影响。当与乙二醇双四乙酸(EGTA)一起孵育时,暴露于这种低浓度洋地黄皂苷的细胞会丧失所有合成能力和排斥台盼蓝的能力,而EGTA对未暴露于洋地黄皂苷的细胞没有影响。基于这一现象采用改进的方法,我们的研究表明,富含门静脉周围区域细胞的肝细胞制剂从乳酸和丙氨酸合成葡萄糖的速率是富含肝静脉周围区域细胞制剂的两倍,而门静脉周围细胞中由C3前体合成糖原的速率是肝静脉周围制剂中的4倍。对于在磷酸丙糖水平进入途径的底物,门静脉周围细胞制剂中的糖异生作用高20%,糖原合成是肝静脉周围制剂中的两倍。通过[2 - 3H]葡萄糖形成3 - HOH、乳酸产量以及[14C]葡萄糖转化为[14C]乳酸来研究糖酵解。在来自两个区域的细胞制剂中,在10 mM葡萄糖浓度下,所有标准下的糖酵解都可忽略不计,但在较高浓度下则很显著。然而,两个区域之间没有差异。我们证实门静脉周围细胞中葡萄糖和糖原的合成能力高于肝静脉周围细胞,但在生理葡萄糖浓度下,两个区域的肝实质中糖酵解都可忽略不计。肝静脉周围细胞的代谢模式不是糖酵解型的。

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