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估计非胰岛素依赖型糖尿病中的糖异生率。

Estimating gluconeogenic rates in NIDDM.

作者信息

Landau B R

机构信息

Department of Medicine, School of Medicine, Case Western Reserve University, Cleveland, OH 44106.

出版信息

Adv Exp Med Biol. 1993;334:209-20. doi: 10.1007/978-1-4615-2910-1_15.

DOI:10.1007/978-1-4615-2910-1_15
PMID:8249684
Abstract

To measure the rate of gluconeogenesis in humans directly, one must administer and determine the specific activity or the enrichment in an intermediate in the gluconeogenic process and in the glucose formed, thus obtaining the fraction of the glucose formed by gluconeogenesis. By a separate determination of the rate of hepatic glucose production, the rate of gluconeogenesis can then be calculated. The closer the intermediate is to glucose-6-P, the more complete will be the measurement of the rate. Thus, if the intermediate is below the level of the triose phosphates, gluconeogenesis from glycerol will not be included in the estimate. Estimates of rates of gluconeogenesis from estimates of PEP enrichment or specific activity require a measure of the extent of exchange of label at the level of oxaloacetate. By using 14C or 13C labeled CO2 as the intermediate and estimating the relative rates of the reactions of the tricarboxylic acid cycle relative to gluconeogenesis from the distribution of 14C from [3-14]lactate in glutamine from the glutamine conjugate of phenylacetate, the enrichment or specific activity of PEP has been estimated. Correction must be made for the incorporation into the glutamine of 14CO2 formed from the [3-14C]lactate. Data support the validity of this approach toward estimating gluconeogenesis in NIDDM, but the approach is complex, time consuming and with uncertainties. Estimates that have been made using [2-14C] acetate are invalid because of the extensive metabolism of [2-14C]acetate in other than liver. Other approaches have promise, but technical problems may exist in their use and other problems, such as hepatic zonation and exchange reactions, may compromise their application.

摘要

要直接测定人体中糖异生的速率,必须给予并测定糖异生过程中间产物以及生成的葡萄糖中的比活度或富集度,从而得出由糖异生生成的葡萄糖所占的比例。通过单独测定肝脏葡萄糖生成速率,进而可以计算糖异生速率。中间产物越接近6-磷酸葡萄糖,对速率的测定就越完整。因此,如果中间产物低于磷酸丙糖水平,甘油生成糖异生的过程将不包括在估算范围内。根据磷酸烯醇式丙酮酸(PEP)的富集度或比活度估算糖异生速率,需要测量草酰乙酸水平的标记物交换程度。通过使用14C或13C标记的二氧化碳作为中间产物,并根据[3-14C]乳酸中14C在苯乙酸谷氨酰胺共轭物谷氨酰胺中的分布,估算三羧酸循环反应相对于糖异生的相对速率,从而估算出PEP的富集度或比活度。必须对[3-14C]乳酸生成的14CO2掺入谷氨酰胺的情况进行校正。数据支持这种估算2型糖尿病患者糖异生的方法的有效性,但该方法复杂、耗时且存在不确定性。使用[2-14C]乙酸进行的估算无效,因为[2-14C]乙酸在肝脏以外有广泛的代谢。其他方法有前景,但在使用中可能存在技术问题,并且其他问题,如肝小叶分区和交换反应,可能会影响其应用。

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Contributions of gluconeogenesis to glucose production in the fasted state.禁食状态下糖异生对葡萄糖生成的贡献。
J Clin Invest. 1996 Jul 15;98(2):378-85. doi: 10.1172/JCI118803.
3
Use of 2H2O for estimating rates of gluconeogenesis. Application to the fasted state.使用重水(2H2O)估算糖异生速率。应用于禁食状态。
J Clin Invest. 1995 Jan;95(1):172-8. doi: 10.1172/JCI117635.
4
Estimates of Krebs cycle activity and contributions of gluconeogenesis to hepatic glucose production in fasting healthy subjects and IDDM patients.禁食健康受试者和胰岛素依赖型糖尿病患者中三羧酸循环活性的估计以及糖异生对肝脏葡萄糖生成的贡献。
Diabetologia. 1995 Jul;38(7):831-8. doi: 10.1007/s001250050360.