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用[1,2 - 13C2]葡萄糖对戊糖循环非氧化途径的质量同位素异构体研究。

Mass isotopomer study of the nonoxidative pathways of the pentose cycle with [1,2-13C2]glucose.

作者信息

Lee W N, Boros L G, Puigjaner J, Bassilian S, Lim S, Cascante M

机构信息

Department of Pediatrics, Harbor-University of California Los Angeles Medical Center, Torrance 90502, USA.

出版信息

Am J Physiol. 1998 May;274(5):E843-51. doi: 10.1152/ajpendo.1998.274.5.E843.

Abstract

We present a single-tracer method for the study of the pentose phosphate pathway (PPP) using [1,2-13C2]glucose and mass isotopomer analysis. The metabolism of [1,2-13C2]glucose by the glucose-6-phosphate dehydrogenase, transketolase (TK), and transaldolase (TA) reactions results in unique pentose and lactate isotopomers with either one or two 13C substitutions. The distribution of these isotopomers was used to estimate parameters of the PPP using the model of Katz and Rognstad (J. Katz and R. Rognstad. Biochemistry 6: 2227-2247, 1967). Mass and position isotopomers of ribose, and lactate and palmitate (products from triose phosphate) from human hepatoma cells (Hep G2) incubated with 30% enriched [1,2-13C2]glucose were determined using gas chromatography-mass spectrometry. After 24-72 h incubation, 1.9% of lactate molecules in the medium contained one 13C substitution (m1) and 10% contained two 13C substitutions (m2). A similar m1-to-m2 ratio was found in palmitate as expected. Pentose cycle (PC) activity determined from incubation with [1,2-13C2]glucose was 5.73 +/- 0.52% of the glucose flux, which was identical to the value of PC (5.55 +/- 0.73%) determined by separate incubations with [1-13C] and [6-13C]glucose, 13C was found to be distributed in four ribose isotopomers ([1-13C]-, [5-13C]-, [1,2-13C2]-, and [4,5-13C2]ribose). The observed ribose isotopomer distribution was best matched with that provided from simulation by substituting 0.032 for TK and 0.85 for TA activity relative to glucose uptake into the model of Katz and Rognstad. The use of [1,2-13C2]glucose not only permits the determination of PC but also allows estimation of relative rates through the TK and TA reactions.

摘要

我们提出了一种使用[1,2 - 13C2]葡萄糖和质量同位素异构体分析来研究磷酸戊糖途径(PPP)的单示踪剂方法。[1,2 - 13C2]葡萄糖通过葡萄糖 - 6 - 磷酸脱氢酶、转酮醇酶(TK)和转醛醇酶(TA)反应进行代谢,产生具有一个或两个13C取代的独特戊糖和乳酸同位素异构体。利用Katz和Rognstad的模型(J. Katz和R. Rognstad. Biochemistry 6: 2227 - 2247, 1967),这些同位素异构体的分布被用于估计PPP的参数。使用气相色谱 - 质谱法测定了用30%富集的[1,2 - 13C2]葡萄糖培养的人肝癌细胞(Hep G2)中核糖、乳酸和棕榈酸(磷酸丙糖的产物)的质量和位置同位素异构体。孵育24 - 72小时后,培养基中1.9%的乳酸分子含有一个13C取代(m1),10%含有两个13C取代(m2)。正如预期的那样,在棕榈酸中也发现了类似的m1与m2的比例。由[1,2 - 13C2]葡萄糖孵育测定的戊糖循环(PC)活性为葡萄糖通量的5.73±0.52%,这与用[1 - 13C]和[6 - 13C]葡萄糖单独孵育测定的PC值(5.55±0.73%)相同。发现13C分布在四种核糖同位素异构体([1 - 13C] - 、[5 - 13C] - 、[1,2 - 13C2] - 和[4,5 - 13C2]核糖)中。相对于葡萄糖摄取,将TK活性设为0.032,TA活性设为0.85代入Katz和Rognstad模型进行模拟,观察到的核糖同位素异构体分布与模拟结果最匹配。使用[1,2 - 13C2]葡萄糖不仅可以测定PC,还可以估计通过TK和TA反应的相对速率。

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