Abstract

Glucose isotopomer analysis following addition of [U-13C]propionate yields relative 13C fluxes through anaplerosis, gluconeogenesis and the substrate cycle in perfused livers. We found that anaplerotic inflow was about 4 times the flux through citrate synthase, with a significant fraction (about 40%) being diverted into the substrate cycle leaving a net gluconeogenic output of about 2.4. In fasted rats, gluconeogenesis is equal to hepatic glucose output since there is no contribution from glycogenolysis. In perfused livers obtained from fasted rats, absolute gluconeogenic output can be easily estimated from direct measurements of glucose secretion into the perfusion fluid, allowing absolute flux measurements for the other pathways, including the substrate cycle, to be measured. However, measurement of hepatic glucose output in vivo requires a separate tracer measurement of glucose turnover. We're utiliziing the irreversible tracer, [1,6-13C2]glucose to measure glucoes turnover. There is no significant production of [1,6-13C2]glucose expected from hepatic metabolism of [U-13C]propionate, hence the labeling from [U-13C]propionate does not interfere with the glucose turnover measurement and the estimate (63mmol/min/kg) is consistent with published values. Correspondingly, there is no significant production of multiply-labeled glucose C2 isotopomers from the [1,6-13C2]glucose label, hence it does not interfere with the quantitation of the relative anaplerotic, gluconeogenic and substrate cycle fluxes from analysis of the glucose C2b multiplet ratios. The results indicate that of the 226 mmol/kg/min of anaplerotic units entering the oxaloacetate pool, about 55% entered the substrate + Cori cycles, with a gluconeogenic balance of about 125 mmol/kg/min of triose phosphate (63 mmol/kg/min of glucose). Given that the Cori cycle contributes only about 10-15% of the total carbon recycling between oxaloacetate and pyruvate it can be seen that there is substantial flux (~130-140 mmol/kg/min) through the substrate cycle in the fasted, anesthetized rat. (Service 10) REPORT PERIOD: (09/01/97-08/31/98)

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Center for Research Resources (NCRR)
Type
Biotechnology Resource Grants (P41)
Project #
2P41RR002584-11
Application #
6121202
Study Section
Project Start
1998-09-15
Project End
1999-08-14
Budget Start
1997-10-01
Budget End
1998-09-30
Support Year
11
Fiscal Year
1998
Total Cost
Indirect Cost

  Institution

Name
University of Texas Sw Medical Center Dallas
Department
Type
DUNS #
City
Dallas
State
TX
Country
United States
Zip Code
75390

  Publications

Chiu, Tsuicheng D; Arai, Tatsuya J; Campbell Iii, James et al. (2018) MR-CBCT image-guided system for radiotherapy of orthotopic rat prostate tumors. PLoS One 13:e0198065
Mishkovsky, Mor; Anderson, Brian; Karlsson, Magnus et al. (2017) Measuring glucose cerebral metabolism in the healthy mouse using hyperpolarized 13C magnetic resonance. Sci Rep 7:11719
Moreno, Karlos X; Harrison, Crystal E; Merritt, Matthew E et al. (2017) Hyperpolarized ?-[1-13 C]gluconolactone as a probe of the pentose phosphate pathway. NMR Biomed 30:
Funk, Alexander M; Anderson, Brian L; Wen, Xiaodong et al. (2017) The rate of lactate production from glucose in hearts is not altered by per-deuteration of glucose. J Magn Reson 284:86-93
Zhang, Liang; Habib, Amyn A; Zhao, Dawen (2016) Phosphatidylserine-targeted liposome for enhanced glioma-selective imaging. Oncotarget 7:38693-38706
Walker, Christopher M; Merritt, Matthew; Wang, Jian-Xiong et al. (2016) Use of a Multi-compartment Dynamic Single Enzyme Phantom for Studies of Hyperpolarized Magnetic Resonance Agents. J Vis Exp :e53607
Wu, Yunkou; Zhang, Shanrong; Soesbe, Todd C et al. (2016) pH imaging of mouse kidneys in vivo using a frequency-dependent paraCEST agent. Magn Reson Med 75:2432-41
Malloy, Craig R; Sherry, A Dean (2016) Biochemical Specificity in Human Cardiac Imaging by 13C Magnetic Resonance Imaging. Circ Res 119:1146-1148
Moss, Lacy R; Mulik, Rohit S; Van Treuren, Tim et al. (2016) Investigation into the distinct subcellular effects of docosahexaenoic acid loaded low-density lipoprotein nanoparticles in normal and malignant murine liver cells. Biochim Biophys Acta 1860:2363-2376
Bastiaansen, Jessica A M; Merritt, Matthew E; Comment, Arnaud (2016) Measuring changes in substrate utilization in the myocardium in response to fasting using hyperpolarized [1-(13)C]butyrate and [1-(13)C]pyruvate. Sci Rep 6:25573

Showing the most recent 10 out of 374 publications