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The Journal of Neuroscience, July 2, 2003, 23(13):5928-5935
Previous Article | Next Article
Energy Contribution of Octanoate to Intact Rat Brain Metabolism Measured by 13C Nuclear Magnetic Resonance Spectroscopy
Douglas Ebert,1 Ronald G. Haller,1,2,3 andMarlei E. Walton1 1Veterans Affairs North Texas Health Care System, Dallas, Texas 75216, 2Department of Neurology, University of Texas Southwestern Medical Center, Dallas, Texas 75235, and 3Institute for Exercise and Environmental Medicine, Presbyterian Hospital of Dallas, Dallas, Texas 75231
Abstract
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Abstract
Introduction
Glucose is the dominant oxidative fuel for brain, but studies have indicated that fatty acids are used by brain as well. We postulated that fatty acid oxidation in brain could contribute significantly to overall energy usage and account for non-glucose-derived energy production. [2,4,6,8-13C4]octanoate oxidation in intact rats was determined by nuclear magnetic resonance spectroscopy. We found that oxidation of 13C-octanoate in brain is avid and contributes20% to total brain oxidative energy production. Labeling patterns of glutamate and glutamine were distinct, and analysis of these metabolites indicated compartmentalized oxidation of octanoate in brain. Examination of liver and blood spectra revealed that label from 13C-octanoate was incorporated into glucose and ketones, which enabled calculation of its overall energy contribution to brain metabolism: glucose (predominantly unlabeled) and 13C-labeled octanoate can account for the entire oxidative metabolism of brain. Additionally, flux through anaplerotic pathways relative to tricarboxylic acid cycle flux (Y) was calculated to be 0.08 ± 0.039 in brain, indicating that anaplerotic flux is significant and should be considered when assessing brain metabolism. Y was associated with the glutamine synthesis compartment, consistent with the view that anaplerotic flux occurs primarily in astrocytes.
Key words: metabolism; brain; glutamate; glutamine; glucose; NMR; 13C spectroscopy
Introduction
Glucose is well established as the major oxidative fuel for brain (Sokoloff et al., 1977), but cell culture (Edmond et al., 1987
We hypothesized that fatty acid oxidation in brain could contribute significantly to overall energy usage. Previous studies of fat oxidation in brain have been limited to acetate, the simplest of fats (Badar-Goffer et al., 1990
Materials and Methods
Animal preparation and experimental design. All experimental procedures were approved by the Institutional Animal Care and Use Committee at the Veterans Affairs North Texas Health Care System (VANTHCS). Adult male Sprague Dawley rats (329.1 ± 10.6 gm; Charles River, Kingston, MA) were housed in the VANTHCS Animal Resources Center with a 12 hr light/dark cycle and had ad libitum access to water and lab chow.Rats were weighed and anesthetized with an intraperitoneal injection of 1–3 ml/kg ketamine/xylazine mixture (6 mg/ml xylazine, 94 mg/ml ketamine). After a tracheotomy was performed, 1–2.5% isoflurane (Isotec 3 vaporizer, Matrix Medical, Buffalo, NY) in 100% O2 was used to maintain anesthesia and delivered via a positive-pressure ventilator (model 683 Small Animal Ventilator, Harvard Apparatus, South Natick, MA) at a rate of 1.25 cc/min,
At time 0 (after
Tissue preparation. Whole brain and liver were extracted by homogenization in ice-cold 3.6% perchloric acid (PCA) with a motor-driven tissue grinder (model 985–370, Biospec Products, Bartlesville, OK). Brain and liver homogenates and PCA-extracted blood samples were then centrifuged, neutralized, and lyophilized overnight in a rotary evaporator (SpeedVac, Savant Instruments, Farmingdale, NY; Flexi-Dry microprocessor lyophilizer, FTS Systems, Stone Ridge, NY). Lyophilates were brought to a volume of 550 µl in deuterium oxide (Cambridge Isotope Laboratories).
Metabolite concentration. Aliquots (150 µl) of arterial blood taken from the carotid artery were obtained before octanoate infusion and at the end of the experiment. Plasma was analyzed using gas chromatography–mass spectrometry to determine enrichment and concentration of octanoate at these time points (Powers et al., 1995
-hydroxybutyrate) were measured fluorometrically (Maughan, 1982
Nuclear magnetic resonance spectroscopy. Proton-decoupled 13C and solvent-suppressed 1H nuclear magnetic resonance (NMR) spectra of the tissue extracts were collected at 37°Cona Varian INOVA 600 MHz spectrometer (Varian, Palo Alto, CA) in a 5 mm broadband probe. 13C NMR spectra were obtained using a 30 K sweep width, 45° pulse, 1.5 sec pulse delay, and bilevel proton decoupling. To achieve adequate signal to noise, the number of scans acquired was typically 4000 for brain and 1000 for liver and blood. Solvent-suppressed 1H spectra were collected with a pulse width of 9.2 µsec, 10 sec pulse delay, and 32 scans per sample. Free induction decays were baseline corrected and multiplied by an exponential function before Fourier transformation; 0.5 Hz line broadening was used for all extracts. Areas and intensities of 13C and 1H spectra were quantitated by a curve-fitting program (NUTS, Acorn Inc.). Line fit was considered adequate if difference spectra were indistinguishable from spectral regions with no visible peaks. For 13C glutamate and glutamine regions, each multiplet area was normalized and reported as a fraction of the total area for that specific carbon resonance.
Data analysis. Acetyl-CoA fractional enrichments were determined by non-steady-state and steady-state isotopomer analysis (Malloy et al., 1987
Isotopic steady state was determined by comparing (1) spectral versus steady-state-calculated peak areas and (2) fractional enrichment values using non-steady-state (Malloy et al., 1990
0.01.
Results
Incorporation of [2,4,6,8-13C4]octanoate in brainA representative 13C spectrum of the extract of whole brain from rats infused with [2,4,6,8-13C4]octanoate for 105 min is shown in Figure 1. The inset shows resonance regions from all five glutamate (E) and glutamine (Q) carbons 1–5 (C1–C5) and GABA carbons C2–C4 (Fig. 1). 13C-labeled octanoate is avidly metabolized by brain, resulting in multiple peaks (multiplets) in each of these resonance areas.
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Figure 1. 13C spectrum of representative extract of intact rat brain infused with [2,4,6,8-13C4]octanoate for 105 min. Glutamate (E) and glutamine (Q) regions of carbons 1–5 (C1–C5) and GABA (Gb) C2–C4 are shown. Multiplets are depicted as follows: singlet (S), doublet (D), and triplet (T). Doublets resulting from carbon–carbon coupling of adjacent carbons are noted [e.g., C3 and C4 (D34) in C4 region].Inset,Full13C spectrum; regions of E, Q, Gb, and lactate (La) carbon resonances are indicated. PPM, Parts per million.
Incorporation of 13C-labeled octanoate in brain results in different labeling patterns between corresponding glutamate and GABA versus glutamine carbons (Fig. 1). The labeling pattern of GABA most closely resembles that of glutamate, as evidenced by a much higher singlet to doublet ratio in GABA and glutamate C3 as compared with glutamine C3 (Fig. 1). In the glutamine C4 region, there is a conspicuous lack of a doublet arising from C4–C5 carbon–carbon coupling (D45) that is clearly present in the glutamate C4 and GABA C2 resonances (Fig. 1). In fact, in both C4 and C5 of glutamate, D45 is readily apparent (Fig. 1).
Glutamate and glutamine isotopomer analysis in brain
Relative peak areas and ratios from glutamate and glutamine resonances are used in steady-state and non-steady-state calculations of fractional contributions to acetyl-CoA in brain. No differences were found in spectral data compared with calculated steady-state values for either glutamate or glutamine. Additionally, non-steady-state analysis was used as a tool to determine whether steady state had been achieved in these experiments. Fc2 values from non-steady-state versus steady-state analysis were not different for either glutamate or glutamine (Table 1). These data indicate that glutamate and glutamine isotopic steady state (ISS) had been reached by 105 min.
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Table 1. Glutamate and glutamine isotopomer analysis
Glutamate steady-state Fc2 values (Table 1) indicated significant oxidation of medium-chain fatty acid by brain TCA cycle. Twenty-three percent of acetyl-CoA in brain was enriched by infusion with [2,4,6,8-13C4]octanoate. Glutamine steady-state isotopomer analysis (Table 1) yielded a higher Fc2 value of 56%. Values for both glutamate and glutamine represent substantial oxidation of fatty acid within brain tissue, and disparate distribution of octanoate-derived label among TCA cycle ancillary reactions indicates a compartmentation of octanoate metabolism within brain.
Because ISS was achieved in these experiments, it was possible to calculate flux through anaplerotic pathways relative to TCA cycle flux (Y) in the brain (Table 1). Y is higher in glutamine versus glutamate isotopomer analysis (Table 1), indicating that most of the anaplerotic flux in brain is occurring in the TCA cycle associated with glutamine production. The percentage of glutamate and glutamine metabolite pools generated through anaplerotic pathways can be calculated using the equation Y/(Y + 1) when the TCA cycle flux is set to 1 (Malloy et al., 1988
Contribution of 13C-labeled glucose to brain metabolism
[2,4,6,8-13C4]octanoate administered in these experiments can only provide acetyl-CoA units labeled in carbon 2 (Fc2) (Fig. 2). Glutamate molecules labeled in both the 4 and 5 positions can only arise from a substrate that provides doubly labeled acetyl-CoA (Fc12) (Fig. 2). Thus exogenously administered 13C-labeled octanoate must have been metabolized elsewhere in the animal, and 13C label redistributed into a substrate that would be available for oxidation in brain. We therefore investigated glucose labeling via gluconeogenesis, as well as the possibility of label arising from ketogenesis.
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Figure 2. 13C isotope isomer (isotopomer) analysis is based on the appearance of 13C label ( ) in the carbons of glutamate originating from labeled acetyl-CoA. Glutamate is in rapid exchange with the TCA cycle intermediate,
-ketoglutarate (
Octanoate, glucose, and ketones were measured from arterial blood samples taken before octanoate infusion began and at the end of the experiment. Glucose concentration was not different between these two time points (11.4 ± 1.7 mM initial; 11.1 ± 2.7 mM final). Initial ketone levels (acetoacetate plus
Liver extracts were examined using 13C magnetic resonance spectroscopy. Glutamate steady-state analysis of livers from animals infused for 105 min revealed that the fractional contribution of [2,4,6,8-13C4]octanoate to acetyl-CoA was 40% and Y was 37%. To evaluate glucose and ketone 13C labeling, 1H spectra were analyzed to obtain the fractional 13C enrichment of glucose and
To verify that Fc1 and Fc12 in brain (Table 1) were caused by labeled glucose arising from gluconeogenesis, correlating carbons were compared. Glucose C1 enrichment ratios from liver and resultant lactate C3 enrichment ratios in brain were measured and compared with brain acetyl-CoA isotopomers labeled in carbon 1 only and labeled in both carbons 1 and 2 (i.e., the fractional contributions that could not have arisen from 13C-labeled octanoate).
Both
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Figure 3. 13C spectral regions of glucose carbon 1 (C1)
Similarly, from steady-state glutamate analysis in brain (Table 1), the ratio of doubly labeled (Fc12) and carbon 1-labeled (Fc1 + Fc12) acetyl-CoA pool could be compared with those ratios in the correlating C1 resonance of glucose and C3 resonance of lactate (Fig. 3). Fc12/(Fc1 + Fc12) is not different from D12/(S + D12) for either anomer of glucose in liver, nor is it different from the lactate D23/(S + D23) ratio in brain (Fig. 3).
Fc1 and Fc12 agree well with a contribution of glucose from liver gluconeogenesis to energy metabolism in brain. However, Fc2 is proportionately much larger because of avid oxidation of octanoate in brain. Assuming randomization of label at succinate and fumarate, labeled glucose produced in these experiments will give rise to approximately equal amounts of singly enriched glucose molecules in C1, C2, C5, and C6. Therefore, Fc2 arising from glucose C1 and C6 will be approximately equal to Fc1 arising from glucose C2 and C5. Subtracting the Fc2 contribution from glucose (0.030) from the total Fc2 (0.227) (Table 1) leaves an Fc2 of
N-acetyl aspartate enrichment
Brain 1H spectra were analyzed to determine 13C fractional enrichment of N-acetyl aspartate (NAA). NAA C6 (corresponding to the methyl carbon of acetyl-CoA) enrichment was 8.5 ± 3.4%. This is not different from fractional enrichment of lactate C3 (4.0%) or of acetyl-CoA C2 (arising from glucose) in brain (Fc2 + Fc12 = 3.9 ± 2.5%) and is consistent with the contribution of enriched 13C-glucose to neuronal acetyl-CoA.
Model of brain metabolism
To verify isotopic distribution of glucose, we constructed a substrate oxidation model based on our data and TCAsim software. With metabolic information about liver in these experiments, it is possible to predict the distribution of the 64 different glucose isotopomers generated via gluconeogenesis using TCAsim (Fig. 4A, columns 1, 2). Isotopomer analysis clearly showed a high level of enrichment from a labeled substrate that enriched acetyl-CoA at carbon 2 (Table 1), consistent with [2,4,6,8- 13C4]octanoate that was administered. On the basis of the measured Fc2 (0.227) and glucose contribution to Fc2 (0.030), octanoate contribution was calculated to be 20% (Table 1). Because it is well established that glucose is the major oxidative fuel in brain and 20% of metabolism had already been accounted for, 80% of oxidative metabolism was ascribed to glucose (Fig. 4A, column 3). The contribution of glucose isotopomers to acetyl-CoA in brain (Fc1, Fc2, Fc12, and Fc0) was calculated by adding all of these isotopomers (Fig. 4A, columns Fc1–Fc0). This allows direct comparison of model values with experimental fractional contributions obtained via glutamate isotopomer analysis (Fig. 4B, Table 1); they are in precise agreement.
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Figure 4. A, Glucose isotopomers and resultant fractional isotopomer contribution to the glucose pool (FC) as generated from TCAsim software using liver data from rats infused with [2,4,6,8-13C4]octanoate for 105 min. Brain energy metabolism was modeled using an 80% glucose contribution (80% of FC) giving rise to acetyl-CoA populations as shown (Fc1, Fc2, Fc12, and Fc0). B, By combining 80% glucose contribution with 20% from exogenous [2,4,6,8-13C4]octanoate, 100% of brain energy metabolism is accounted for (not different from steady-state analysis values in Table 1; p
Discussion
These data demonstrate that a medium-chain fatty acid (octanoate) can directly contributeAlthough glucose is the major oxidative fuel for brain, fatty acids are used as well (Edmond et al., 1987
As demonstrated previously using labeled glucose (Badar-Goffer et al., 1990
Isotopomer analysis can be performed on any metabolite in exchange with the TCA cycle. We expected that glutamate isotopomer analysis would provide information about brain metabolism as a whole because it reflects a combination of all TCA cycles in the brain in exchange with a pool of glutamate. The most likely sources of glutamate labeling in our experiments arise from (1) octanoate oxidation in astrocytes contributing to the small astrocytic pool of glutamate, (2) octanoate oxidation in astrocytes resulting in labeled glutamine, subsequently exported to neurons and converted to glutamate by the action of the neurotransmitter cycle, which contributes to the large neuronal glutamate pool, and (3) oxidation of labeled glucose contributing primarily to the large neuronal glutamate pool. Glutamine isotopomer analysis, on the other hand, gives information primarily regarding the astrocytic TCA cycle, because glutamine synthetase is an astrocyte-specific enzyme (Norenberg and Martinez-Hernandez, 1979
It was expected that octanoate metabolism would take place exclusively in the astrocytes (Edmond et al., 1987
NAA was also examined to further investigate compartmentation of brain metabolism. This modified amino acid is a well established neuronal marker (Simmons et al., 1991
The overall brain relative anaplerotic flux value reported here (Table 1) is in excellent agreement with previously reported estimations of anaplerotic flux (10%) (Cheng et al., 1967
Although the rate of neurotransmitter cycling has been calculated previously (Lebon et al., 2002
Oxidative entry of doubly labeled acetyl-CoA (Fc12) was clearly demonstrated in brain spectra. Because labeled fatty acid oxidized by astrocytes rapidly gives rise to label in glutamine (Badar-Goffer et al., 1990
It is conceivable that a contribution to Fc2 may have been caused by ketones from liver ketogenesis, which would preserve the labeling paradigm of [2,4,6,8-13C4]octanoate. Several points dispute significant oxidation of ketones by brain under these conditions. First, concentration of ketones at the end of the experiment was 357.4 ± 97.8 µM. Although this represents a 2.7-fold increase over the endogenous concentration, 13C enrichment of ketones was only 22.6 ± 8.1%; the remaining 77% unlabeled ketones would contribute to Fc0 when metabolized, for which there is not much latitude in the data. Additionally, oxidation of octanoate and glucose can account for the entire oxidative metabolism of brain (Fig. 4). If the 80% glucose/20% octanoate metabolic model is shifted to either side of this 80:20 ratio by even 4%, modeled fractional enrichment of acetyl-CoA in brain becomes significantly different from our experimental data (Table 1). Thus, there is very little margin in the data or in the model for additional sources of unlabeled (or partially labeled) oxidizable substrates. Second, ketones are not a primary fuel for brain in fed animals. Hawkins et al. (1971
A recent study that used labeled acetate in human subjects estimated that 14% of brain oxygen consumption was caused by astroglial TCA cycle flux (Lebon et al., 2002
In summary, results reported here provide evidence that fatty acid metabolic pathways are active in brain and that octanoate can contribute 20% of oxidative metabolism in brain in an intact, physiological system. Taken together, these data are consistent with octanoate oxidation and substantial anaplerotic flux in astrocytes and with oxidation of glucose primarily occurring in neurons. The data fit well with a simple model in which the combination of octanoate and glucose can account for all of brain energy metabolism.
Footnotes
Received Oct. 10, 2002; revised Mar. 4, 2003; accepted Apr. 18, 2003.This study was supported by Veterans Affairs Merit Grant 98-139 and Veterans Integrated Service Network17 Grant 99-89. We thank Drs. Mark Jeffrey and Craig Malloy for constructive conversations regarding this work and gratefully acknowledge the laboratory of Dr. Henri Brunengraber for measurement of octanoate concentrations and enrichments.
Correspondence should be addressed to Douglas Ebert, Veterans Affairs North Texas Health Care System, 4500 South Lancaster Road (151), Dallas, TX 75216. E-mail: mwde{at}swbell.net.
Copyright © 2003 Society for Neuroscience 0270-6474/03/235928-08$15.00/0
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