Activation of Central Lactate Metabolism Lowers Glucose Production in Uncontrolled Diabetes and Diet-Induced Insulin Resistance

doi:10.2337/db07-1464

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Activation of Central Lactate Metabolism Lowers Glucose Production in Uncontrolled Diabetes and Diet-Induced Insulin Resistance

Madhu Chari¹^,2, Carol K.L. Lam¹^,2, Penny Y.T. Wang², and Tony K.T. Lam¹^,2^,3

¹ Department of Physiology, University of Toronto, Toronto, Ontario, Canada
² Toronto General Hospital Research Institute, University Health Network, Toronto, Ontario, Canada
³ Department of Medicine, University of Toronto, Toronto, Ontario, Canada

Address correspondence and reprint requests to Dr. Tony Lam, MaRS Centre, Toronto Medical Discovery Tower, Room 10-706, 101 College St., Toronto, Ontario M5G 1L7, Canada. E-mail: tony.lam{at}uhnres.utoronto.ca

Abbreviations: CNS, central nervous system; ICV, intracerebroventricular

ABSTRACT

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ABSTRACT
RESEARCH DESIGN AND METHODS
RESULTS AND DISCUSSION
REFERENCES

OBJECTIVE—Hypothalamic lactate metabolism lowers hepaticglucose production and plasma glucose levels in normal rodents.However, it remains unknown whether activation of hypothalamiclactate metabolism lowers glucose production and plasma glucoselevels in rodents with diabetes and obesity.

RESEARCH DESIGN AND METHODS—We performed intracerebroventricular(ICV) administration of lactate to enhance central lactate metabolismin 1) early-onset streptozotocin-induced uncontrolled diabeticrodents, 2) experimentally induced hypoinsulinemic normal rodents,and 3) early-onset diet-induced insulin-resistant rodents. Tracer-dilutionmethodology was used to assess the impact of ICV lactate onthe rate of glucose production in all three models.

RESULTS—We first report that in the absence of insulintreatment, ICV lactate administration lowered glucose productionand glucose levels in rodents with uncontrolled diabetes. Second,ICV lactate administration lowered glucose production and glucoselevels in normal rodents with experimentally induced hypoinsulinemia.Third, and finally, ICV lactate administration lowered glucoseproduction in normal rodents with diet-induced insulin resistance.

CONCLUSIONS—Central lactate metabolism lowered glucoseproduction in uncontrolled diabetic and normal rodents withhypoinsulinemia and in rodents with diet-induced insulin resistance.These data suggest that insulin signaling is not required forcentral lactate to lower glucose production and that the activationof hypothalamic lactate metabolism could consequently bypassinsulin resistance and lower glucose levels in early-onset diabetesand obesity.

Recent studies indicate that the hypothalamus detects a risein nutrients and hormones in order to regulate peripheral metabolicprocesses in normal rodents (1–9). Specifically, hypothalamicadministration of glucose and its subsequent conversion to lactatelowers glucose production and plasma glucose levels in the presenceof basal insulin levels (10). No studies to date, to our knowledge,have examined whether activation of hypothalamic lactate metabolismlowers glucose production and plasma glucose levels in modelswith diabetes or obesity. We hypothesized that hypothalamiclactate metabolism regulates glucose homeostasis independentof insulin signaling and could consequently bypass insulin resistanceto lower glucose production and glucose levels in diabetes andobesity.

Here, we first tested whether an enhancement of central lactatemetabolism regulates glucose homeostasis in uncontrolled diabeticrodents. Since uncontrolled diabetes is associated with metabolicdisturbances and hypoinsulinemia, we next alternatively andselectively evaluated whether central lactate metabolism regulatesglucose homeostasis in normal rodents with experimentally inducedhypoinsulinemia. Finally, we tested whether central lactatemetabolism bypasses insulin resistance to regulate glucose homeostasisin high-fat diet–induced insulin-resistant rodents. Thesestudies could reveal novel therapeutic targets in the hypothalamusto bypass insulin resistance and lower glucose levels in diabetesand obesity.

RESEARCH DESIGN AND METHODS

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ABSTRACT
RESEARCH DESIGN AND METHODS
RESULTS AND DISCUSSION
REFERENCES

We studied 8-week-old male Sprague-Dawley rats (Charles RiverLaboratories, Montreal, Canada). Rats were housed in individualcages and subjected to a standard light-dark cycle. We implanteda single catheter into the third cerebral ventricle, for intracerebroventricular(ICV) infusions, by stereotaxic surgery. After $~$ 1 week of recovery,additional catheters were placed in the internal jugular veinand carotid artery for infusion and sampling, respectively,during the eventual in vivo infusion procedure. Recovery fromsurgery was monitored by measuring daily food intake and bodyweight gain in days preceding the infusion procedure. All studyprotocols were reviewed and approved by the institutional animalcare and use committee of the Toronto General Hospital ResearchInstitute, University Health Network.

Early-onset uncontrolled diabetes model.
Uncontrolled diabetes was induced with a single injection ofstreptozotocin (STZ) (60 mg/kg i.v.; Sigma, St. Louis, MO),a potent diabetogenic agent that is cytolytic against pancreaticβ-cells, dissolved in sterile saline, at the end of thevascular surgery. The glycemic status of diabetic rats was monitoreddaily using a hand-held glucometer (Accu-Chek Compact Plus;Roche Diagnostics, Laval, Canada); only rats that were sufficientlyhyperglycemic (blood glucose >15 mmol/l) were included inthe diabetes studies. Fifty-four to sixty hours post-STZ injection,the in vivo ICV infusion experiments were carried out, and lasteda total of 3 h, in rats that were limited to 20 g of standardchow the previous night. We infused ICV vehicle (0.9% wt/volNaCl) or ICV 5 mmol/l L-lactate throughout the experiments.A primed-continuous infusion of [3-³H]glucose (40 µCibolus, 0.4 µCi/min thereafter; Perkin Elmer) was initiatedat 90 min and maintained throughout the study to assess glucosekinetics. Plasma samples were collected in the final 0.5 h (150–180min) for determination of [³H]glucose specific activity as wellas hormone levels.

Experimentally induced hypoinsulinemic model.
These in vivo infusion experiments lasted a total of 270 minand were carried out in normal rats that were limited to 20g of standard chow the previous night. A primed-continuous infusionof [3-³H]glucose (40 µCi bolus, 0.4 µCi/min thereafter;Perkin Elmer) was initiated at the start of the protocol alongwith somatostatin (1 µg · kg^–1 · min^–1;Sigma). An infusion of ICV saline or 5 mmol/l lactate was initiatedat 90 min and maintained until the end of the experiments (270min). Plasma glucose level was monitored every 10 min throughoutthe protocol. Plasma samples were collected throughout the protocolfor the determination of [³H]glucose specific activity as wellas hormone levels. This experimental approach decreased plasmainsulin levels by 50% in both ICV saline- or lactate-infusedrats. In ICV saline-infused rats, plasma glucose level was elevatedby 180–200 min, and this elevation was sustained untilthe end of the experiments. Thus, this is an acute model ofhypoinsulinemia/hyperglycemia that does not have long-term metabolicdisturbances, as seen in uncontrolled diabetes.

Early-onset, high-fat diet–induced, insulin-resistant model.
Animals were fed a high-fat (lard oil enriched) diet (catalogno. 9389; Purina Mills) that was generated by supplementingthe standard chow with 10% lard for 3 days. The caloric contentof the high-fat diet was 45% carbohydrate, 22% protein, and33% fat and 44, 24, and 6.19%, respectively, for the standardchow. The total calories provided by digestible nutrients was5.14 kcal/g for the high-fat diet versus 3.3 kcal/g for thestandard chow. The in vivo infusion experiments lasted a totalof 4.5 h. A primed-continuous infusion of [3-³H]glucose (40µCi bolus, 0.4 µCi/min thereafter; Perkin Elmer)was initiated at 0 min. We infused ICV vehicle (0.9% wt/volNaCl) or ICV 5 mmol/l L-lactate from time 90 min and onwarduntil 270 min. A basal pancreatic insulin clamp was performedin the final 2 h (150–270 min) of the study: a continuouscoinfusion of insulin (0.8 mU · kg^–1 · min^–1)and somatostatin (3 µg · kg^–1 · min^–1)was administered, and a variable infusion of 25% glucose solutionwas administered as needed to clamp and maintain the plasmaglucose concentration at levels similar to those of the basalstate. Plasma samples were collected in the final 0.5 h (240–270min) for determination of [³H]glucose specific activity as wellas hormone levels. Plasma insulin (Fig. 3C) and glucagon (Fig. 3D)levels were maintained at $~$ 0.9 ng/ml and $~$ 37 pg/ml, respectively.A separate set of hyperinsulinemic (insulin dosage: 3 mU ·kg^–1 · min^–1)-euglycemic clamp experimentswas performed in this high-fat–fed model to evaluate whetherthe high-fat diet induces insulin resistance.

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FIG. 3. Activation of central lactate metabolism lowers glucose production in the high-fat diet–induced insulin-resistant model. A: Normal male Sprague-Dawley rats (weight $~$ 240 g, n = 5) had a caloric intake of $~$ 85 kcal/day (standard chow at Toronto General Hospital) ( ${square}$ ). Once the rats were switched to a lard oil–enriched diet (n = 5; ${blacksquare}$ ), the rats increased their caloric intake to $~$ 130 kcal within 1 day, and the elevation of caloric intake was maintained for 3 days (**P < 0.01 vs. regular diet). B: Administration of ICV lactate lowered glucose production in the high-fat–fed rats (***P < 0.001 vs. ICV saline high-fat diet) to the same extent as in the regular chow–fed rats (***P < 0.001 vs. ICV saline regular diet) during the clamp. C: Insulin levels were comparable in all groups during the clamp. D: Glucagon levels were comparable in all groups during the clamp.

Biochemical analysis.
Plasma glucose concentrations were measured by the glucose oxidasemethod (Glucose Analyzer GM9; Analox Instruments, Lunenberg,MA). Plasma insulin, glucagons, and leptin concentrations weremeasured by RIA (Linco Research, St. Charles, MO).

Calculation and statistical analysis.
One-way ANOVA was performed to compare differences between treatments(ICV saline versus ICV lactate) in specific individual groups.Two-way ANOVA was performed to compare differences between theeffects of ICV lactate in STZ, experimentally induced hypoinsulinemia,and high-fat–fed rodents using treatment (ICV saline vs.ICV lactate) and experimental (STZ vs. experimentally inducedhypoinsulinemia vs. high-fat fed) groups as independent variables.Statistical calculations were performed using SAS software (SAS,Cary, NC). Analysis revealed no interaction between the treatmentand the experimental groups, indicating that ICV lactate similarlylowered glucose production in all three models. Data are presentedas means ± SEM. The final 30 min of the experiments wereaveraged for the "ICV" time period and used for the calculationof plasma glucose, insulin, and glucagon levels and glucoseproduction rates. The start of the experiment (t = 0 min) wasused for the "pre-ICV" time period and for the calculation ofstarting plasma glucose levels.

RESULTS AND DISCUSSION

TOP
ABSTRACT
RESEARCH DESIGN AND METHODS
RESULTS AND DISCUSSION
REFERENCES

To examine whether the activation of central nervous system(CNS) lactate sensing mechanisms lower glucose production andglucose levels in diabetes (Fig. 1A), we first established anearly-onset uncontrolled diabetic rat model with an intravenousSTZ injection (11). Within 30 h of the STZ injection (60 mg/kg),plasma glucose levels were elevated to at least 15 mmol/l. Themetabolic effects of CNS lactate sensing were tested in theSTZ rats whose plasma glucose levels were elevated to $~$ 20 mmol/lfor $~$ 24–30 h (or 54–60 h post-STZ injections) (Fig. 1C).We first examined the peripheral glucose metabolism in theseSTZ rats using tracer-dilution methodology (Fig. 1B) (10). Hepaticglucose production in ICV saline–administered STZ ratswas elevated to $~$ 22 from 11.2 ± 0.7 mg · kg^–1· min^–1 (as seen in normal rats) (Fig. 1D). Thiselevation of glucose production increased plasma glucose levelsto $~$ 20 mmol/l (Fig. 1C) in the presence of very low plasma insulin(Fig. 1E) but normal glucagon levels (Fig. 1F).

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FIG. 1. Activation of central lactate metabolism lowers glucose production and plasma glucose levels in uncontrolled diabetes. A: Schematic representation of the working hypothesis. Activation of hypothalamic lactate metabolism lowers glucose production and plasma glucose in the early onset of uncontrolled diabetes, selective hypoinsulinemia, and diet-induced insulin resistance. B: Experimental protocol of ICV infusion in normal and STZ-induced diabetic rats. C: STZ injections increased plasma glucose level to $~$ 18–20 mmol/l in ICV saline (n = 6) (^##P < 0.01 vs. ICV saline normal, n = 7). Administration of ICV lactate (n = 6) lowered plasma glucose levels compared with ICV saline in STZ rats (*P < 0.05). Lactate ICV lowered plasma glucose levels by 4 mmol/l or 25% from pre-ICV (or basal) (**P < 0.01 or *P < 0.05 vs. ICV saline STZ). D: STZ injection increased glucose production to $~$ 22 mg · kg^–1 · min^–1 in ICV saline (^##P < 0.01 vs. normal). Administration of ICV lactate lowered glucose production (*P < 0.05 vs. ICV saline STZ). E: STZ injection lowered plasma insulin levels in ICV saline-administered or lactate-treated STZ rats (^###P < 0.001 vs. normal). F: Glucagon levels were comparable in all groups. The plasma glucose levels for pre-ICV (or basal) were 7.2 ± 0.2 (ICV saline normal), 22.5 ± 2.6 (ICV saline STZ), and 18.3 ± 2.7 mmol/l (ICV lactate STZ) (STZ ICV saline or lactate vs. ICV saline normal, P < 0.01).

To test the metabolic impact of CNS lactate sensing in STZ rats,lactate was administered ICV at a concentration (10) that rapidlylowers glucose production and plasma glucose levels in normalrodents (Fig. 1B). Lactate ICV administration lowered glucoseproduction by $~$ 6 mg · kg^–1 · min^–1(Fig. 1D), which led to a drop in plasma glucose levels of 4.3± 0.8 mmol/l or a suppression of 25 ± 4% frompre-ICV lactate (Fig. 1C) in STZ rats. Importantly, this occurredin the presence of very low insulin (Fig. 1E) but normal glucagonlevels (Fig. 1F). Given the fact that the activation of hypothalamicinsulin signaling via direct insulin injection lowers glucoselevels in uncontrolled diabetes (11), activation of hypothalamiclactate metabolism could serve as a complementary approach thattargets the brain to lower glucose levels in diabetes. An activationof central lactate metabolism lowers glucose levels in uncontrolleddiabetes in the absence of insulin injections.

Because uncontrolled diabetes is associated with metabolic disturbancesand hypoinsulinemia, we alternatively and selectively examinedwhether central lactate metabolism regulates glucose homeostasisin the presence of hypoinsulinemia. We first established anexperimentally induced hypoinsulinemic model in normal rodentswith a method similar to that used previously in dogs (12) (Fig. 1Aand Fig. 2A). Somatostatin administered at a dosage of 1 µg· kg^–1 · min^–1 in normal rats decreasedplasma insulin levels by 50% (Fig. 2D), but plasma glucagonlevels were not affected (Fig. 2E, as seen in STZ rats). Thisexperimental approach resulted in an elevation of glucose production(15.8 ± 1.4 mg · kg^–1 · min^–1)and plasma glucose levels (10.8 ± 0.3 mmol/l) by 180–200min. Glucose production was elevated to 15.6 ± 1.1 mg· kg^–1 · min^–1 (Fig. 2C) and plasmaglucose levels to 10.9 ± 0.5 mmol/l (Fig. 2B) in normalrodents with ICV saline administration by the end of the infusionstudies (240–270 min). In contrast, in rats that receivedICV lactate administration starting at 90 min, the rise in glucoseproduction (10.2 + 2.1 mg · kg^–1 · min^–1)(Fig. 2C) and plasma glucose levels (7.3 + 0.6 mmol/l) was prevented(Fig. 2B) throughout the infusion protocol. Together with thefindings on STZ rats, these data indicate that insulin signalingis not required for central lactate metabolism to lower glucoseproduction and glucose levels and suggest that the activationof hypothalamic lactate metabolism could bypass insulin resistanceand lower glucose production in diet-induced insulin-resistantmodels.

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FIG. 2. Activation of central lactate metabolism lowers glucose production and plasma glucose level in experimentally induced hypoinsulinemia. A: Experimental protocol of ICV infusion in normal or hypoinsulinemic rats. Administration of intravenous somatostatin with ICV saline (n = 6) increased plasma glucose levels (^###P < 0.001 vs. ICV saline normal, n = 6) (B) and glucose production (^##P < 0.01 vs. ICV saline normal) (C) and lowered insulin levels (^##P < 0.01 vs. ICV saline normal rats) (D). E: Administration of intravenous somatostatin with ICV lactate (n = 6) prevented the rise in plasma glucose levels (***P < 0.001 vs. ICV saline hypoinsulinemic rats, n = 6) (B) and glucose production (*P < 0.05 vs. ICV saline hypoinsulinemic rats) (C) in the presence of low insulin levels (^#P < 0.05 vs. ICV saline normal rats) (D). E: Glucagon levels were comparable in all groups.

To directly test this hypothesis, the metabolic effects of lactateICV were tested in an early-onset high-fat diet–inducedinsulin-resistant model (13,14) (Fig. 1A). Here, we confirmthat rats fed a lard oil–enriched diet rapidly increasedtheir food intake (Fig. 3A), developed hepatic insulin resistance(% glucose production suppression from basal obtained by hyperinsulinemic-euglycemicclamps: 75 ± 5% [regular chow, n = 4] vs. 23 ±3% [high-fat diet, n = 6], P < 0.001), and had elevated plasmainsulin (0.8 ± 0.2 ng/ml [regular chow] vs. 1.9 ±0.3 ng/ml [high-fat diet], P < 0.01) and leptin (1.1 ±0.3 nmol/l [regular chow] vs. 2.1 ± 0.2 nmol/l [high-fatdiet], P < 0.01) levels. In this high fat–fed model,ICV lactate administration lowered glucose production duringthe pancreatic basal insulin clamps (Fig. 3B). Importantly,this metabolic effect of lactate ICV was comparable with thatin regular chow–fed rats (Fig. 3B). These data indicatethat central lactate metabolism bypassed insulin resistanceto lower glucose production in a diet-induced insulin-resistantmodel.

Here we report that a selective central activation of lactatemetabolism similarly lowered glucose production in the early-onsetmodels of uncontrolled diabetes, hypoinsulinemia, and diet-inducedinsulin resistance. It still remains unknown whether hypothalamiclactate sensing regulates glucose homeostasis in chronic modelsof diabetes and obesity. Furthermore, metabolic effects of lactatesensing in other regions of the brain (i.e., hindbrain) warrantfuture investigations, since inhibition of neuronal lactatetransport (the reverse of direct lactate administration, asdone in the current study) in the hindbrain increases plasmaglucose levels (15). Finally, although selective activationof central lactate metabolism lowered glucose production andplasma glucose levels in uncontrolled diabetes in the absenceof insulin injections, glucose production and glucose levelswere not fully normalized. Taken together, we postulate thattherapeutic strategy designed to activate hypothalamic lactatemetabolism could bypass insulin resistance and serve as oneof the complementary approaches to insulin injections to lowerglucose levels in diabetes and obesity.

ACKNOWLEDGMENTS

This work was supported by a research grant to T.K.T.L. fromthe J.P. Bickell Foundation. M.C. was supported by a Bantingand Best Diabetes Centre Charles Hollenberg summer studentship.T.K.T.L. holds the John Kitson McIvor Endowed Chair in DiabetesResearch at the University of Health Network and Universityof Toronto.

FOOTNOTES

Published ahead of print at http://diabetes.diabetesjournals.orgon 9 January 2008. DOI: 10.2337/db07-1464.

The costs of publication of this article were defrayed in partby the payment of page charges. This article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.Section 1734 solely to indicate this fact.

Received for publication October 12, 2007 and accepted in revised form January 5, 2008

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