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TRANSLATIONAL PHYSIOLOGY

Effect of meal and propranolol on whole body and splanchnic oxygen consumption in patients with cirrhosis

Departments of ¹Gastroenterology and ³Clinical Physiology, Hvidovre Hospital, and ²Department of Clinical Physiology, Bispebjerg Hospital, University of Copenhagen, Copenhagen, Denmark

Submitted 10 July 2005 ; accepted in final form 15 February 2006

ABSTRACT

Our aim was to measure whole body energy expenditure after a mixed liquid meal, with and without simultaneous propranolol infusion, in patients with cirrhosis. We also wanted to investigate the effect of propranolol on substrate fluxes and oxygen uptake in the tissues drained by the hepatic vein and azygos vein in the postprandial period in these patients. Whole-body oxygen uptake, hepatic blood flow, hepatic venous pressure gradient and net-hepatic fluxes of oxygen, lactate, glucose, glycerol, and free fatty acids (FFA) were measured in 12 patients with alcoholic cirrhosis before and for 2 h after ingestion of a mixed liquid meal (700 kcal). Half of the patients (n = 6) were randomized to a treatment group receiving intravenous infusion of propranolol in combination with the meal. The meal-induced energy expenditure was significantly lower in patients given propranolol [15.0 ± 18.9 vs. 67.0 ± 26.1 kJ/120 min (means ± SD), P < 0.01]. Meal-induced whole body oxygen uptake was lower in patients receiving propranolol (19.2 ± 38 vs. 135.7 ± 61 mmol/120 min, P < 0.01), and the meal-induced increase in splanchnic oxygen uptake was nonexistent when propranolol was administered in combination (–13.2 ± 34.8 vs. 110.4 ± 34.8 mmol/120 min, P = 0.04). Postprandially, the propranolol group had a tendency toward a reduced splanchnic glucose output, and the FFA uptake was significantly reduced. Propranolol reduces meal-induced whole body oxygen uptake and energy expenditure as well as splanchnic oxygen uptake. The splanchnic reduction in oxygen consumption can explain almost the entire reduction in whole body oxygen consumption.

calorimetry; catheterization; azygos vein; portal hypertension

The aims of the present study were 1) to measure whole body EE in patients suffering from cirrhosis after a mixed liquid meal with and without simultaneous propranolol infusion and 2) to investigate the effect of propranolol on substrate fluxes and oxygen uptake in the tissues drained by the hepatic vein and azygos vein during the postprandial period in these patients.

MATERIALS AND METHODS

Patients. Twelve patients with biopsy-proven alcoholic cirrhosis and portal hypertension were studied. All patients had endoscopically verified esophageal varices without previous bleeding. All had abstained from alcohol for at least 3 wk before the study. After measurements of basal hemodynamic variables in the fasting patient, the patients were randomized to treatment groups receiving either a liquid meal alone or in combination with intravenous infusion of propranolol. Six patients ingested the meal alone, and six received propranolol in addition. Patient's characteristics of the two study groups are listed in Table 1. Nine patients received diuretic treatment: five in the propranolol group [5 received spironolacton (100–200 mg/day), and 5 were given furosemide (40–160 mg/day)] and four in the control group [4 received spironolacton (100–200 mg/day), and 4 furosemide (40–160 mg/day)]. The diuretic treatment was withheld 24 h before the study. The patients had not previously been treated with propranolol or any other drug, with a potential influence on portal pressure. All gave written informed consent, and the ethics committee for medical research in Copenhagen approved the study (V100.770/87) as being in accordance with the Helsinki II declaration.

Propranolol infusion. Patients randomized to a meal in combination with propranolol received a bolus intravenous injection of 0.1 mg/kg propranolol immediately after the termination of the meal. Subsequently, a constant infusion of 1 µg·min^–1·kg^–1 propranolol was administered until cessation of the measurements 2 h after ingestion of the meal. To ensure that the propranolol did not influence the absorption of the meal, plasma glucose was measured at baseline and in 30-min intervals for the whole period. All patients had an increase in plasma glucose of >20%, and no difference was observed between the two treatment groups. Maximal plasma glucose occurred 60–90 min after the meal, irrespective of treatment.

Whole body oxygen uptake. Whole body oxygen uptake (Vo₂), carbon dioxide output, and respiratory exchange ratio (RER) were measured continuously by indirect calorimetry using an open-circuit ventilated hood system before and for 2 h after the meal. For calculations, mean values for every half hour were used. Oxygen was measured with an electrochemical oxygen sensor (Amtec Thermox, Pittsburg, PA), and carbon dioxide was measured by an infrared carbon dioxide sensor (Amtec Thermox). Airflow through the system, relative air humidity, and air temperature were measured, and all the parameters were monitored online by computer. A detailed description of this system and the calibration procedure has been given in previous studies (41).

EE was calculated as EE = (15.48 + 5.55 x RER) x Vo₂ (kJ) (18).

The meal-induced thermogenesis was calculated as the difference between resting EE and the integrated postprandial EE, as area under curves by the trapezoid method. Meal-induced thermogenesis is also expressed as the postprandial increase in EE as percentage of the energy content of the meal in the control group.

Catheterization. After an overnight fast, hepatic venous catheterization was performed. In brief, a Cournand catheter, size 7-Fr, was inserted through the right femoral vein under local analgesia and guided to a hepatic vein under fluoroscopy. In addition, a venous introducer, size 8-Fr, was placed in the right femoral vein to permit passage of an azygos catheter. A short indwelling catheter (5-Fr) was introduced in the right femoral artery by the Seldinger technique. Azygos vein catheterization was performed by a double-termistor coronary sinus catheter (Webster Laboratories, Altadena, CA), and blood flow was measured by thermodilution (11). At each observation, at least three measurements were performed, and the mean value was applied.

Assessment of splanchnic hemodynamics. HBF was measured by the indocyanine green (ICG) technique (24). Proceeded by a priming dose (2 mg), a constant intravenous infusion of ICG (0.2 mg/min; calibrated pump, O Dich, Copenhagen, Denmark) in a 5% human albumin was given until termination of the catheterization. An equilibrium period of 20 min was required before blood samples were simultaneously drawn from the hepatic vein and artery for analyses of ICG. ICG clearance was determined as infusion rate of ICG (I_ICG; corrected for unsteady plasma concentration) divided by arterial plasma concentrations of ICG. A hepatic extraction of ICG >10%, required for the assessment of HBF, was present in all patients. HBF = I_ICG/(ICG_a – ICG_hv)/(1 – Hct), where ICG_a represents arterial ICG concentration, and ICG_hv represents hepatic venous ICG concentration. The hepatic blood flow was not measured at 90 min. The 90-min value was extrapolated from values at 60 and 120 min.

Blood sampling and analyses. Blood samples were simultaneously drawn from all three catheters after discharge of catheter dead space. Blood was collected for analyses of hemoglobin, glucose, pyruvate, glycerol, lactate, and free fatty acids (FFA). Glycerol and FFA were determined as described by Laurell and Tibbling (28, 29). Lactate and pyruvate were determined after precipitation of protein by perchloric acid as described by Bergmeyer (10). Blood gas analyses were performed electrometrically (Radiometer ABL, OSM, Copenhagen) on simultaneously drawn samples from femoral artery, hepatic vein, and azygos vein. Oxygen uptake (Vo₂) was determined as HBF x Hb x 22.4 x (SO_2,a – SO_2,v), where Hb is the concentration of hemoglobin in blood and SO_2,a and SO_2,v are oxygen saturation in the artery and vein, respectively. The oxygen content of the blood was adjusted for physically dissolved oxygen by determination of oxygen tension. Meal-induced increases in oxygen uptake, in tissues drained by the hepatic vein (splanchnicus), and the azygos vein were calculated as the integrated increase in oxygen uptake above the baseline fasting level during the 2 h after the meal. Fluxes of lactate, glucose, pyruvate, glycerol, and FFA across the tissues drained by the hepatic vein and the azygos vein were calculated by Fick's principle (arteriovenous concentration differences multiplied by the appropriate blood flow/plasma flow). Plasma flow was used in FFA and blood flow in oxygen, lactate, pyruvate, glucose, and glycerol. Glucose and lipid oxidation rates were calculated by a protein oxidation rate (0.35 mg·kg^–1·min^–1) from a previous study in cirrhotic patients by Shmueli et al. (40).

Statistics. All results are presented as means ± SD. Comparisons within each group were performed with Student's t-test for paired data. ANOVA was used for comparison between groups. Analyses of effect of time between groups were done in SAS statistical software package using the method of "repeated measurements." Fixed factors were group and time and random factor person. P < 0.05 is considered statistically significant.

RESULTS

Clinical data and biochemical test values of the study groups are given in Table 1. No significant differences between the two groups were observed regarding age, sex, and severity of the disease (Child-Pugh score). As earlier reported (9), we observed the well-known effects of -adrenergic blockade on systemic and splanchnic hemodynamics (Table 2): postprandial rise in hepatic venous pressure gradient and HBF were both reduced by propranolol. Heart rate also decreased after the meal in combination with propranolol. The HBF increased in the control group. However, in the propranolol group, it did not change significantly after the meal and remained significantly lower compared with the control group.

View larger version (14K): [in this window] [in a new window]   Fig. 1. Individual values of whole body oxygen uptake after a meal with and without propranolol infusion.

View larger version (10K): [in this window] [in a new window]   Fig. 2. Meal-induced changes in whole body and hepatic oxygen uptake in patients receiving propranolol compared with controls. Bars represent average increases in oxygen uptake above baseline in the 2 h following meal ingestion. *P < 0.01. Error bar = SD.

View larger version (24K): [in this window] [in a new window]   Fig. 3. Splanchnic uptake/output of metabolites at baseline and in the 2 h following meal ingestion.

The present study showed that meal-induced whole body oxygen uptake and splanchnic oxygen uptake are reduced by propranolol in patients with cirrhosis. The splanchnic reduction in oxygen consumption can explain almost the entire reduction in whole body oxygen consumption (Table 3, Fig. 2). Our results are in contrast to findings in healthy persons, where -blockade has no effect on the postprandial thermogenic response after a mixed meal (42). The meal-induced thermogenesis consists of two components: the obligatory thermogenesis refers to the EE for digestion, absorption, conversion, and storage of nutrients, and the facultative thermogenesis is the energy spend in excess of the obligatory requirements. The facultative thermogenesis has been shown by Acheson et al. (1) to be mediated by the sympathico-adrenal system.

The patients were followed 2 h after meal ingestion, a period that does not cover the total postprandial metabolism. In a study by Jensen et al. (26), normal subjects were investigated 6 h postprandially after a mixed meal and diet-induced increase in whole body and splanchnic oxygen uptake was not back to baseline after the end of the study. On the other hand, despite the elevated plasma glucose at 120 min, splanchnic substrate exchange may be completed because splanchnic glucose output was back to normal (Fig. 3), which has previously been observed in patients with cirrhosis(19). The elevated plasma glucose at 120 min more likely reflects peripheral insulin resistance, which is well known in patients with cirrhosis (37, 40).

Crossover design was not done, although it could have adjusted for baseline heterogeneity. However, we could not ethically justify performing two long-lasting catheterizations within a short interval, and the numerous blood samples may cause anemia. Furthermore the patients had significant portal hypertension and esophageal varices, a clinical condition that should be treated with propranolol to prevent bleeding from esophageal varices. The patients are in this randomized setup and are matched regarding child class, decompensation, and splanchnic and systemic hemodynamics.

-Adrenergic blockade.

To obtain a stable -adrenergic blockade and to avoid interference between intestinal food absorption and propranolol absorption, we infused propranolol. With respect to duration of catheterization, we could not wait 90 min for an oral dose of propranolol to be absorbed (4, 32). Mean dose of propranolol was 14.2 mg during the 2 h. This dose correspond to a plasma level of 50–60 ng/ml in normal controls (42) and a blockade of 60–70% of exercise-induced tachycardia (15).

To shorten the catheterization period, a baseline period during -adrenergic blockade without the meal was omitted. This would have been preferred, but with these types of patients, the studies have to be of limited duration and with limited blood sampling. In a similar setup, MacMathuna et al. (32) found unaltered systemic and hepatic oxygen consumption following intravenous propranolol. However, we have shown earlier that splanchnic oxygen consumption decreases 18% after an oral dose of 80 mg propranolol (7). In the present study, the splanchnic oxygen consumption in the control group increased by 30% after the meal, whereas no response was observed in the propranolol group. This indicates that the difference in response represents a combined effect of propranolol on both the hemodynamics and the meal-induced thermogenesis.

In patients with cirrhosis, 16–34% are hypermetabolic, which is partly explained by increased sympathetic activity (36). In the present study, the level of catecholamine was not measured, but is well known that the level of circulating catecholamine is increased in patients with cirrhosis and portal hypertension (5, 8). Muller et al. (36) has observed that propranolol infusion reduces whole body oxygen uptake, maximum 6%, even in hypermetabolic persons. When comparing the resting EE (REE) of the patients in the present study with resting EE in healthy humans, our patients were without signs of significant hypermetabolism, when hypermetabolism is defined as REE exceeding the predicted value by >20% (20, 36). This minor effect does not explain our findings, because we observed a postprandial reduction of 25% (90 min after the meal). On the other hand, Jensen et al. (26) found a significant increase in plasma norepinephrine concentrations after ingestion of a mixed meal (but no increase in epinephrine), indicating a meal-induced increase in sympathetic activation, which can be involved in mediating the meal-induced increase in oxygen consumption and can be inhibited by the infusion of propranolol.

In healthy subjects, an increased hepatic oxygen demand can be met by increasing the oxygen extraction from the blood. In cirrhosis, hepatic and splanchnic oxygen uptake is decreased and the splanchnic oxygen demand is dependent on the splanchnic blood flow (27, 43). In the present experiment, we observed a postprandial increase in HBF and oxygen extraction across the splanchnic tissue in the control group, whereas the propranolol group did not experience postprandial change in oxygen extraction despite a significant decrease in HBF compared with the control group. Therefore, it could be speculated that propranolol may reduce hepatic metabolic functions by decreasing splanchnic blood flow and thereby splanchnic oxygen uptake (7). Apart from the reduction in splanchnic oxygen consumption, the extrasplanchnic effects include reduced cardiac oxygen uptake parallel to reduction in heart rate and mean arterial pressure.

In the baseline fasting period, it can be calculated that gluconeogenesis may contribute to 30–40% of the splanchnic glucose output assuming that all the splanchnic uptake of lactate and glycerol is used for gluconeogenesis. This is probably a minimum estimate because alanine, which was not measured, also contributes to gluconeogenesis. Postprandially, uptake of gluconeogenetic precursors decreases in both groups, which probably represents a decrease in hepatic glucose production. If we assume that all glucose (58 g) is absorbed at 120 min (see Fig. 3; splanchnic substrate exchange seems to be completed) and that hepatic glucose production is reaching zero, we can assume that most of the absorbed glucose is taken up in the liver. The splanchnic glucose output was 5 mmol/min (Table 5), which is equivalent to 11 g/120 min of glucose. This corresponds to the integrated increase in peripheral glucose oxidation after the meal, which is 7 g/120 min (see Table 3) in both groups. Gluconeogenesis is an energy-consuming process, and because there is a tendency of lower postprandial glucose output in the propranolol group (Table 5), this may explain some of the difference in postprandial splanchnic thermogenesis. Gluconeogenesis decreases due to reduced precursor uptake; however, the increase in glucose output may partly be due to glycogenolysis, which is an energy-consuming process via cAMP-dependent protein kinase, although not as energy consuming as gluconeogenesis. The postprandial arterial FFA concentration decreased as expected, most likely due to an increase in circulating insulin. However, the decrease was more pronounced in the propranolol group, indicating that propranolol may also have peripheral antilipolytic effects in cirrhotic patients. The pronounced decrease in FFA gives rise to a decreased delivery of FFA to the liver. This is in accordance with the present results where the postprandial splanchnic FFA uptake was significantly lower in the propranolol group compared with the control group. Ketone body production from fatty acid metabolism is an energy-consuming process, and in the propranolol group, it could explain some of the decreased postprandial splanchnic oxygen consumption. However, postprandial oxygen consumption is substrate specific, and amino acids have the strongest thermic effect on hepatic metabolism, due to protein synthesis, ureagenesis, and gluconeogenesis from amino acids (35). In the present study, we did not measure the protein metabolism, but it has been shown that -blockade reverses muscle protein catabolism in severely burned patients and thereby decreases the amino acid delivery to the liver (25).

Decreased splanchnic oxygen uptake in cirrhosis has been shown to be associated with a decrease in metabolic liver functions, because a decrease in splanchnic Vo₂ correlates significantly with decreased splanchnic glucose production as well as a decrease in splanchnic FFA extraction (43). Therefore, hepatic blood flow can become limiting for the metabolic capacity of the liver, and in the postprandial period, there may be a risk of severe hypoxemia and local injury in the liver. We found no significant difference in oxygen concentrations between patients who received propranolol and those who did not (data not shown). The oxygen concentration decreased after the meal in both groups in the azygos and hepatic veins. Only one patient had a severe drop in oxygen concentration in the hepatic vein (from 3.46 to 1.16 mM). However, this did not lead to anaerobic metabolism reflected by pyruvate and lactate. The postprandial lactate-to-pyruvate ratio (Table 4) in the hepatic vein decreased in both groups, which indicates improved energy balance. This is in accordance with a study by MacMathuna et al. (32), who measured what the ratio between the ketone bodies acetoacetate and -hydroxybutyrate was in the hepatic vein as an indirect measurement of the hepatic mitochondrial state. They found that -blockade did not alter the hepatic redox state in the total group of patients with cirrhosis but found an improvement in the patients with the most advanced disease.

The main energy-requiring processes in the liver are ureagenese, futile cycling of substrates, gluconeogenese, protein synthesis, Na⁺ K⁺-ATPase activity, and ketogenesis (34, 35). It has been reported that the cirrhotic liver seems to have reduced glycogen stores and limited gluconeogenetic capacity (35, 44). The present study indicates that ketogenesis and gluconeogenesis may be impaired by propranolol infusion, although we did not measure ketogenesis or gluconeogenesis. On the other hand, the postprandial increases in RER in both groups, together with the increased glucose concentration, indicate that the extrahepatic carbohydrate metabolism is unaltered during -blockade.

Azygos vein in cirrhosis.

In healthy persons, the azygos vein is mainly draining the interscapular region of the thoracic wall. However, in patients with portal hypertension, portosystemic collaterals develop; these are mainly drained by the azygos vein, and the azygos blood flow is often markedly increased compared with controls (500 vs. 115 ml/min) (13, 14, 23). The magnitude of collateral flow seems to influence the course of variceal bleeding (12, 13). The blood flow in other portosystemic collaterals is very difficult to quantify and thereby the oxygen consumption and flux of metabolites is in these (6, 22). Therefore, the calculations regarding collaterals are minimum values and probably an underestimate. In the patients studied, the Vo₂ in the azygos is 6% of whole body Vo₂ at rest and increases after the meal (Table 3). This is in accordance with the concept that the azygos vein is partly derived from the splanchnic area, because in normal subjects, the Vo₂ in the tissues drained by the azygos vein amounts to 2% of whole body Vo₂ and does not increase after a meal (14). Furthermore propranolol prevented a significant increase in azygos flow after the meal (Table 2).

In conclusion, propranolol reduces meal-induced whole body oxygen uptake and EE as well as splanchnic oxygen uptake in patients with cirrhosis. The splanchnic reduction in oxygen consumption can explain almost the entire reduction in whole body oxygen consumption. Postprandially, in the propranolol group, a tendency toward a reduced splanchnic glucose output and a significant reduction in FFA uptake was observed.

FOOTNOTES

Address for reprint requests and other correspondence: A. Krag, Dept. of Gastroenterology 439, Hvidovre Hospital, Kettegaard Allé 30, 2650 Hvidovre, Denmark (e-mail: Aleksander.Krag{at}hh.hosp.dk)

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

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