Introduction
Hypoxemia complicates critical care settings, ranging from progressed lung disease to certain medical interventions [
1‐
3]. Clearly, reversing hypoxemia is pivotal [
4], but adapting pharmacological interventions to support the subject during impending or actual hypoxemia also appears beneficial. Systemic hypoxemia triggers multiple patho-mechanisms [
5] also affecting the cardiovascular system: among others, at the cardiac level hypoxia depresses cardiac function by myofilament Ca
2+-desensitization [
6,
7], and at the vascular level hypoxia triggers activation of K
ATP
+
channels [
8], facilitating blood flow to tissues otherwise at risk for hypoperfusion by intense vasoconstriction.
In this context, the inodilator levosimendan (LEVO) appears to be an attractive option to support the cardiovascular system at risk in (impending) hypoxemia since it acts both as cardiac myofilament Ca
2+-sensitizer and K
ATP
+
channel opener, thus reversing hypoxia-induced cardiodepression and supporting regional vasodilation. This appears to be particularly of interest in hypoxic settings, since LEVO putatively increases cardiac output (CO) partly independent of an additional increase in oxygen consumption (VO
2) [
9].
Hypoxia, like other cardiovascular stressors, triggers impairment of splanchnic oxygenation, likely through a combination of abnormal mesenteric perfusion [
10‐
12] and hypoxemia. However, particularly the gastrointestinal mucosa is susceptible to hypoxia, and mucosal hypoxia appears to trigger the development of critical illness [
13]. Thus, interventions intended to improve systemic (hemodynamic) variables during hypoxia should not further compromise regional mucosal circulation or oxygenation [
14]. Therefore, in addition to systemic variables, we measured the effects on regional gastromucosal oxygenation.
Clinically, LEVO is primarily indicated for the treatment of acute and chronic ischemic cardiac failure, with promising clinical data available [
15,
16]. Moreover, LEVO is also increasingly advocated to treat nonischemic cardiac failure, including septic or toxic cardiodepression [
17‐
23]. The beneficial effects of LEVO, in addition to positive inotropic effects, may be caused by vasodilation [
24]. Mechanistically, vasodilation by LEVO is mediated by activation of K
ATP
+
channels, which also appear involved in the vasodilation triggered by hypoxia [
8,
25].
These K
ATP
+
channels, activated by LEVO or hypoxia, are pharmacologically blocked by glibenclamide (GLIB) [
26‐
30]. In this context, GLIB pretreatment has previously been published as a research tool to study the contribution of GLIB-sensitive K
ATP
+
channels to the effects of LEVO and other cardiovascular challenges [
26‐
30]. Thus, to elucidate the contribution of K
ATP
+
channels in the present study, we tested if K
ATP
+
channel blockade by GLIB pretreatment would alter the (circulatory) condition during hypoxia, both with and without a LEVO pretreatment.
GLIB, based on the same mechanism, i.e., antagonizing K
ATP
+
channel-dependent vasodilation, is of growing interest in intensive care medicine [
31]. In this context, GLIB is studied as nonadrenergic vasopressor in various shock-related vasodilatory states, caused by excessive K
ATP
+
channel activation. Examples for this therapeutic concept are septic or hemorrhagic vasodilation [
32,
33]. In this regard, GLIB increases systemic vascular resistance and thus arterial blood pressure [
32].
In the present study, the combination of LEVO (to increase cardiac contractility) and GLIB (to increase systemic vascular resistance) could achieve the putatively beneficial combination of antagonizing both possible cardiodepressant and vasodilatory effects of systemic hypoxia.
Materials and methods
The data derive from repetitive experiments on healthy dogs (foxhounds, n = 6, 24–32 kg) treated in accordance with the National Institutes of Health guidelines for animal care and with approval of the District Governmental Animal Investigation Committee.
For the continuous measurement of cardiac output (CO), ultrasonic flow transducers (S-series, Transonic, Ithaca, NY, USA) were chronically implanted around the pulmonary artery [
34]. Before the experiments, food was withheld for 12 h. The experiments were performed under sedation with sevoflurane (end-tidal concentration 3.0 vol%, corresponding to ~1.25 MAC in dogs [
35]) and neuromuscular block (rocuronium 0.6 mg kg
−1, followed by 1.0 mg kg
−1 h
−1). Mechanical ventilation (FiO
2 0.3; tidal volume 12.5 mL kg
−1 in dogs [
36], respiratory rate ~20 min
−1) was adjusted to maintain normocapnia as verified by continuous capnography (end-tidal CO
2 35 torr) and arterial blood gas analysis. The dogs were covered with warming blankets to maintain body temperature (~37.5°C, rectal thermoprobe).
Measurements
Systemic oxygen consumption
Systemic oxygen consumption (VO
2) was measured continuously by indirect calorimetry (Deltatrac-II metabolic monitor, Datex, Helsinki, Finland) and thus was methodologically independent from the determination of CO and DO
2 [
9].
Systemic hemodynamics and oxygenation
We continuously measured heart rate (HR, electrocardiogram), mean arterial (aortic) pressure (MAP; P23ID, Elk Grove, CA, USA), central venous pressure (P23ID; right atrial catheter tip position confirmed by fluoroscopy), and ultrasound-derived CO (flowmeter T106, Transonic). At the end of each intervention, we performed transpulmonary thermodilution (PiCCO monitor with thermistor-tipped carotid catheter PV-2014L, Pulsion, Munich, Germany; measurements performed according to the manufacturer; with ~0.4 mL kg
−1 iced saline) to determine the following: global end diastolic volume (GEDV), derived intrathoracic blood volume (ITBV), and extravascular lung water (EVLW). The PiCCO system also provided the pulse-contour-derived stroke volume variation (SVV) and the estimate of cardiac contractility +d
P/d
t
max. This system is validated to measure EVLW in dogs [
37] and has also been applied in other canine studies [
38].
Intermittently we measured arterial blood gas tensions (PaO2, PaCO2) and acid/base-related variables [pH, base excess (BE); ABL-700, Radiometer, Copenhagen, Denmark; no buffer solutions were used]. Additionally, we determined arterial serum metabolites (glucose, lactate) and electrolytes ([K+], [Ca2+], [Na+], [Cl−]). According to standard formulas, we calculated systemic vascular resistance (SVR), arterial oxygen content (CaO2), and systemic oxygen transport (DO2).
Gastromucosal oxygenation
Gastromucosal oxygenation was continuously assessed by reflectance spectrophotometry [
9,
39]. Briefly, light (502–628 nm) is transmitted to the tissue via a micro light guide, and the reflected light is analyzed for the percentage of oxygenated microvascular hemoglobin (μHbO
2). The flexible probe (diameter 2.0 mm) was introduced into the stomach via an orogastric silicone tube (14 Charrière). During the experiments, correct probe position was confirmed by online evaluation of the signal quality (software version 2.0).
Experimental program
After induction (propofol 4 mg kg−1 i.v.) and endotracheal intubation, all catheters were inserted and 30 min was allowed to establish steady-state conditions. Blood was sampled for baseline analysis, and thereafter a randomization was performed to allocate the dogs to the experimental groups.
Hypoxia episodes
The hypoxic episodes were induced by switching FiO
2 from 0.30 to 0.11 [
40], as continuously measured (Capnomac ultima, Datex Instrumentarium, Helsinki, Finland). Each hypoxic episode was maintained for 15 min to allow steady states of the measured variables to be achieved.
Drugs
The agents LEVO and GLIB were infused as follows by a pressure-limited infusion pump via the central venous catheter.
LEVO
After baseline measurements, LEVO (Simdax, Abbott, Wiesbaden, Germany) was administered with an initial loading dose of 20.0 μg kg
−1 over 15 min, followed by continuous infusion of 0.25 μg kg
−1 min
−1 for the remaining experimental period, a dosing regimen adapted from a similar canine model [
9].
GLIB
GLIB (G0639, Sigma, Frankfurt, Germany), as K
ATP
+
channel antagonist, was infused at a dose of 0.2 mg kg
−1 over 10 min, and 30 min were allowed for stabilization. This dose was derived from previous canine studies addressing the contribution of K
ATP
+
channels to the effects of LEVO and other cardiovascular modulators [
26‐
30].
Experimental protocols
Group I
This protocol served to study the effects of hypoxia per se and to study the associated effects of GLIB pretreatment. After steady-state baseline measurements, a first hypoxic challenge was performed. After 60 min recovery from this hypoxia (measurements after 30 and 60 min recovery), GLIB was infused. Following this GLIB pretreatment, a second hypoxic episode was induced.
Group II
This protocol served to study the effects of LEVO pretreatment on hypoxia and further to study the role of GLIB pretreatment in this regard. After a baseline period, LEVO pretreatment was administered, and thereafter a first hypoxic episode was induced. After 60 min recovery from this hypoxia (measurements after 30 and 60 min recovery), with LEVO continuously infused, GLIB pretreatment was administered. Thereafter, with the combined LEVO + GLIB pretreatment, a second hypoxic challenge was induced.
Statistical analysis
Statistical analysis was performed using Prism software (version 5.0, GraphPad, La Jolla, CA, USA). Data are presented as absolute values of mean ± SEM for n = 6 animals per group in the manuscript and tables. Direct drug effects (before onset of hypoxemia) were described by one-way ANOVA for repeated measurements, corrected for multiple comparisons (Bonferroni). Differences during hypoxemia were tested both between groups (i.e., I and II) and between the hypoxia conditions (i.e., without and with GLIB pretreatment) using a two-way ANOVA, corrected for multiple comparisons (Bonferroni). Significance was assumed at p < 0.05.
Discussion
For the present study we developed a model of moderate hypoxic hypoxemia, adapting reported canine hypoxia models [
40,
41]. Repetitive experiments were performed in a randomized mode on healthy, chronically instrumented dogs with intervals of ≥2 weeks to exclude carryover effects and to minimize interindividual differences. Furthermore, the use of chronically instrumented animals avoided acute, surgical instrumentation and thus confounders such as endocrine stress responses to surgery. In addition, our model allowed us to study the animals during sedation with sevoflurane and rocuronium alone, i.e., without need for analgesics or other confounding drugs [
42].
In this study, two subsequent episodes of hypoxia were induced per group. While the first hypoxic episode served to elucidate the effect of LEVO pretreatment, the second hypoxic episode served to elucidate the role of K
ATP
+
channels (by subsequently adding GLIB pretreatment, reported to block GLIB-sensitive K
ATP
+
channels [
26‐
30]). Between the two hypoxic episodes, an extended normoxic period was interposed to allow complete recovery of measured variables. In addition, to exclude the possibility that the first hypoxic episode was affecting the second with respect to measured variables, pilot experiments were performed, comparing a first with a second hypoxic period without adding any medication (i.e., no GLIB) in between. These pilot experiments demonstrated no differences between the first and second hypoxic episode, with respect to the measured variables.
Gastromucosal μHbO
2 was continuously measured by reflectance spectrophotometry [
43], with the light guide nontraumatically introduced via an orogastric tube [
9,
39]. Reflectance spectrophotometry allows determination of microcirculatory oxygen availability [
44], and gastric endoluminal reflectance spectroscopy has been reported predominantly to measure capillary hemoglobin oxygenation of the mucosa [
45].
Both hypoxia and the administered drugs may affect pulmonary endothelial permeability. Thus, we assessed EVLW by the PiCCO system, a method validated in anaesthetized dogs [
37]. The EVLW data do not support pulmonary edema as cause of the small but significant differences in PaO
2 between distinct hypoxia conditions (i.e., slightly lower with LEVO and/or GLIB), rendering an altered pulmonary shunt, as also reported for other vasoactive agents [
46], as the most likely explanation.
LEVO appears to be a promising candidate agent to support the cardiocirculatory system during hypoxemia, particularly because circulatory stimulation by LEVO is reportedly independent of metabolic stimulation [
9]. Our data support this concept, demonstrating that LEVO pretreatment resulted in improved systemic circulation (CO) also during hypoxemia without fueling aerobic (VO
2) metabolism. Thus, the pattern of increased CO at stable VO
2 was present also during hypoxemia in LEVO-pretreated subjects and, in turn, other factors triggered by hypoxemia, e.g., changed pharmacology [
47], did not alter this pattern. Measured key modulators of vascular tone (PaCO
2, pH, temperature, arterial [K
+] and [Ca
2+]) did not differ between the hypoxemic episodes, supporting that LEVO-specific mechanisms cause the differences in cardiovascular response.
The present study was designed to suggest a concept to improve the condition of the subject before an anticipated hypoxemia evolves; however, the majority of clinical hypoxemia episodes occur unexpectedly. Therefore, future studies will have to demonstrate if our findings are confirmed in the clinically more likely setting, i.e., with LEVO administered in a therapeutic rather than prophylactic approach [
24,
48].
Increased CO during hypoxemia after LEVO pretreatment, compared to unpretreated hypoxemia, was associated with an increased +d
P/d
t
max, compatible with positive inotropic effects of LEVO by myocardial Ca
2+ sensitizing. LEVO, besides acting as a cardiac Ca
2+ sensitizer, also activates K
ATP
+
channels. Physiologically, various K
ATP
+
channel isoforms exist, classified by their respective sulfonylurea receptors (SUR) in pancreatic β-cells (SUR-1), and striated (SUR-2A) and smooth muscle cells (SUR-2B). Vascular smooth muscle K
ATP
+
channels link regional metabolism to perfusion, since intracellular ATP depletion (e.g., during hypoxia) triggers these channels, leading to hyperpolarization and thus vasorelaxation [
8]. However, excessive activation of these K
ATP
+
channels is involved in multiple pathological vasodilatory states, e.g., septic shock [
8,
25]. Thus, whether pharmacological activation of K
ATP
+
channels under pathological conditions by LEVO is beneficial might also depend on the individual vasodilatory state. Pharmacologically, K
ATP
+
channels are antagonized by sulfonylurea derivatives, with GLIB (glyburide) reported to unspecifically block all receptor isoforms, SUR-1, SUR-2A, and SUR-2B. GLIB has been reported to be effective as a K
ATP
+
channel antagonist in dogs before, in similar dosages as applied in the present study [
26‐
30]. Activity of GLIB in our model is suggested by the hypoglycemic response after GLIB pretreatment (SUR-1 effect), with arterial glucose decreased from baseline values of ~100 to ~50 mg dL
−1 (end of experiments). In addition, GLIB pretreatment significantly increased SVR, suggesting (partial) blockade of vascular K
ATP
+
channels.
Thus, although GLIB pretreatment significantly increased SVR in this model, the demonstrated marked hypoglycemic effect of GLIB may limit its clinical use.
Combined GLIB + LEVO pretreatment resulted in significantly higher CO and +d
P/d
t
max than GLIB pretreatment alone during hypoxemia, compatible with the notion that mechanisms other than K
ATP
+
channel opening contribute to LEVO effects, also during hypoxemia. Besides Ca
2+ (re-)sensitization, LEVO’s action as a phosphodiesterase (PDE) inhibitor could also contribute. In this regard, other PDE-III inhibitors have demonstrated positive systemic and regional gastrointestinal mucosal effects during hypoxemia [
14].
Despite significant systemic differences, regional gastromucosal oxygenation did not differ between LEVO-pretreated and unpretreated hypoxemia, which decreased equally to ~30%. Regional regulation of mucosal perfusion during hypoxemia could overrule the effects of LEVO, despite an increased CO and reduced SVR in LEVO-pretreated hypoxia. A possible mechanism is that local hypoxia activates vasodilatory K
ATP
+
channels to such extents that LEVO can not confer significant additional vasodilation. Indeed after GLIB pretreatment, administered to block these vasodilatory K
ATP
+
channels and thus to induce vasoconstriction, we observed clear trends towards lower μHbO2 both in LEVO-pretreated (from 32 ± 4 to 24 ± 4%) and unpretreated hypoxemia (from 30 ± 4 to 25 ± 3%). Interestingly, also in both groups arterial lactate concentrations were significantly lower after GLIB pretreatment. Since arterial pH and the other acid/base-related variables remained close to baseline under all hypoxemia conditions, we doubt that these significant differences in lactate concentration are caused by different perfusion states, rendering direct metabolic effects of GLIB more likely to contribute.
LEVO is clinically indicated for the treatment of chronic or acute cardiac failure, with promising results [
15,
16], and indications have already extended to septic and toxic cardiac depression [
17‐
23]. If our experimental data apply to the clinical setting, LEVO pretreatment may also be an option to support the cardiovascular system during hypoxemia, without fueling VO
2, without aggravating systemic anaerobiosis markers, and without further compromising the regional gastromucosal oxygenation. Further studies will have to extend these experimental results to other hypoxia models and ultimately to the clinical setting.