Bronchoalveolar Lavage and Oleic Acid-Injection in Pigs as a Double-Hit Model for Acute Respiratory Distress Syndrome (ARDS)

Summary

Different, complex animal models exist to study the pathophysiology of acute respiratory distress syndrome (ARDS). Bronchoalveolar lavage and oleic acid injection induced lung injury is suitable as a new double-hit animal model for studying the acute respiratory distress syndrome.

Abstract

The treatment of ARDS continues to pose major challenges for intensive care physicians in the 21st century with mortality rates still reaching up to 50% in severe cases. Further research efforts are needed to better understand the complex pathophysiology of this disease. There are different well-established animal models to induce acute lung injury but none has been able to adequately mimic the complex pathomechanisms of ARDS. The most crucial factor for the development of this condition is the damage to the alveolar capillary unit. The combination of two well-established lung injury models allow us to mimic in more detail the underlying pathomechanism. Bronchoalveolar lavage (BAL) leads to surfactant depletion as well as alveolar collapse. The repeated instillation of fluid volumes causes subsequent hypoxemia. Surfactant depletion is a key factor of ARDS in humans. BAL is often combined with other lung injury approaches, but not with a second hit followed by oleic acid injection (OAI) yet. Oleic acid injection leads to severely impaired gas exchange, a deterioration of lung mechanics and disruption of the alveolo-capillary barrier. The OAI mimics most of the expected effects of ARDS consisting of extended inflammation of lung tissue with an increase of alveolar leakage and gas exchange impairment. A disadvantage of the combination of different models is the difficulty to determine the influence to the lung injury caused by BAL alone, OAI alone or both together. The model presented in this report represents the combination of BAL and OAI as a new double-hit lung injury model. This new model is easy to implement and an alternative to study different therapeutic approaches in ARDS in the future.

Introduction

Acute respiratory distress syndrome (ARDS) is a disease consisting of impaired gas exchange and lung infiltration, which often needs intensive care therapy. The mortality of severe ARDS remains high (up to 50%) worldwide despite almost 50 years of extensive research¹. The ARDS is defined by the Berlin Definition, including diagnostic criteria as timing, chest imaging, origin of edema and hypoxemia². To better categorize patients with different levels of ARDS severity, three different degrees of hypoxemia are defined: mild (200 mmHg < PaO₂/FIO₂ ≤ 300 mmHg), moderate (100 mmHg < PaO₂/FIO₂ ≤ 200 mmHg), and severe (PaO₂/FIO₂ ≤ 100 mmHg)². Different animal models with a focus on lung injury are widely used and accepted to examine the pathophysiological changes and different therapeutic approaches in ARDS³.

Animal models using endotoxins (e.g., intravenous infusion of bacteria, cecal ligation and puncture to mimic a sepsis-induced lung injury), ischemia/reperfusion models, smoke/burn ARDS models, infusion of oleic acid and bronchoalveolar lavage models are known³. Each model represents only a few pathophysiological changes with advantages and disadvantages to the study results³. This does not reflect the complexity of the ARDS disease. The combination of two proven models allows better conclusions about the pathophysiology of ARDS. In the presented model, we combined bronchoalveolar lavage and oleic acid infusion to mimic the complexity of the human ARDS. Oleic acid is an unsaturated fatty acid and acts directly on the alveolo-capillary unit of the lungs by triggering activation of innate immune receptors subsequently causing neutrophil accumulation, proinflammatory cytokine production and cell death^4,5. Oleic acid infusion induces severe hypoxemia, increases in pulmonary arterial pressure and accumulation of extravascular lung water. Hypotension and myocardial depression due to right ventricular failure often occur. The induction of lung injury by repeated bronchoalveolar lavage (BAL) with balanced electrolyte solution reduces the alveolar surfactant lipid concentration³. Surfactants decrease alveolar surface tension and prevent alveolar collapse. BAL causes immediate hypoxemia and an increase of the alveolar-arterial oxygen difference³. Human ARDS is also associated with depletion of surfactant³. The disadvantages of this combined model are the necessity for central venous access, intubation and general anesthesia. Furthermore, the questionable mechanistic relevance (e.g., the oleic acid infusion) for translational aspects remains unclear. At least, it is difficult to determine which part of the lung injury (BAL vs. OAI, or both together) contributes to lung damage. The advantages of this model are its usability in large animals with familiar monitoring and instrumentation similar to human patients (no special equipment required), the good reproduction of the main aspects of ARDS and the possibility to study isolated ARDS without systemic inflammation (e.g., endotoxin models). In the following article, we give a detailed description of the double-hit (BAL and OAI) lung injury in pigs and provide representative data to characterize the stability of the compromises in lung function.

Protocol

All animal experiments described here have been approved by the institutional and state animal care committee (Landesuntersuchungsamt Rheinland-Pfalz, Koblenz, Germany; approval number G18-1-044) and were conducted in accordance with the guidelines of the European and German Society of Laboratory Animal Sciences.

1. Anesthesia, intubation and mechanical ventilation

1. Withhold food for 6 hours before anesthesia to reduce the risk of aspiration, but allow free access to water to reduce stress.
2. Inject a combination of ketamine (4 mg∙kg^-1) and azaperone (8 mg∙kg^-1) intramuscularly for sedation while the animal is in the animal box.
3. Establish a venous line with a common peripheral venous catheter (20 G) in an ear vein after local disinfection with alcohol.
4. Start monitoring the peripheral oxygen saturation (SpO₂) by clipping the sensor onto one of the ears or the tail of the animal.
5. Inject fentanyl (4 µg∙kg^-1), propofol (3 mg∙kg^-1) and atracurium (0.5 mg∙kg^-1) for induction of anesthesia.
6. Place the pig in a supine position on the stretcher.
7. Ventilate the pig with a mask suitable for animals with a peak inspiratory pressure below 20 cmH₂O, a PEEP of 5 cmH₂O, a frequency of 14-16 /min and a FiO₂ of 1.0.
8. Start a continuous infusion with balanced electrolyte solution (5 mL∙kg^-1∙h^-1), propofol (8-12 mg∙kg^-1∙h^-1) and fentanyl (0.1-0.2 mg∙kg^-1∙h^-1) to maintain anesthesia.
9. For the intubation, use a common endotracheal tube suitable for the animal (e.g., weight of 25-30 kg, endotracheal tube ID 6-7) armed with endotracheal tube introducer, and a common laryngoscope with a Macintosh Blade 4. Two people are necessary.
   1. Person 1: Pull out the tongue with one hand and press the snout down with the other.
   2. Person 2: Insert the laryngoscope and advance it as usual until the epiglottis can be visualized.
10. Pull the laryngoscope upwards to visualize the vocal cords. Sometimes the epiglottis “sticks” to the soft palatine. If so, mobilize it with the tip of the tube.
11. Insert the tube through the vocal cords and pull out the introducer.
12. Block the balloon of the tube.
13. Connect the tube to the ventilator and check correct positioning with capnography and auscultation.
14. Start mechanical ventilation (tidal volume 6-8 mL/kg, PEEP 5 cmH₂O, FiO₂ 0.4, frequency to keep etCO₂ between 35 – 45 mmHg).

2. Instrumentation

1. Retract the hind legs with bandages for catheterizing necessary vessels. An arterial line, an arterial introducer sheath, a central venous line and a venous introducer sheath for pulmonary artery catheter placement are necessary.
2. Generously disinfect the femoral area with alcoholic disinfection. Depending on the planned examinations, a more or less aseptic approach is used.
3. Prepare catheters by flushing them with saline.
4. Place the ultrasound probe on the inguinal ligament and scan for femoral vessels.
5. Turn the probe 90° to fully visualize the femoral arteria in the long axis. If necessary, it is also possible in different circumstances to use the short axis view to fully visualize the femoral arteria.
6. Cannulate the femoral arteria under in-line ultrasound visualization with the needle of the introducer set in Seldinger’s technique. When pulsating bright blood flows out, introduce the guidewire and retract the needle.
7. Visualize the femoral vein and cannulate the vein under in-line ultrasound visualization and continuous aspiration with the needle of the introducer set. When venous blood is aspirable, disconnect the syringe and insert the guidewire. Retract the needle.
8. Check position of the wires with ultrasound.
9. Insert the arterial and the venous line over the placed guidewires.
10. Repeat arterial and venous punctuation on other side and insert the introducer sheaths per Seldinger´s technique as described above.
11. Connect the arterial line and the venous line each to a transducer.
12. Position both transducers at heart level and switch the three-way stopcocks of both transducers open to the atmosphere to calibrate the system to zero.
    NOTE: It is necessary to avoid any air bubbles and bloodstains in the system to generate plausible values.
13. Switch infusion of propofol and fentanyl to one of the ports of the central venous line.
14. Calibrate the probe for ultrafast pO₂-measurements and insert it through the arterial introducer sheath.
    NOTE: The measurement of pO₂ with the probe for ultrafast pO₂-measurement is not obligatory but helps visualizing the real-time changes in pO₂.

3. Inserting pulmonary artery catheter

1. Check the balloon of the pulmonary artery catheter (PAC) for damage.
2. Connect to the transducer and calibrate it.
3. Insert the PAC through the introducer sheath (balloon deflated).
4. When the PAC has passed through the introducer sheath (15-20 cm), inflate the balloon.
5. Advance the PAC and monitor the typical waveforms (venous vessels, right atrium, right ventricle, pulmonary arteria, pulmonary capillary wedge pressure). Deflate the balloon and check if blood can be aspirated through all ports of the PAC.

4. Induction of lung injury: first hit by bronchoalveolar lavage

1. Prepare sterile balanced electrolyte solution (e.g., Sterofundin) warmed to 40 °C.
   NOTE: Sterile balanced electrolyte solution is used to avoid pulmonary pollution.
2. Change the FiO₂ from 0.4 to 1.0 over 10 min before performing the bronchoalveolar lavage.
3. Start the ultrafast pO₂-measurement.
4. Prepare norepinephrine for continuous infusion and for bolus injection (if mean arterial pressure < 60 mmHg). Connect the norepinephrine syringe pump to one of the ports of the central venous catheter without starting it.
5. Fill 30 mL∙kg^-1 from the warmed sterile balanced electrolyte solution into a funnel. Check that the funnel can be connected to the endotracheal tube.
6. Disconnect the tube without PEEP loss in inspiration from the ventilator.
7. Connect the funnel to the endotracheal tube.
8. Raise the funnel 1 m above the animal manually.
9. Open the cap and instill the entire amount of the warmed balanced electrolyte solution from the funnel into the endotracheal tube over 30 s by using the hydrostatic pressure.
10. After 30 s, remove the infused solution by lowering the funnel 1 meter below the animal and drain the lavage fluid passively. Reconnect the animal to the ventilator for oxygenation.
11. Collect the removed lavage fluid and note the amount. It is needed to calculate the alveolar fluid clearance.
    NOTE: Do not reuse the balanced electrolyte solution after a lavage to maximize surfactant wash out.
12. Aspirate the remainders of the solution in the tube by using suction catheters.
13. Closely monitor hemodynamics after the bronchoalveolar lavage and keep norepinephrine at hand. If necessary, give norepinephrine as bolus or continuous infusion to stabilize blood pressure (compare to step 4.4).
14. Repeat infusion of 30 mL∙kg^-1 balanced electrolyte solution as described in the steps 4.5-4.13 until PaO₂/FiO₂-ratio is below 250 mmHg. Four to five repetitions of the bronchoalveolar lavage may be necessary.
15. If PaO₂/FiO₂-ratio is lower than 250 mmHg, start with the induction of lung injury by oleic acid injection. Do not change the ventilator settings during this procedure.

5. Induction of lung injury: second hit by oleic acid injection

1. Prepare oleic-acid solution: 0.1 mL∙kg^-1 of oleic acid in a 20 mL syringe and connect it to a 3-way-stopcock. Take 2 mL of blood in another 20 mL syringe. Add saline to a total volume of 20 mL in both syringes and connect the second syringe also to the 3-way-stopcock.
   CAUTION: Use gloves and eye protection when working with oleic acid.
2. Prepare norepinephrine for continuous infusion and for bolus injection (if mean arterial pressure < 60 mmHg). Connect the norepinephrine syringe pump to one of the ports of the central venous catheter without starting it.
3. Continue to monitor the ultrafast pO₂-measurement that still measuring. FiO₂ is still 1.0.
4. Connect the 3-way-stopcock to the proximal port of the PAC.
5. Mix the oleic acid and the blood/saline mixture thoroughly by repeated shifting of the solution from one syringe to the other syringe and vice versa via the three-way-stopcock and keep mixing all the time. When it is a homogenous emulsion, inject 2 mL of the emulsion and continue mixing.
   NOTE: If mixing stops, the emulsion may separate into a lipophilic and a hydrophilic part.
6. Closely monitor hemodynamics after injection of oleic acid and keep norepinephrine at hand. If necessary, give norepinephrine as bolus or continuous infusion to stabilize blood pressure (compare to step 5.2).
   NOTE: Be vigilant; the animals can die during this procedure.
7. Repeat injection of 2 mL of the solution every 3 min until PaO₂/FiO₂-ratio is below 150 mmHg.
8. If the syringe is empty before PaO₂/FiO₂-ratio is between 100 and 200 mmHg, prepare 2 more syringes as described in step 5.1. Repeat the steps 5.5-5.8 until the PaO₂/FiO₂-ratio falls between 100 and 200 mmHg.
   NOTE: A half to full syringe of the oleic acid and the blood/saline mixture is usually required.
9. If the PaO₂/FiO₂-ratio is between 100 and 200 mmHg, wait 30 min and check again. If it is consistently below 200 mmHg, start the experiment/treatment; otherwise prepare 2 more syringes as described in step 5.1 and repeat steps 5.5-5.9.
   NOTE: After induction of lung injury as described, the impairment of lung function can remain stable or deteriorate or even improve within certain limits.

6. End of experiment and euthanasia

1. Inject 0.5 mg of fentanyl additionally to the continuous anesthesia and wait 5 min. Inject 200 mg of propofol and 40 mmol of potassium chloride to kill the animal in deep anesthesia.

Results

The PaO₂/FiO₂-ratio decreases after bronchoalveolar lavage and fractionated application of oleic acid (Figure 1). Because it is unclear to predict the impact of bronchoalveolar lavage (e.g., the impact of fractionated oleic acid dose) on PaO₂/FiO₂-ratio, it is recommended to monitor PaO₂/FiO₂-ratio while inducing the lung injury. Ultrafast pO₂-measurement allows to monitor PaO₂ in real-time and is well es...

Discussion

The described double-hit method to cause a severe lung injury in pigs is suitable to study different treatment options in ARDS. The double-hit model mimics two central elements of the pathomechanism of ARDS: loss of the alveolar-capillary unit and disruption of the endothelial barrier⁷. Due to the two hits, it is important to have a study protocol with predefined target values (e.g., PaO₂/FiO₂-ratio).

The main disadvantage of this double-hit method...

Materials

Name	Company	Catalog Number	Comments
1 M Kaliumchlorid-Lösung 7.46% 20 mL	Fresenius, Kabi Deutschland GmbH	potassium chloride
Absaugkatheter Ideal CH14, 52 cm, gerade	B. Braun Melsungen AG, Germany	suction catheter
Arterenol 1 mg/mL, 25 mL	Sanofi- Aventis, Seutschland GmbH	norepinephrine
Atracurium Hikma, 50 mg/5 mL	Hikma Pharma GmbH , Martinsried	atracurium
BD Discardit II Spritze 2, 5, 10, 20 mL	Becton Dickinson S.A. Carretera Mequinenza Fraga, Spain	syringe
BD Luer Connecta	Becton Dickinson Infusion Therapy AB Helsingborg, Schweden	3-way-stopcock
BD Microlance 3 20 G	Becton Dickinson S.A. Carretera Mequinenza Fraga, Spain	canula
Datex Ohmeda S5	GE Healthcare Finland Oy, Helsinki, Finland	hemodynamic monitor
Engström Carestation	GE Heathcare, Madison USA	ventilator
Fentanyl-Janssen 0.05 mg/mL	Janssen-Cilag GmbH, Neuss	fentanyl
Führungsstab, Durchmesser 4.3	Rüsch	endotracheal tube introducer
Incetomat-line 150 cm	Fresenius, Kabi Deutschland GmbH	perfusorline
Ketamin-Hameln 50 mg/mL	Hameln Pharmaceuticals GmbH	ketamine
laryngoscope	Rüsch	laryngoscope
logicath 7 Fr 3-lumen 30 cm lang	Smith- Medical Deutschland GmbH	central venous catheter
Masimo Radical 7	Masimo Corporation Irvine, Ca 92618 USA	periphereal oxygen saturation
Neofox Oxygen sensor 300 micron fiber	Ocean optics Largo, FL USA	ultrafast pO2-measurements
Ölsäure reinst Ph. Eur NF C18H34O2 M0282.47g/mol, Dichte 0.9	Applichem GmbH Darmstadt, Deutschland	oleic acid
Original Perfusor syringe 50 mL Luer Lock	B.Braun Melsungen AG, Germany	perfusorsyringe
PA-Katheter Swan Ganz 7.5 Fr, 110 cm	Edwards Lifesciences LLC, Irvine CA, USA	PAC
PE-Trichter, 60 mm	Aquintos-Wasseraufbereitung GmbH, Germany	funnel
Percutaneous sheath introducer set 8.5 und 9 Fr, 10 cm with integral haemostasis valve/sideport	Arrow international inc. Reading, PA, USA	introducer sheath
Perfusor FM Braun	B.Braun Melsungen AG, Germany	syringe pump
Propofol 2% 20 mg/mL (50 mL Flaschen)	Fresenius, Kabi Deutschland GmbH	propofol
Radifocus Introducer II, Größe 5-8 Fr	Terumo Corporation Tokio, Japan	introducer sheath
Rüschelit Super Safety Clear 6.5 /7.0	Teleflex Medical Sdn. Bhd, Malaysia	endotracheal tube
Seldinger Nadel mit Fixierflügel	Smith- Medical Deutschland GmbH	seldinger canula
Sonosite Micromaxx Ultrasoundsystem	Sonosite Bothell, WA, USA	ultrasound
Stainless Macintosh Größe 4	Welsch Allyn69604	blade for laryngoscope
Sterofundin Infusion	B. Braun Melsungen AG, Germany	bronchoalveolar lavage
Stresnil 40 mg/mL	Lilly Deutschland GmbH, Abteilung Elanco Animal Health	azaperon
Vasofix Safety 22 G	B.Braun Melsungen AG, Germany	venous catheter