Comparing the Effects of Electronic Cigarette Vapor and Cigarette Smoke in a Novel In Vivo Exposure System

Summary

This protocol describes a method for exposing rodents to electronic cigarette vapor (E-vapor) and cigarette smoke. Exposure chambers are constructed by modifying anesthesia chambers with an automated pumping system that delivers E-vapor or cigarette smoke to rodents. This system can easily be modified to accommodate many experimental endpoints.

Abstract

Electronic cigarettes (E-cigarettes) are being widely used, and growing in popularity. It is estimated that more than 9 million adults use them regularly. The potential adverse health effects of electronic cigarette vapor (E-vapor) exposure are poorly defined. While several animal models of E-vapor exposure have been developed, few models expose rodents to clinically relevant quantities of nicotine and make direct comparisons to cigarette smoke within the same exposure system. Here, we present a method for constructing and operating an E-vapor chamber and cigarette smoke chamber. The chambers are constructed by outfitting anesthesia chambers with a computer controlled pumping system that delivers consistent amounts of E-vapor or cigarette smoke to rodents. Nicotine exposure is measured indirectly by quantifying pre and post-exposure serum cotinine levels. This exposure system can be modified to accommodate various types of E-cigarettes and tobacco cigarettes, and can be used to compare the effects of E-vapor and cigarette smoke in vivo.

Introduction

Since entering the US market in 2004, electronic cigarettes (E-cigarettes) have expanded into a billion-dollar industry, and it is estimated that nearly 9 million adults use them regularly¹. In 2014 and 2015, more high school students had used E-cigarettes than conventional cigarettes². The growing number of E-cigarettes users has spawned a research effort to evaluate their potential adverse health effects.

E-cigarettes generate a vapor (dubbed "E-vapor") by heating a viscous solution that typically contains a mixture of water, polyethylene glycol or vegetable glycerin, nicotine, and flavorings^3,4. It has been shown that E-vapor contains several harmful compounds including Reactive Oxygen Species (ROS), nicotine, various aldehydes, and polycyclic aromatic hydrocarbons^5,6. Many of these compounds are formed during the vaporization process of E-liquid prior to inhalation⁷. Notably, several of these harmful compounds are also present in cigarette smoke, raising concern that E-cigarettes use may have similar adverse health consequences⁷.

There is little consensus on the health effects of E-cigarettes. To address this, several animal models of E-vapor exposure have been developed (Table 1). These models employ a variety of methods such as whole-body E-vapor exposure and mechanical ventilation. While current models have provided insightful data, few make direct comparisons to cigarette smoke within the same exposure system (Table 1). Additionally, while several human studies have shown E-cigarettes users and cigarette smokers to have serum cotinine levels between 30-200 ng/mL, many models of E-vapor and cigarette smoke exposure fall outside this range^8,9,10,11,12.

Herein we present a method for comparing the effects of cigarette smoke and E-vapor exposure in vivo that yields serum cotinine levels similar to human studies.

Protocol

The following protocol has been performed under the guidance and approval of the University of Michigan Institutional Animal Care and Use Committee (IACUC).

1. Electronic Cigarette-vapor Chamber Assembly

NOTE: The complete chamber should be placed in a fume hood during use. The chamber here was housed in a temperature controlled and filtered laboratory environment. Investigators may elect to monitor such aspects of the system to ensure consistency of the room air quality. As an option, covering the monitors with a metal cage can prevent rodent tampering while allowing the monitors to sample the interior chamber environment. 

1. Acquire an anesthesia chamber with air tight removable lid with volume of 20 L.
2. Using a jig saw fitted with a blade appropriate for cutting the material, cut a 10.2 cm diameter hole in the lid of the chamber approximately 7.6 cm from the back edge of the chamber.
3. Insert the adjustable vent into the hole and mount into place with any caulk adhesive.
   NOTE: Ensure that the adhesive caulk is not accessible to the rodents in the chamber, as they may chew the caulk. To prevent this possible issue, apply the caulk to the outside of the chamber wall to mount the vent.
4. Cut silicone tubing into two 15 cm segments, and attach ends to either side of a T-connector.
   NOTE: Silicone tubing has the potential to react with some components of e-vapor or cigarette smoke. Thus, investigators may consider using non-reactive tubing.
5. Thread both of the silicone tubes through premade holes near the front of the chamber lid so that the T-connector is inside the chamber. Ensure that the tubing is secured to the lid with either adhesive caulk or electrical tape.
6. Connect the free ends of the silicone tubing to the output ends of two micro air pumps. Pumps should be mounted to the lid of the chamber with double-sided adhesive tape or caulk.
   NOTE: The length of tubing connected to the output end of the pump should be short to limit the amount of vapor collection on the inside surface of the tubing during use.
7. With a new silicone tube, attach one end to the input side of one of the air pumps (Pump A in Figure 1), and cut this tube to approximately 4 cm in length. This is where the electronic cigarette will be inserted during chamber use. Ensure that the diameter of the tube allows for a snug fit around the end of the e-cig.
8. With a new silicone tube, attach one end to the input side of the other air pump (Pump B in Figure 1). This pump will introduce room air into the chamber. As such, the end of the tube must be placed outside the fume hood. The length of this tube is not critical, but should be as short as possible to limit airflow resistance.
9. Inside the chamber attach two small hooks with double-sided adhesive to hold oxygen and carbon monoxide gas monitors.

Figure 1. Schematic of Electronic Cigarette-vapor Chamber.
Chamber is housed in fume hood (not shown). Room air pump (Pump B) introduces room air from outside the fume hood into chamber continuously at 2 L/min. E-cig pump (Pump A) puffs 133 mL of E-vapor over 4 s, with a 30 s rest interval. E-vapor and room air mix prior to being pumped into chamber. Gas monitors continuously measure carbon monoxide (CO) and oxygen (O₂) concentrations inside the chamber. E-vapor is exhausted passively through vent into fume hood. Please click here to view a larger version of this figure.

2. Cigarette Smoke-chamber Assembly

NOTE: Virtually any brand of cigarette can be used with this system, however standardized research cigarettes such as the University of Kentucky 1R6F Research Cigarette are cost-effective, reliable, and best for this application.

1. Follow steps 1.1 - 1.6, & step 1.9.
2. With a new silicone tube, attach one end to the cigarette lighting device, and the other end to the input side of the air pump (Pump A in Figure 2). The cigarette lighting device should be placed inside the fume hood and outside the chamber during use.
   Note: Construction of the cigarette lighting device requires knowledge of metal fabrication and electrical engineering. While a step-by-step guide to construction will not be given here, see supplementary materials for plans.
3. With a new silicone tube, attach one end to the other air pump (Pump B in Figure 2). This pump will introduce room air into the chamber, thus the end of the tube must be placed outside the fume hood.
4. Cut several 5 mm wide vertical slits in the front wall of the chamber, and mount a computer fan on the outside of the chamber so that it covers this opening. Ensure that the front of the fan is facing towards the chamber such that the fan will blow air into the chamber through this opening.

Figure 2. Schematic of Cigarette-smoke Chamber.
Room air pump (Pump B) introduces room air from outside the fume hood into chamber continuously at 2 L/min. Pump A draws on lit cigarette for 40 s with rate of 2 L/min, and 20 s later the computer fan evacuates the chamber over 3 min. Smoke and room air mix prior to being pumped into chamber. Gas monitors continuously measure carbon monoxide (CO) and oxygen (O₂) chamber concentrations. Smoke is exhausted through vent into fume hood. Please click here to view a larger version of this figure.

3. Microcontroller Assembly and Software

1. Control the pumping system of the E-cigarette vapor chamber and cigarette smoke chamber by separate microcontrollers. Download the microcontroller software and upload the operating codes provided in the Supplementary Materials. The electronic cigarette vapor code will run the room air pump continuously and activate the E-cigarette pump for a 4 s duration every 30 s. The cigarette smoke code will run the room air pump continuously, activate the cigarette pump for 40 s, and activate the computer fan 20 s after the cigarette pump has stopped. The fan will shut off after running for 3 min.
   Note: The timing of the pumps and fan can be adjusted as needed. Reference manufacturer instructions on how to upload relevant codes to the microcontroller.
2. To assemble the microcontroller, connect zip wires, diodes, resisters, and capacitors to the bread board as depicted in Figure 3 and attach alligator-clip wires to the corresponding air pumps (and computer fan for cigarette smoke chamber). House the microcontroller outside of the fume hood if possible.

Figure 3. Schematic of Microcontroller.
Schematic of microcontroller and bread board to operate timing of air pumps and fan. Please click here to view a larger version of this figure.

4. Animals

1. Use adult rats weighing 450 - 520 g.
2. Group rats according to exposure type (e.g., electronic cigarette, cigarette smoke, room air pumped into chamber).
3. At this time prior to exposure, collect 500 µL of blood in EDTA coated tubes from tail vein using syringe to measure baseline serum cotinine concentration.
4. Spin down blood samples at 20,000 x g for 30 min at 4 ˚C and collect serum. Ensure that samples are chilled on ice throughout this process.
5. Following the manufacturer protocol, assay for cotinine in the serum samples collected. Samples may also be stored at -80 ˚C for later use.

5. Operating the Electronic cigarette Chamber

1. Clean the inside of the chamber with 70% ethanol, then with deionized water, and let air dry until the chamber is completely dry (or about 30 min).
2. Calibrate gas monitors and mount entire monitor on the wall inside the chamber.
3. Place rats inside the chamber. Note that up to three animals can be exposed simultaneously.
4. Ensure the E-cigarette is fully charged with adequate E-liquid and insert the E-cigarette  into input tube. It is critical to ensure that the E-cigarette battery and E-liquid levels are adequate throughout the duration of the 90-min exposure.
5. Turn the air pumps on, and start the timer.
6. During exposure observe the gas monitors to ensure chamber contains >20% O₂ and 0 ppm CO.
   Note: If oxygen levels fall, the chamber may not be well ventilated or the oxygen monitor may not be appropriately calibrated.
7. Once the exposure time has reached 90 min, remove the E-cigarette and continue to run the gas pumps to vent the remaining vapor. Additionally, the top of the chamber can be lifted to hasten ventilation.
8. Once the vapor has cleared, remove the rats and clean the chamber.
9. Collect 500 µL blood from tail vein from each rat approximately 1 h after exposure at the conclusion of the experimental protocol.
10. Follow steps 4.4 - 4.5 to isolate serum and assay for cotinine.

6. Operating the Tobacco Cigarette Chamber

1. Follow steps 5.1 - 5.3.
2. Insert cigarette into cigarette lighting device, with the end of the cigarette against the heating elements.
3. Turn on the cigarette lighting device until cigarette butt begins to smolder (about 5 s).
4. Once the cigarette is lit, turn on the pumping system, start the timer, and observe the cigarette burn to completion (about 40 s).
5. Once the cigarette has burned, carefully remove the spent cigarette from the cigarette lighting device with forceps.
6. Ensure that CO levels do not rise above 1000 ppm and O₂ levels do not fall below 20%. Computer fan timing and duration is critical in preventing carbon monoxide accumulation.
7. After 4 min turn the pumping system off and return to step 6.2 until rats are exposed to tobacco smoke for 90 min (or approximately 23 cigarettes).
   NOTE: Carbon monoxide levels 4 min following cigarette burning should fall below 400 ppm, otherwise carbon monoxide may begin to accumulate in chamber.
8. When exposure is complete, continue to leave the pumping system on to ventilate residual smoke. When carbon monoxide falls below 100 ppm remove rats from chamber. This should take 5 - 10 min.
9. Remove rats and clean the chamber.
10. Collect 500 µL blood from tail vein approximately 1 h after exposure at the conclusion of the experimental protocol as with the E-cigarettes.
11. Follow steps 4.4 - 4.5 to isolate serum and assay for cotinine.

Representative Results

Carbon monoxide and oxygen monitoring

Oxygen concentrations did not fall below 20% during e-vapor exposure and CO concentrations remained undetectable throughout exposure. Gas monitors during cigarette smoke exposure indicated that oxygen concentration remained above 20%. Carbon monoxide concentrations did not exceed 1,000 ppm (Figure 4).

Figure 4: Carbon Monoxide Concentrations in cigarette-smoke Chamber. Carbon monoxide concentration was recorded every 30 s over the course of introducing smoke from 1R6F cigarettes. Results shown are averages from 3 consecutive 4 min cycles. Carbon monoxide concentrations did not exceed 1,000 ppm. The cigarette is burned to completion over 40 s, and the fan is activated 20 s later (i.e. fan is activated 1 min following cigarette ignition).

Pre- and Postexposure Serum Cotinine

Pre-exposure and 1 h postexposure serum cotinine for E-vapor group (n = 3) was 4.2 ±0.4 ng/mL and 171.6 ±20.5 ng/mL, respectively. Pre-exposure and 1 h postexposure serum cotinine for cigarette smoke group (n = 3) was 3.9 ±0.3 ng/mL and 98.8 ±2.1 ng/mL, respectively (Figure 5).

Figure 5: Serum Cotinine Levels Following Cigarette-smoke or Electronic Cigarette-vapor Exposure. Serum cotinine was measured prior to protocol initiation, and 1 h after a 90 min exposure session. Pre-exposure and 1 h post-exposure serum cotinine for e-vapor group was 4.2 ±0.4 ng/mL and 171.6 ±20.5 ng/mL, respectively. Pre-exposure and 1 h postexposure serum cotinine for cigarette smoke group was 3.9 ±0.3 ng/mL and 98.8 ±2.1 ng/mL, respectively. Difference between pre- and postexposure serum cotinine concentrations were statistically significant. *P <0.05.

Figure 6: Electronic Cigarette-vapor Chamber and Cigarette Smoke-chamber. Image of the electronic cigarette vapor (right) and cigarette smoke chamber (left) within the fume hood. Red boxes contain microcontrollers. Please click here to view a larger version of this figure.

Animal model		Electronic cigarette		Tobacco cigarette		Reference
Exposure method	Model organism	Brand (nicotine)	Cotinine ng/mL (serum, [urine])	Brand	Cotinine ng/mL (serum, [urine])
whole-body exposure	C57BL/6J mice	Joytech 510-T (1.8%)	62.3 ±3.3, [892.5 ±234]	N/A	N/A	McGrath-Morrow
mechanical ventilator	BALB/cJ mice	not reported	[400 - 500]	not reported	[500 - 800]	Ponzoni
whole-body exposure	CD-1 mice	multiple* (0.6 - 24%)	not reported	N/A	N/A	Hwang
whole-body exposure	Wistar albino rats	Ego T (0.9%)	not reported	not reported	not reported	Salturk
whole-body exposure	C57BL/6 mice	NJOY (1.8%)	267 ±17	N/A	N/A	Sussan
whole-body exposure	C57BL/6J mice	CoolCart, Vapor Titan	500 ±10	3R4F Reference Cigarettes	76 ±7.6	Husari
*Xtreme Vaping, Vapure, Vape Addict Juice, Grimm Creations, Green Smart Living, Free Masons Elixer

Table 1: Characteristics of Electronic Cigarette Exposure Models.

Discussion

Here we describe a method for constructing chambers that expose rodents to E-vapor and cigarette smoke in a controlled fashion (Figure 6). Construction of the E-cigarette chamber is relatively simple and inexpensive compared to commercial exposure systems^14,15,16. The parts and tools required to build the chamber are readily available from commercial suppliers online. Similarly, constructing the cigarette smoke chamber is relatively simple with the exception of the cigarette lighting device which must be fabricated (see Supplementary Materials for plans).

Once the chambers are constructed, a critical step of the exposure system is calibrating the chambers to expose the rodents to the desired amount of nicotine. In both the E-cigarette chamber and the cigarette chamber, adjusting the amount of total exposure time is perhaps the easiest method for increasing or decreasing the amount of nicotine exposure. Increasing the puff time in the E-cigarette exposure system may increase the nicotine dose, however drawing vapor from the E-cigarette for an extended length of time has been shown to increase the levels of ROS, aldehydes, and other hazardous compounds, and may or may not reflect the typical habits of an E-cigarette user⁵. The puff duration and total exposure time can be adjusted by modifying the code uploaded to the microcontroller. Also, it should be noted that the concentration of nicotine in E-cigarette solutions, as well as the voltage of the E-cigarette heating element, can vary significantly and should be taken into account when calibrating the system.

One of the greatest advantages of this exposure system is its versatility. Virtually any brand of e-cig or e-cig solution can be used with this system. This is an especially useful feature given that the E-cigarette market now includes over 400 brands and thousands of E-cigarette solutions¹³. Additionally, the exposure system is compatible with multiple experimental endpoints allowing for the effects of E-cigarette on various organ systems and disease processes to be studied. We also acknowledge that there are several limitations to this exposure paradigm, such as the method by which the animals are exposed to the vapor. E-cigarette users directly inhale E-vapor while in this paradigm the rodents inhale E-vapor passively. Additionally, the rodents will also likely absorb compounds within the vapor or smoke by other routes (i.e. direct dermal absorption, and ingestion while preening). However, we think that the benefits of the exposure system far outweigh the limitations.

Overall, this exposure paradigm delivers consistent and clinically relevant E-vapor and cigarette smoke exposure, and may help aid the research effort in determining the adverse health effects of E-cigarette and cigarette smoke.

Materials

Name	Company	Catalog Number	Comments
blu PLUS Rechargeable Kit	blu eCigs	N/A
1R6F Reference Cigarettes	Center for Tob Ref  Prod UK	N/A
Lexan Anesthesia Chamber 20 L	Jorgensen Laboratories	JOR265
Arduino UNO	Arduino	2877
Diode Rectifier - 1 A; 50 V	Spark Fun	COM-08589
Resistor 10 KOhm 1/6th W PTH - 20 pack	Spark Fun	COM-11508
Electrolytic Decoupling Capacitors - 100 uF/25 V	Spark Fun	COM-00096
Solderless Plug-in BreadBoard	BusBoard Prototype Systems	BB400
Alligator-Clip Wires	BusBoard Prototype Systems	CA-M-20
ZipWire	BusBoard Prototype Systems	ZW-MM-10
Standard Fan 80 ST2	Cooler Master	R4-S8R-20AK-GP
ARIC 4" adjustable vent	Bestlouver	N/A
ToxiPro  Carbon Monoxide (CO) Monitor	Honeywell Analytics	54-00-10316
ToxiPro Oxygen (O2) Monitor	Honeywell Analytics	54-45-90-VD
ToxiPro IQ Express Docking Station	Honeywell/Sperian Biosystems	54-46-9100
Command Wall Hook Small Wire 6-Pack	3M	N/A
Micro Water/Air Pump	Xiamen Conjoin Electronics	CJWP40-A12A1
1/4" Silicon Tubing	NewAge	2801470-100
T Connector	Bel-Art Scienceware	F196060000
Plastic Whole Blood tube with spray-coated K2EDTA	Becton, Dickinson and Company	367841
Cotinine ELISA kit	Calbiotech	CO096D