Activity of Cardiorespiratory Networks Revealed by Transsynaptic Virus Expressing GFP

Mustapha Irnaten,1 Robert A. Neff,1 Jijiang Wang,1 Arthur D. Loewy,2 Thomas C. Mettenleiter,3 and David Mendelowitz1

 1Department of Pharmacology, George Washington University, Washington, DC 20037;  2Department of Anatomy and Neurobiology, Washington University School of Medicine, St. Louis, Missouri 63110; and  3Federal Research Centre for Virus Diseases of Animals, Institute of Molecular Biology, Friedrich-Loeffler Institutes, D-17498 Insel Riems, Germany


    ABSTRACT
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Irnaten, Mustapha, Robert A. Neff, Jijiang Wang, Arthur D. Loewy, Thomas C. Mettenleiter, and David Mendelowitz. Activity of Cardiorespiratory Networks Revealed by Transsynaptic Virus Expressing GFP. J. Neurophysiol. 85: 435-438, 2001. A fluorescent transneuronal marker capable of labeling individual neurons in a central network while maintaining their normal physiology would permit functional studies of neurons within entire networks responsible for complex behaviors such as cardiorespiratory reflexes. The Bartha strain of pseudorabies virus (PRV), an attenuated swine alphaherpesvirus, can be used as a transsynaptic marker of neural circuits. Bartha PRV invades neuronal networks in the CNS through peripherally projecting axons, replicates in these parent neurons, and then travels transsynaptically to continue labeling the second- and higher-order neurons in a time-dependent manner. A Bartha PRV mutant that expresses green fluorescent protein (GFP) was used to visualize and record from neurons that determine the vagal motor outflow to the heart. Here we show that Bartha PRV-GFP-labeled neurons retain their normal electrophysiological properties and that the labeled baroreflex pathways that control heart rate are unaltered by the virus. This novel transynaptic virus permits in vitro studies of identified neurons within functionally defined neuronal systems including networks that mediate cardiovascular and respiratory function and interactions. We also demonstrate superior laryngeal motorneurons fire spontaneously and synapse on cardiac vagal neurons in the nucleus ambiguus. This cardiorespiratory pathway provides a neural basis of respiratory sinus arrhythmias.


    INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Heart rate is determined primarily by the centrally mediated tonic and reflex activity of parasympathetic outflow to the heart (Heymans and Neil 1958; Spyer 1981). Cardiac vagal activity is diminished and unresponsive in many disease states, and a delay in the inhibitory actions of this autonomic motor system following exercise is a powerful predictor of overall mortality (Cole et al. 1999; Eckberg et al. 1971; Larovere et al. 1988; Vanoli et al. 1991). The control of heart rate is also intertwined with the generation of respiratory rhythm within the CNS (Anrep et al. 1935; Gilbey et al. 1984). In each respiratory cycle, the heart beats more rapidly in inspiration and slows during postinspiration and expiration (referred to as respiratory sinus arrhythmia) (Anrep et al. 1935). The degree of respiratory sinus arrhythmia is often a clinical indicator of cardiorespiratory function, particularly during the neonatal and postnatal period (Hathorn 1978; Hrushesky 1991). Despite the clinical importance of respiratory modulation of heart rate, the neuronal circuit for this cardiorespiratory interaction has not yet been identified. One possible source of cardiorespiratory interactions may involve superior laryneal neurons that are active in respiration and are colocalized with cardiac vagal neurons in the nucleus ambiguus. Here we demonstrate that superior laryngeal motorneurons project to cardiovagal neurons. The Bartha strain of pseudorabies virus (PRV), an attenuated swine alphaherpesvirus, can be used as a transsynaptic marker of neural circuits. Bartha PRV invades neuronal networks in the CNS through peripherally projecting axons, replicates in these parent neurons, and then travels transsynaptically to continue labeling the second- and higher-order neurons in a time-dependent manner (Jansen et al. 1995; Jons and Mettenleiter 1997; Loewy 1998). Superior laryngeal motorneurons were tested as likely mediators of cardiorespiratory interaction because they are active in the postinspiration phase of respiration and, apart from their innervation of laryngeal muscles, they send axonal branches in close proximity to cardiovagal neurons within the brain stem (Gauthier et al. 1980; Zheng et al. 1991).


    METHODS
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

Retrograde transneuronal virus and fluorescent labeling

The gene encoding enhanced GFP, a bioluminescent protein of 238 amino acids originally isolated from the jellyfish Aequorea victoria, was inserted in the nonessential glycoprotein G (gG) gene of the transneuronal viral tracer Bartha-PRV. The coding sequence was cloned in frame behind the first seven codons of the gG gene under control of the strong gG promotor in the Bartha-PRV. To label cardiovagal neurons and the neurons that project to them, 0.5-20 µL of virus [titer =108 plaque forming units per milliliter (pfu/ml)] was injected into the pericardial sac of methoxyflurane anesthetized Sprague Dawley rats (p4-p13) of either sex. In control experiments, injections of Bartha-PRV-GFP into the chest cavity, but outside the pericardial sac, did not produce any labeling in the brain stem. In immunohistochemical and electrophysiological experiments, a bilateral stellectomy was performed to remove the sympathetic innervation to the heart (Pardini et al. 1989). To independently identify superior laryngeal motorneurons and cardiovagal neurons, crystals of the fluorescent tracer tetramethylindocarbocyanine perchlorate (DiI) were placed onto the superior laryngeal nerve and rhodamine (1% solution XRITC, 20-50 µL) was injected into the pericardial sac.

Immunohistochemistry procedures

In immunohistochemistry studies, the animals were anesthetized with methoxyflurane and perfused through the heart with 0.9% saline, followed by 4% paraformaldehyde, stored for 12-24 h, and then the brain stem was cut into 30-µm-thick sections using a cryostat. Tissue sections were incubated for 1 h in 0.1 M PBS, 2% bovine serum albumin (BSA), and 0.3% Triton X-100, washed, and incubated overnight at 4°C in a 1:1000 dilution of GFP monoclonal antibody (Clontech), followed by a 1:100 dilution of goat anti-mouse IgG fluorescein isothiocyanate (FITC) conjugate secondary antibody (Sigma). Specificity was determined by omitting the primary antibody from the incubation or by omitting the secondary antibody. Slices that included the nucleus ambiguus were imaged with a Bio-Rad (Hercules, CA) MRC-1000 confocal microscope.

Electrophysiological and in vivo studies

For electrophysiological experiments, the animals were anesthetized with methoxyflurane and killed by cervical dislocation, and the brain was sectioned into 250-µm sections. Neurons were imaged with infrared and fluorescent illumination. Standard patch-clamp electrophysiological techniques were used while the slices were continuously perfused (2-3 ml/min) with a perfusate of the following composition (in mM): 125 NaCl, 3 KCl, 2 CaCl2, 26 NaHCO3, 5 dextrose, and 5 HEPES, constantly bubbled with 95% O2-5% CO2, and maintained at pH 7.4. Patch pipettes were filled with a solution consisting of (in mM): 130 KGluconate, 10 HEPES, 10 EGTA, 1 CaCl2, and 1 MgCl2, in perforate patch experiments nystatin (258 U/ml) was included. Action potentials were recorded using the perforated-patch access and current-clamp configuration. Voltage-gated ionic currents were studied using the voltage-clamp configuration. Studies of the baroreceptor reflex were conducted in age-matched animals 10-12 days old (anesthetized with urethan, 1.3 mg/kg, IP) using standard phenylephrine infusions to increase blood pressure and evoke the baroreflex decrease in heart rate. The baroreflex curves were generated (Origin 5.0) using a sigmoidal logistic fit, y A2 + (A1 - A2)/[1 + (x/x0)p]. Two animals had a paradoxical increase in heart rate and were omitted from analysis. A paradoxical response in rats this age has also been observed by others (Kasparov and Paton 1997). All experiments were performed in compliance with institutional guidelines at George Washington University.


    RESULTS
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

To identify cardiovagal neurons and in particular the neurons that synapse on them, we first performed a series of experiments in which Bartha PRV-GFP was injected into the pericardial sac of Sprague-Dawley rats with increasing survival periods. After two days of survival, only cardiovagal neurons were labeled in the nucleus ambiguus (Fig. 1). The labeling pattern was identical to the population of cardiovagal neurons labeled with conventional retrograde fluorescent tracers such as rhodamine (XRITC) (Fig. 1). To label superior laryngeal motorneurons, the fluorescent tracer DiI was applied to the superior laryngeal nerve 2 days prior to death. Superior laryngeal motorneurons were in close proximity to cardiovagal neurons labeled 2 days after injection of Bartha-PRV-GFP into the pericardial sac, but no superior laryngeal motorneurons contained the virus (Fig. 1).



View larger version (118K):
[in this window]
[in a new window]
 
Fig. 1. Cardiovagal neurons were labeled with Bartha pseudorabies virus-green fluorescent protein (PRV-GFP) 2 days after injection of the virus into the pericardial sac. A: Bartha-PRV-GFP (green) was present only in cardiovagal neurons identified with the traditional fluorescent rhodamine tracer XRITC (red). All cardiovagal neurons contained both virus and rhodamine (yellow, n = 6). B: superior laryngeal motorneurons labeled with the fluorescent tracer DiI (red) were in close proximity to, but were not colocalized in, neurons labeled with the Bartha PRV-GFP (green) 2 days after injection of the virus into the pericardial sac (n = 7). Scale bar is 25 µm.

The utility of Bartha-PRV-GFP as a transneuronal tracer in living tissue was examined electrophysiologically 2 days after virus injection into the pericardial sac. Cardiovagal neurons could be easily visualized by both a traditional fluorescent tracer (XRITC) and the GFP fluorescent signal in an in vitro 250-µm slice of tissue 2 days after injection of the virus and XRITC into the pericardial sac (Fig. 2). The electrophysiological properties of both XRITC-labeled and PRV-infected cardiovagal neurons were analyzed by patch-clamp recordings. The voltage-gated currents and firing properties in Bartha PRV-GFP or XRITC-labeled cardiovagal neurons were indistinguishable. Cardiovagal neurons were silent with a typical resting membrane potential of -70 mV. On injection of depolarizing current cardiovagal neurons had a pattern of action potential firing with little delayed excitation or spike frequency adaptation (Fig. 2). Depolarizations to potentials more positive than -50 mV evoked a rapidly activating and inactivating sodium current that has been shown previously to be tetrodotoxin resistant, requiring 1 µM tetrodotoxin for complete block (Mendelowitz 1996, 1999). Immediately following the sodium current transient outward and long-lasting potassium currents were elicited which consist of an A-type and a delayed rectifier potassium current, respectively (Mendelowitz 1996, 1999).



View larger version (50K):
[in this window]
[in a new window]
 
Fig. 2. Bartha-PRV-GFP is compatible with normal electrophysiological recordings in vitro. A: cardiovagal neurons could be identified by the GFP fluorescent signal (green), visualized using infrared wavelengths (middle) as well as the traditional fluorescent tracer XRITC (red) in an in vitro 250-µm slice of tissue 2 days after injection of the virus and XRITC into the pericardial sac. Scale bar is 10 µm. B: the voltage-gated currents, absence of firing at rest, and the depolarization evoked firing activity of cardiovagal neurons identified with Bartha PRV-GFP (left, n = 11) were identical to the properties of cardiovagal neurons labeled with rhodamine (right, n = 12). Scale bars in current traces are 1 nA and 500 ms.

After establishing that Bartha PRV-GFP could be used to identify neurons in specific functional circuits for subsequent electrophysiological experiments, a second series of immunohistochemical experiments was performed in which animals were killed 3 days after injection of virus into the pericardial sac. In addition DiI was applied to the superior laryngeal nerve 3 days prior to sacrifice. After 3 days, the labeling was still present in cardiovagal neurons and advanced to other neurons in the nucleus ambiguus as well as additional brainstem regions including the nearby periambigual area and the nucleus tractus solitarius. Within the nucleus ambiguus, superior laryngeal motorneurons were colabeled with both DiI and Bartha-PRV-GFP, demonstrating that they innervate cardiovagal neurons (Fig. 3). Superior laryngeal motorneurons transsynaptically labeled 3 days after injection of Bartha-PRV-GFP into the pericardial sac could also be readily visualized by GFP fluorescence in an in vitro slice of tissue (Fig. 3). The traditional retrograde tracer DiI also identified these neurons. Superior laryngeal motorneurons typically fire spontaneously and continuously at a frequency of 5-7 Hz. The firing properties and individual action potentials in Bartha PRV-GFP- or DiI-labeled superior laryngeal motorneurons were identical.



View larger version (79K):
[in this window]
[in a new window]
 
Fig. 3. Superior laryngeal motorneurons project to cardiovagal neurons. Three days after injection of Bartha-PRV-GFP into the pericardial sac, virus-labeled neurons included cardiovagal neurons and the neurons that project to them. A: these neurons included superior laryngeal motorneurons (green), which were also identified by the retrograde fluorescent tracer DiI (red). Double-labeled superior laryngeal motorneurons (yellow) contained both the traditional fluorescent tracer DiI and the trans-synaptic tracer Bartha-PRV-GFP (n = 6). Scale bar is 25 µm. B: superior laryngeal motorneurons were identified in vitro by the presence of the virus (green), visualized with infrared wavelengths (middle) and by the traditional tracer DiI (red, n = 5). Scale bar is 15 µm. C: electrophysiological recordings in superior laryngeal motorneurons labeled with the virus (n = 5) and DiI (n = 14) were indistinguishable and are electrophysiologically normal 3 days after injection of Bartha-PRV-GFP into the pericardial sac.

Since the electrophysiological studies indicate both cardiac vagal neurons and superior laryngeal neurons labeled with the virus were electrophysiologically indistinguishable from these neurons identified with traditional tracers, we examined whether the baroreceptor reflex was altered in animals 3 days after injection of the virus into the pericardial sac. Phenylephrine was infused to increase blood pressure and evoke baroreflex mediated decreases in heart rate. The baroreflex responses in animals labeled with PRV-GFP were not different from sham-labeled animals (Fig. 4).



View larger version (19K):
[in this window]
[in a new window]
 
Fig. 4. Increases in blood pressure evoke baroreflex mediated decreases in heart rate. The reflex responses were unaltered in animals (n = 7) labeled with virus compared with sham-operated controls (n = 7). Initial heart rate, midpoint of the reflex, minimal heart rate, or gain of the reflex were not statistically different in virus compared with control animals.


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

It is well known that the neuronal projections from the brain to the heart strongly influence cardiac function, and an abnormal cardiovagal activity has been implicated in diseases such as cardiac arrhythmia (Spyer 1981). Respiratory sinus arrhythmia is present in healthy fetuses, newborns, and mature animals and humans (Elghozi et al. 1991). However, in distressed fetuses, as well as partially asphyxiated newborns, a slowing of the heart rate and diminished respiratory sinus arrhythmia is strongly correlated with low postnatal Apgar scores (a quick clinical assessment of overall newborn well being) and subsequent neonatal mortality such as in Sudden Infant Death syndrome (Meny et al. 1994; Schechtman et al. 1992). This study, using the Bartha-PRV-GFP transneuronal retrograde tracer has identified a pathway that can mediate the normal interactions between the respiratory system and the control of cardiac function that may be altered in diseases of the cardiorespiratory systems. The projection from superior laryngeal motorneurons to cardiovagal neurons may be responsible for respiratory modulation of heart rate. The nonbursting spontaneous activity in superior laryngeal neurons is unlikely to be responsible for generating respiratory rhythms but is more likely involved in coordinating motor activity to the heart and respiratory muscles. Superior laryngeal neurons may provide an excitatory input to cardiac vagal neurons during postinspiration. In addition to this pathway, other work has shown cardiac vagal neurons are inhibited by a GABAergic input during inspiration (Gilbey et al. 1984). The use of the PRV-GFP transneuronal retrograde tracer may provide an opportunity to study this and other pathways that are also involved in cardiorespiratory interactions.

A very recent report has examined the utility of using a PRV that also expresses enhanced GFP in an in vitro study of retinal pathways. Transsynaptically labeled neurons in the suprachiasmatic nucleus and retinal ganglia retained their major excitatory and inhibitory inputs, suggesting this virus does not interfere with the synaptic function in retinal pathways (Smith et al. 2000). This study, however, did not determine whether PRV-GFP caused any changes in firing properties or voltage-gated currents in the labeled neurons or evoked any functional changes in the retinal pathways. The present work demonstrates that the firing properties and voltage-gated currents in PRV-GFP-labeled cardiorespiratory neurons are unaltered by PRV-GFP. Moreover, this study demonstrates the function of the brain stem reflexes in the labeled pathway that control heart rate are maintained and have normal arterial baroreflex characteristics. This study also identifies a previously undescribed synaptic pathway from superior laryngeal neurons to cardiac vagal neurons that may be involved in mediating cardiorespiratory rhythms.

The present work, and that of Smith et al. (2000), indicates fluorescent viral transneuronal tracers, such as Bartha PRV-GFP are useful tools for in vitro physiological studies, particularly since in the early phases of the infection (in these studies 2-3 days), the electrophysiological properties of the neurons appear normal. In addition, the synaptic input to neurons and the reflex control of the labeled pathways are not altered by these viruses. It is anticipated that this virus can be used in the cardiorespiratory system to identify other neurons that synapse on cardiac vagal neurons and neurons involved in other cardiorespiratory functions, which can then be studied electrophysiologically. It is also likely this virus can be utilized to introduce gene products other than GFP to deliberately alter the function of specific neurons in CNS pathways that control cardiorespiratory function.


    ACKNOWLEDGMENTS

This work was supported by National Heart, Lung, and Blood Institute Grants HL-49965 and HL-59895 to D. Mendelowitz, HL-25449 to A. Loewy, and Deutsche Forschungsgemeinschaft Grant Me854/4 to T. Mettenleiter.


    FOOTNOTES

Address for reprint requests: D. Mendelowitz, Dept. of Pharmacology, George Washington University, 2300 Eye St. NW, Washington, DC 20037 (E-mail: dmendel{at}gwu.edu).

Received 18 August 2000; accepted in final form 27 September 2000.


    REFERENCES
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES

0022-3077/01 $5.00 Copyright © 2001 The American Physiological Society