Abstract
BACKGROUND: Low airway surface pH is associated with many airway diseases, impairs antimicrobial host defense, and worsens airway inflammation. Inhaled Optate is designed to safely raise airway surface pH and is well tolerated in humans. Raising intracellular pH partially prevents activation of SARS-CoV-2 in primary normal human airway epithelial (NHAE) cells, decreasing viral replication by several mechanisms.
METHODS: We grew primary NHAE cells from healthy subjects, infected them with SARS-CoV-2 (isolate USA-WA1/2020), and used clinical Optate at concentrations used in humans in vivo to determine whether Optate would prevent viral infection and replication. Cells were pretreated with Optate or placebo prior to infection (multiplicity of infection = 1), and viral replication was determined with plaque assay and nucleocapsid (N) protein levels. Healthy human subjects also inhaled Optate as part of a Phase 2a safety trial.
RESULTS: Optate almost completely prevented viral replication at each time point between 24 h and 120 h, relative to placebo, on both plaque assay and N protein expression (P < .001). Mechanistically, Optate inhibited expression of major endosomal trafficking genes and raised NHAE intracellular pH. Optate had no effect on NHAE cell viability at any time point. Inhaled Optate was well tolerated in 10 normal subjects, with no change in lung function, vital signs, or oxygenation.
CONCLUSIONS: Inhaled Optate may be well suited for a clinical trial in patients with pulmonary SARS-CoV-2 infection. However, it is vitally important for patient safety that formulations designed for inhalation with regard to pH, isotonicity, and osmolality be used. An inhalational treatment that safely prevents SARS-CoV-2 viral replication could be helpful for treating patients with pulmonary SARS-CoV-2 infection.
Introduction
Airway surface lining fluid (ALF) coats the extracellular space of the epithelial cells that line the airways. ALF acidification contributes to the pathophysiology of asthma and other respiratory diseases.1–3 Specifically, ALF acidification is known to increase cough and bronchospasm, facilitate bacterial growth, increase mucus viscosity, decrease ciliary beat frequency, and cause general epithelial dysfunction.2,4–10 ALF acidification occurs during inflammatory and infectious airway disease exacerbations.2,6,8–12 Therefore, we have been investigating the effects of raising human ALF pH using an inhalational treatment, Optate (Airbase Breathing Company, Indianapolis, Indiana). Optate is an inhaled isotonic, isosmotic, alkaline medication designed to safely modify airway pH without irritating the airway epithelium. We previously demonstrated in several safety trials (Phase 1 and Phase 2) that Optate inhalation is well tolerated in healthy humans and those with stable asthma and COPD.9 We also demonstrated that a single inhalation of Optate effectively raises ALF pH, as indicated by a decrease in exhaled nitric oxide and an increase in exhaled breath condensate pH.9
Pandemic infection with SARS-CoV-2 (COVID-19) has cost hundreds of thousands of lives within the last year (https://www.who.int, Accessed August 9, 2020). In vitro, raising intracellular pH partially prevents activation of SARS-CoV-2 in primary normal human airway epithelial (NHAE) cells; indeed, intracellular alkalinization decreases viral replication by several mechanisms.13–16 Because Optate is effective at raising extracellular pH in the human airway, we studied whether it would prevent SARS-CoV-2 replication in NHAE cells. Specifically, we hypothesized that Optate would increase intracellular pH and decrease SARS-CoV-2 replication in NHAE cells compared to those treated with a placebo with the hope that it could serve as a treatment for this disease.
QUICK LOOK
Current knowledge
Low airway epithelial surface pH impairs antimicrobial host defense and worsens airway inflammation. Low airway epithelial intracellular pH facilitates SARS-CoV-2 cell entry and replication. Inhaled Optate is designed to raise airway epithelial surface pH.
What this paper contributes to our knowledge
At the dose inhaled in human trials, Optate raises airway epithelial intracellular pH and almost completely prevents SARS-CoV-2 replication in NHAE cells, ablating both viral plaque formation and nucleocapsid protein expression. Optate is thus an effective antiviral in vitro that was safe for human inhalation in healthy subjects.
Methods
Cell Culture
Primary NHAE cells were grown as previously described from healthy, non-smoking donors.17,18
Optate (120 mM) was prepared and assayed for purity, potency, osmolality (target ∼ 330 mOsm), pH (target 9.8), and sterility prior to all experiments (IND #139144; Arena District Pharmacy, Columbus, Ohio). For the in vivo study, 10 healthy subjects > 18 y old with no history of lung disease were recruited under our approved protocol (Case Western Reserve University Institutional Review Board #03-18-28). FEV1, FVC, heart rate, , and adverse events were monitored before and after a single nebulization of 2.5 mL Optate (120 mM) as previously described9 and reviewed by our data safety monitoring board. No change was noted in any vital signs of any subject before and after treatment.
For the in vitro studies, cells were exposed to the same batch of 120-mM Optate described above in a 1:1 ratio with cell culture media to mimic the expected dilution effects of airway lining fluid in vivo. Phosphate-buffered saline (PBS) was used as the in vitro placebo. Airway cells were acquired by brush biopsy with informed consent (Indiana University Institutional Review Board Protocol #1408855616).
Intracellular pH Assays
Intracellular pH was evaluated with 2 fluorescent dyes: 1.25-μM 2',7'-bis-(2-carboxyethyl)-5-(and-6)-carboxyfluorescein, acetoxymethyl ester (BCECF-AM, Invitrogen, Carlsbad, California), which increases in green fluorescent intensity (E:E 500:531 nm) as pH increases19; and 20-µM pHrodo Red (Invitrogen), which decreases in red fluorescent intensity (E:E 560:585 nm) as pH increases.20 After washing with PBS, cells were treated with Optate (clinical solution, 1:1 dilution in medium) or PBS. As a negative control, cells were treated with ZnCl2 (100 µM), which acidifies the intracellular space by inhibiting Hv1.21
Viral Growth and Plaque Assays
SARS-CoV-2 Isolate USA-WA1/2020 was provided by Biodefense and Emerging Infection Resources (Manassas, Virginia). In our Biosafety Level 3 facility, viral stocks were prepared in Vero E6 cells (African green monkey kidney cell line, ATCC, Manassas, Virginia) at 37°C for 2–4 d until cytopathic effect was observed. Media from the cells were collected and centrifuged (1,000 g; 5 min). Virus was quantified with plaque assay (see the supplementary materials at http://www.rcjournal.com).
Vero E6 or NHAE cells were plated the day prior to the experiment. Cells were pretreated with Optate or PBS for 5–10 min prior to SARS-CoV-2 infection (multiplicity of infection = 1). After 1 h, cells were washed with PBS, and medium with or without Optate was added. For viral titers, the media was not changed prior to harvesting supernatant for viral titers at 24 h after infection. Supernatant was harvested every 24 h, and viral replication was determined with plaque assay. Data are from 3 experiments, each done in duplicate. NHAE infection studies used 2 different donors to reduce donor effect on results.
Immunoblots
Using the same protocol as that for plaque assay, cells were lysed in radioimmunoprecipitation assay buffer. Capillary electrophoresis was performed on the automated JESS system (ProteinSimple, San Jose, California). Briefly, 0.5 μg/μL lysate was plated and run according to the manufacturer's recommendations. Antibodies are listed in the supplementary materials (available at http://www.rcjournal.com). Compass software (ProteinSimple) generated digitally rendered bands on the basis of chemiluminescence electrophoretogram.
RNA Processing
RNA was extracted from control and Optate-treated NHAE cells (48 h) using RNeasy Plus kit (Qiagen, Hilden, Germany) following the manufacturer-recommended protocol. Total RNA was first evaluated for its quantity and quality (Bioanalyzer 2100, Agilent Technologies, Santa Clara, California); all samples had an RNA integrity number of 9 or higher. Total RNA (100 ng) was used for cDNA library preparation and quantitation, (supplementary material related to this paper is available at http://www.rcjournal.com). More than 95% of the sequencing reads reached Q30 (ie, 99.9% base call accuracy).
Sequenced libraries were mapped to the human genome (UCSC hg38) using STAR RNA-seq aligner 2.5 with the following parameter: -outSAMmapqUnique 60. Read distribution across the genome was assessed using bamutils (from ngsutils 5.9). Uniquely mapped sequencing reads were assigned to hg38 refGene genes using featureCounts (subread 1.5.1) with the following parameters: -s 2 -Q 10. Reads with count per million < 0.5 in more than 3 samples were removed.
Cytotoxicity Assays
Cytotoxicity of Optate was measured with both lactate dehydrogenase (LDH) concentration (Cayman Chemical assay, Ann Arbor, Michigan) and Trypan Blue exclusion (TC20 automated cell counter, Bio-Rad Laboratories, Hercules, California) according to the manufacturers' specifications as previously described.22
Data Analysis
The Student unpaired, 2-tailed t test was used to evaluate cytotoxicity, pH, viral plaque, and protein levels comparing control groups and treatment groups. The Wilcoxon rank-sum test was used for non-Gaussian distributed data as determined with the Shapiro-Wilk test. A mixed-effects analysis of variance model was used for repeated measures, with a Tukey post hoc correction for multiple comparisons. For RNA sequencing, gene symbols were converted to entrez ids using biomaRt and analyzed with the clusterProfiler package in R (R Foundation for Statistical Computing, Vienna, Austria).23,24 Data were normalized using trimmed mean of M values. Differential expression analysis was performed using edgeR 3.12.1. Family error rate was controlled for using Bonferroni.
Results
Optate Raises Intracellular pH in NHAE Cells
After loading with BCECF-AM (green) or pHrodo Red (red) dye, cells were treated with Optate or placebo and imaged for intracellular fluorescent intensity. Cells treated with Optate showed a significant increase in green fluorescent intensity (n = 4, P = .039) and decrease in red fluorescent intensity (n = 4, P = .001) compared to those treated with placebo, indicating an increase in intracellular pH (Fig. 1). ZnCl2, which is known to acidify the intracellular space,21 had an effect opposite compared to Optate (n = 3 and 5, P = .036 and .001, respectively).
Optate Decreases SARS-CoV-2 Viral Replication
SARS-CoV-2 plaque-forming units (PFUs) were measured in culture media from Optate- and placebo-treated Vero E6 cells (the cells used to expand viral stock) infected with SARS-CoV-2. All cells were treated once, immediately after infection. Optate ablated viral PFUs in the Vero E6 cells (n = 3 experiments, 2 replicates each, P < .001) (Fig. 2). Under similar conditions, NHAE cells were then infected with SARS-CoV-2 and treated with Optate or placebo; then SARS-CoV-2 PFUs and N protein levels were measured daily for 5 d. After infection was established (24 h), both viral PFUs and N protein levels were ablated in the Optate-treated cells, unlike the cells treated with placebo (3 experiments using cells from 2 subjects, 2 replicates each, P < .001) (Fig. 2).
Optate Alters Endosomal Trafficking in NHAE Cells
RNA sequencing results were compared between control and Optate-treated NHAE cells. Genes with significant differences between the groups are presented in a volcano plot (Fig. 3). Genes decreased in the Optate-treated group are negative (left) and those that increased are positive (right). Downregulated genes for endocytosis and endosomal trafficking are labeled in green. A list of downregulated genes is provided in the supplementary materials (available at http://www.rcjournal.com). Genes in blue have a Bonferroni-corrected P value < .001 and the absolute log(FC) < 1.5; genes in magenta have a Bonferroni-corrected P value < .001 and the absolute log(FC) > 1.5. Genes in black are below the significance threshold of .001.
Optate Is Safe and Well Tolerated
Human subjects (n = 10 normal volunteers) who inhaled Optate (120 mM) had no significant change in FEV1 (P = .84), FVC (P = .99), heart rate (P = .42), or (P = .99) after inhalation, consistent with previous data (Fig. 4).9 To validate that the observed antiviral effects were not due to Optate killing the host cells, we evaluated cytotoxicity in the control cells and the Optate-treated cells. Primary NHAE cells exposed to 120-mM Optate did not differ from the control group in cytotoxicity as determined with Trypan Blue exclusion or LDH levels (Fig. 4).
Discussion
Our group previously reported that inhaled compounds can alter airway pH in vivo.1,9 Alterations of airway pH for therapeutic purposes have been proposed for chlorine gas inhalation, asthma, and cystic fibrosis.1,25,26 These applications have all focused on altering extracellular pH, likely due to the fact that most commonly known toxicities of ALF pH disturbance are extracellular. However, most respiratory viruses require an intracellular acidic event within airway epithelial cells to enter and to replicate.13,16 Our findings indicate that Optate, which was previously shown to increase ALF (extracellular) pH,9 indeed raises the intracellular pH of NHAE cells and ablates SARS-CoV-2 viral replication after infection. A safe, inhaled medication for raising intracellular pH could be of benefit for treating respiratory viral diseases even beyond SARS-CoV-2.
This work has several limitations. As with any in vitro experiment, the cell culture models used here are not necessarily representative of the in vivo systems and disease processes, and our observations may not translate. Moreover, COVID-19 involves many physiologic processes downstream from SARS-CoV-2 infection and replication. It is possible that different therapeutic targets rather than viral replication will be necessary to benefit patients. However, the fact that Optate inhalation does alkalinize the extracellular milieu in vivo suggests the observed effects may occur in patients with SARS-CoV-2. Thus, we are preparing to conduct a randomized, placebo-controlled, multicenter trial to better evaluate the therapeutic value of Optate. There were also technical limitations regarding the experiments used. For instance, viral infection of NHAE cells took > 24 h and resulted in lower titers than that seen with Vero E6 cells. This was previously observed in NHAE infection models of SARS-CoV-127,28 and was therefore unsurprising; however, it did warrant validation in several replicates and required the use of multiple cell lines. Further studies are needed to optimize this model, including evaluation of different time courses, the ability for viral replication to occur after treatment cessation, and the duration of effects. Finally, although our results suggest that our mechanism of action results from intracellular alkalinization leading to altered endocytic pathways and endosomal trafficking, there could be other mechanisms by which Optate ablates SARS-CoV-2 infection in Vero E6 and NHAE cells.
Inhalation of pH-altering compounds should be done with caution. Exposures to pH > 10 and < 6.5 are known to adversely affect NHAE cell function.7,22 Moreover, inhalation of hypotonic and hyposmotic solutions, such as many intravenous medications, causes airway irritation, bronchial hyperreactivity, and coughing.29 Our 1:1 PBS/cell culture media placebo group had a pH of 8 and still had significant viral infection, suggesting a fairly narrow therapeutic window for this purpose. Therefore, a specific formulation designed for inhalation with regard to isotonicity and osmolality that is buffered to an ideal pH within the therapeutic window needed to inhibit viral replication is required.
Conclusions
Optate raises intracellular pH and prevents SARS-CoV-2 replication in NHAE cells. Inhaled Optate raises ALF pH in human subjects, and it is non-toxic in vitro and in vivo, suggesting that a clinical trial to prevent treat life-threatening SARS-CoV-2 respiratory infection could be contemplated.
Acknowledgments
We thank Ms Kenzie Mahan for her administrative support.
Footnotes
- Correspondence: Benjamin Gaston MD, Wells Center for Pediatric Research, 1044 W Walnut St, Indianapolis, IN 46202. E-mail: begaston{at}iu.edu
Supplementary material related to this paper is available at http://www.rcjournal.com.
Drs Davis and Gaston are partially supported by NIH P01 HL128192-01A1, and P01 HL158507 are patent holders of Optate, and are co-founders of Airbase Breathing Company. Drs Gilk and Robinson are also patent holders of Optate. The remaining authors have disclosed no conflicts of interest.
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