Abstract
Background Signalling through platelet-derived growth factor receptor (PDGFR), colony-stimulating factor 1 receptor (CSF1R) and mast/stem cell growth factor receptor kit (c-KIT) plays a critical role in pulmonary arterial hypertension (PAH). We examined the preclinical efficacy of inhaled seralutinib, a unique small-molecule PDGFR/CSF1R/c-KIT kinase inhibitor in clinical development for PAH, in comparison to a proof-of-concept kinase inhibitor, imatinib.
Methods Seralutinib and imatinib potency and selectivity were compared. Inhaled seralutinib pharmacokinetics/pharmacodynamics were studied in healthy rats. Efficacy was evaluated in two rat models of PAH: SU5416/Hypoxia (SU5416/H) and monocrotaline pneumonectomy (MCTPN). Effects on inflammatory/cytokine signalling were examined. PDGFR, CSF1R and c-KIT immunohistochemistry in rat and human PAH lung samples and microRNA (miRNA) analysis in the SU5416/H model were performed.
Results Seralutinib potently inhibited PDGFRα/β, CSF1R and c-KIT. Inhaled seralutinib demonstrated dose-dependent inhibition of lung PDGFR and c-KIT signalling and increased bone morphogenetic protein receptor type 2 (BMPR2). Seralutinib improved cardiopulmonary haemodynamic parameters and reduced small pulmonary artery muscularisation and right ventricle hypertrophy in both models. In the SU5416/H model, seralutinib improved cardiopulmonary haemodynamic parameters, restored lung BMPR2 protein levels and decreased N-terminal pro-brain natriuretic peptide (NT-proBNP), more than imatinib. Quantitative immunohistochemistry in human lung PAH samples demonstrated increased PDGFR, CSF1R and c-KIT. miRNA analysis revealed candidates that could mediate seralutinib effects on BMPR2.
Conclusions Inhaled seralutinib was an effective treatment of severe PAH in two animal models, with improved cardiopulmonary haemodynamic parameters, a reduction in NT-proBNP, reverse remodelling of pulmonary vascular pathology and improvement in inflammatory biomarkers. Seralutinib showed greater efficacy compared to imatinib in a preclinical study.
Abstract
Seralutinib is an inhaled, small-molecule kinase inhibitor that targets PDGFRα/β, CSF1R and c-KIT, and upregulates BMPR2 protein expression; these pathways play important roles in PAH. The efficacy of seralutinib is demonstrated in two animal models of PAH. https://bit.ly/3wObkEN
Introduction
Pulmonary arterial hypertension (PAH) is characterised by perivascular inflammation and proliferation of pulmonary artery smooth muscle cells (PASMCs), myofibroblasts and endothelial cells, resulting in pulmonary arterial blood flow obstruction [1–6]. The emergence of apoptosis-resistant cells within pulmonary vascular lesions led to the cancer paradigm hypothesis to explain the abnormal cell proliferation observed in PAH lesions [1, 4, 5, 7, 8].
Within the context of this cancer-like paradigm, evidence from human PAH lung explants, cell-based assays and preclinical models points to a pivotal role of platelet-derived growth factor (PDGF) signalling in PAH pathogenesis [9–14]. Expression of PDGF ligands and receptors (PDGF receptors α and β (PDGFRα/β)) was increased in small pulmonary arteries of patients with idiopathic PAH (iPAH) versus controls, and PDGFB gene expression was increased in a single-cell RNA sequencing study in iPAH [11, 15]. Genetic knockout studies suggest that PDGFRα and PDGFRβ mediate overlapping and distinct effects across PAH-associated pathways: both receptors regulate cell proliferation, migration and inflammation, while PDGFRβ may uniquely affect angiogenesis [16]. Crosstalk between PDGFR and other signalling cascades implicated in PAH, such as transforming growth factor β (TGF-β), has been reported [17, 18]. Furthermore, PDGF signalling decreased bone morphogenetic protein receptor type 2 (BMPR2) expression in PASMCs via miRNA-376b-mediated degradation [9]. These findings highlight the therapeutic potential of PDGFR kinase inhibitors for iPAH [19].
Imatinib (a potent PDGFR/ABL/c-KIT kinase inhibitor) reversed pulmonary hypertension in the rat monocrotaline (MCT) model, demonstrating histological and functional improvements [12]. In clinical trials, imatinib improved pulmonary vascular resistance (PVR) and exercise capacity in patients with advanced PAH; however, serious adverse events and discontinuations were common, limiting its development as a PAH treatment [20, 21].
Given the robust evidence implicating PDGFR signalling in PAH pathogenesis and limitations associated with systemic administration of PDGFR inhibitors [21], seralutinib (N-[3-[(1S)-1-[[6-(3,4-dimethoxyphenyl)pyrazin-2-yl]amino]ethyl]phenyl]-5-methylpyridine-3-carboxamide, formerly PK10571 and also known as GB002) was designed and formulated as a dry powder for inhalation drug delivery. In addition to its potent inhibition of PDGFRα and PDGFRβ, seralutinib inhibits PDGFR-related kinases, colony-stimulating factor 1 receptor (CSF1R) and mast/stem cell growth factor receptor kit (c-KIT), which are implicated in PAH pathogenesis and progression [22–26]. c-KIT is expressed on endothelial progenitor cells and mast cells, potentially contributing to perivascular inflammation and vascular remodelling [8, 23, 27]. Increased infiltration of c-KIT+ cells has been observed in pulmonary arterial plexiform lesions in PAH patient lungs [23]. CSF1R is expressed on monocytes and macrophages [22]. Macrophages secrete PDGF ligands and pro-inflammatory cytokines contributing to pathological remodelling in PAH [24, 25, 28]. Thus, a compelling rationale exists to target PDGFR, CSF1R and c-KIT as a treatment for PAH. Seralutinib targets these pathways and is the first tyrosine kinase inhibitor in clinical development specifically designed as an inhalation therapy for PAH. Given the limitations of imatinib, seralutinib was intentionally developed with low oral bioavailability and rapid clearance characteristics to minimise systemic exposure and associated adverse events.
The objectives of the preclinical studies reported here were to investigate the in vitro potency and selectivity of seralutinib and characterise its efficacy as compared to imatinib in relevant animal models of PAH.
Methods
The potency and selectivity of seralutinib and imatinib were determined in vitro. Pharmacokinetic and pharmacodynamic effects of inhaled seralutinib were studied in healthy rats. Efficacy was evaluated in the rat SU5416/Hypoxia (SU5416/H) (Study 1 and 3) and MCT pneumonectomy (MCTPN) (Study 2) models. In Study 1, treatment was initiated 1 day after a 3-week hypoxia exposure; in Study 2, treatment was started on day 25 after pneumonectomy (day 15 after MCT administration). In Study 3, seralutinib or imatinib was started 2 weeks after return to normoxia, subsequent to the 3-week hypoxia period. Treatment effects on echocardiographic parameters, cardiopulmonary haemodynamic parameters, N-terminal pro-brain natriuretic peptide (NT-proBNP), BMPR2 and inflammatory markers were examined. PDGFR, CSF1R and c-KIT immunohistochemistry (IHC) was performed with rat and human lung PAH and control samples. microRNA (miRNA) analysis of SU5416/H lungs (Study 3) was performed. Detailed methods are available in the supplementary material.
Results
In vitro activity of seralutinib
Seralutinib inhibited proliferation of H1703 (a PDGFRα-driven human lung epithelial cell line), human pulmonary arterial smooth muscle cells (HPASMCs) (which express similar levels of PDGFRα and PDGFRβ) and human lung fibroblasts (HLFs) (which express PDGFRβ more than PDGFRα) with median inhibitory concentrations (IC50s) of 32 nM, 33 nM and 29 nM, respectively (figure 1, supplementary table S1). Although imatinib inhibited H1703 proliferation with an IC50 of 62 nM, its potency was 13–20-fold less than seralutinib in human PASMC and HLF proliferation assays. Both compounds potently inhibited PDGF-BB-induced extracellular signal-regulated kinase (ERK) phosphorylation in H1703 cells; however, only seralutinib inhibited ERK phosphorylation in HLFs (figure 1, supplementary table S1). Furthermore, seralutinib was more potent than imatinib against c-KIT and CSF1R kinases. Seralutinib inhibited stem-cell factor (SCF)-induced c-KIT autophosphorylation in human pulmonary artery endothelial cells (HPAECs) with an IC50 of 7.8 nM and displayed an IC50 of 14.4 nM in macrophage colony-stimulating factor (M-CSF)-induced phosphorylation of CSF1R in human primary differentiated macrophages (34-fold more potent than imatinib) (supplementary table S1, figure 1).
Pharmacokinetic and pharmacodynamic studies
Seralutinib lung concentration peaked immediately after a 2-h passive inhalation and steadily declined over time in rats. Substantially lower plasma exposures were observed relative to lung exposures (figure 2a). Four independent rat pharmacokinetic studies demonstrated an average seralutinib lung-to-plasma ratio of 30 (range 16–80) over a 24-h period. Seralutinib inhalation significantly inhibited PDGF-BB-induced PDGFRα/β autophosphorylation in the lung across all three dose levels tested (figure 2b, c). In a separate experiment, with co-administered intratracheal PDGF-BB and SCF, seralutinib inhibited c-KIT Y719 phosphorylation by 43% (figure 2d). Seralutinib inhibition of PDGFRβ phosphorylation in this experiment was similar to that observed when PDGF-BB was given alone. Furthermore, seralutinib demonstrated a 2-to-2.5-fold dose-dependent increase in lung BMPR2 protein expression over time (figure 2e).
Seralutinib efficacy in preclinical models of PAH
SU5416/H model (Study 1)
Two cohorts, with and without telemetry monitoring, received seralutinib 2.5 mg·kg−1 and 4.6 mg·kg−1 twice daily, respectively, for 2 weeks (figure 3a). Prior to initiating treatment, elevated pulmonary artery systolic pressure (PASP) was confirmed in vehicle (100.8±5 mmHg) and seralutinib (99.1±8 mmHg) groups by telemetry. Seralutinib 2.5 mg·kg−1 twice daily reduced PASP by 43% (p<0.0001) relative to vehicle at the end of treatment (figure 3b). End-of-study right ventricular systolic pressure (RVSP) measurements revealed a dose-dependent reduction with seralutinib compared to vehicle (2.5 mg·kg−1: 49.6±3.1 mmHg versus 64.4±5.4 mmHg, p<0.05; 4.6 mg·kg−1: 34.7±2.2 mmHg versus 64.4±5.4 mmHg, p<0.001) (figure 3c). A reduction in RV hypertrophy was observed in both seralutinib groups (2.5 mg·kg−1: 0.36±0.01, p<0.0001; 4.6 mg·kg−1: 0.40±0.02, p<0.005) compared to vehicle (0.54±0.03) (figure 3d).
Small pulmonary artery occlusion analysis (vessel diameter <80 μm) was performed in lung tissues from vehicle and seralutinib 4.6 mg·kg−1 twice daily groups. A significant decrease was observed in the number of grade 2 lesions in the seralutinib-treated group compared to vehicle (p<0.05; figure 3e, f). Small pulmonary artery lumen-to-media area was increased in the seralutinib-treated group compared to vehicle (p<0.05; figure 3g). IHC of lungs for phospho-PDGFRβ revealed reduced intensity in the seralutinib-treated group compared to vehicle (figure 3h).
MCTPN model (Study 2)
In the MCTPN model, seralutinib 2.5 mg·kg−1 twice daily was initiated after PAH development, and continued for 11 days (figure 4a). PASP remained stable in the seralutinib group but continued to increase in the vehicle group (figure 4b). On days 9, 10 and 11, PASP was 34%, 37% and 41% lower, respectively, in the seralutinib group compared to vehicle (p<0.05). A 50% reduction in RVSP was observed in the seralutinib group compared to vehicle (p<0.001; figure 4c). Right ventricular hypertrophy was reduced by 49% in the seralutinib group compared to vehicle (p<0.0001; figure 4d). Lumen-to-media area was increased in the seralutinib-treated group compared to controls, which indicates favourable reverse remodelling (p<0.001; figure 4e, f), with fewer grade 1 and 2 lesions (figure 4e, g). A qualitative decrease in perivascular fibrosis was observed in seralutinib-treated lungs compared to vehicle (supplementary figure S1).
Seralutinib significantly improved tidal volume (p<0.005) and decreased respiratory rate (p<0.001) as compared to vehicle (supplementary figure S2a, b). Minute ventilation and airway resistance were similar between seralutinib- and vehicle-treated animals (supplementary figure S2c, d).
SU5416/H model (Study 3): comparison to imatinib
Seralutinib (12.8 mg·kg−1 twice daily), imatinib (15.0 mg·kg−1 once daily) or vehicle control (once daily) was administered for 2 weeks following disease induction and a 2-week period of normoxia (figure 5a, b). The imatinib dose selected for the in vivo study displayed potent inhibition of PDGFRβ phosphorylation in healthy rats (supplementary figure S3).
At treatment initiation, disease severity was evaluated by echocardiography. Stroke volume index and cardiac index were decreased in diseased animals compared to healthy controls (figure 5c, d). Vehicle-treated PAH rats had elevated RVSP (85.2±11.0 mmHg) and mean pulmonary artery pressure (mPAP) (50.9±5.0 mmHg) compared to healthy controls (RVSP 19.5±1.0 mmHg; mPAP 12.6±0.6 mmHg; p<0.001 for both; figure 5e, f). Seralutinib improved haemodynamic parameters, with reductions of 45% in RVSP (46.7±3.9 mmHg) and 37% in mPAP (31.9±2.6 mmHg) compared to vehicle (p<0.001; figure 5e f). The decrease in mPAP and improvement in cardiac index resulted in a 60% improvement in PVR index (PVRI) in the seralutinib group (p<0.0001; figure 5g). Imatinib reduced RVSP by 28% (61.1±7.4 mmHg) and mPAP by 27% (37.4±3.9 mmHg) (p<0.05 versus vehicle; figure 5e, f). Compared to imatinib, seralutinib had a significantly greater effect on stroke volume index and cardiac index (figure 5c, d). The reduction in PVRI from imatinib treatment was ∼37%. Disease induction increased NT-proBNP by nine-fold. Seralutinib decreased NT-proBNP by 55% versus vehicle control (p<0.05), while no significant effect was observed with imatinib (figure 5h). Although the effects of seralutinib on these parameters were statistically greater than the effects of imatinib compared to vehicle, there was no statistically significant difference between seralutinib and imatinib with regard to mPAP, RVSP, PVRI or NT-proBNP.
Haemodynamic improvements were accompanied by a decrease in small pulmonary vessel muscularisation (figure 5i, j). Analysis of haematoxylin and eosin-stained lung sections and α-smooth muscle actin-stained sections demonstrated a decrease in small pulmonary artery muscularisation in the seralutinib group compared to both the vehicle and imatinib-treated groups (figure 5i, j, supplementary figure S4). Seralutinib significantly increased BMPR2, whereas no significant effect on BMPR2 was observed with imatinib (figure 5k). An increase in SMAD1/5 phosphorylation in seralutinib-treated animals was observed, suggesting activation of signalling through BMPR2 (supplementary figure S5).
Effects on biomarkers of inflammation
Seralutinib decreased circulating levels of plasma tumour necrosis factor α (TNF-α) (p<0.001) and increased interleukin (IL)-10 compared to vehicle (p<0.05; figure 6a, b). Imatinib did not significantly alter TNF-α or IL-10 levels. A trend towards decreased PDGF-BB was observed in the seralutinib-treated group (figure 6c). Seralutinib also decreased lung mRNA and protein levels of monocyte chemoattractant protein 1 (MCP-1), a pro-inflammatory cytokine that regulates macrophage recruitment and contributes to MCT-induced pulmonary hypertension [29] (SU5416/H model: p<0.05 compared to vehicle; supplementary figure S6b, c). Imatinib did not modulate MCP-1. Seralutinib reduced MCP-1 secretion in a dose-dependent manner in CSF1R+ human macrophages (supplementary figure S6a).
Effect of seralutinib on miRNAs in the lung
Six miRNAs predicted to repress both human and rat BMPR2 were differentially expressed in seralutinib-treated SU5416/H rat lungs relative to vehicle (supplementary table S2). Two of the six miRNAs decreased following treatment with seralutinib compared to vehicle (miR-135a-5p: p=0.01; miR-146a-5p: p=0.02), consistent with the observed increase in BMPR2 protein (figure 5k, l). Four miRNAs were increased by seralutinib, including miR-381-3p, which exhibited the largest expression shift and was significantly higher in seralutinib and imatinib groups relative to vehicle groups.
IHC in iPAH versus control lungs
We evaluated expression of PDGFRα/β, CSF1R and c-KIT proteins in human lung tissue samples to demonstrate relevance of seralutinib targets in iPAH (figure 7). Increases in PDGFRα, PDGFRβ, CSF1R and c-KIT were observed in PAH lung sections compared to controls. IHC in rat lungs from the MCTPN and SU5416/H models showed patterns of PDGFRα/β and CSF1R similar to those seen in human PAH samples (supplementary figures S7 and S8). In both animal models, treatment with seralutinib was associated with decreased signal for PDGFRα/β and CSF1R.
Discussion
PDGFR, CSF1R and c-KIT signalling play crucial roles in the pathology and progression of PAH [9–15, 21–26, 30, 31]. Targeting these pathways therefore holds promise as a therapeutic strategy in PAH. Seralutinib is a highly potent PDGFR, CSF1R and c-KIT kinase inhibitor, and is the first and only tyrosine kinase inhibitor intentionally designed as a treatment for PAH. The unique physical properties of seralutinib make it suitable for the inhaled route of administration, potentially optimising therapeutic efficacy while limiting systemic exposure and associated side-effects.
Clinical trials of imatinib in PAH provided proof of concept that targeting PDGFR signalling can affect PAH disease progression [21]. However, further development of imatinib was limited owing to side-effects attributable to relatively high systemic exposure. The clinical experience with imatinib provided impetus and rationale to develop a tyrosine kinase inhibitor targeting pathways relevant to PAH and optimised for delivery directly to the diseased lung by inhalation.
In addition to its optimisation for inhaled delivery, seralutinib displays several other unique features compared to imatinib. For example, only seralutinib inhibited ERK phosphorylation in HLFs. This difference could be important because constitutive activation of ERK1/2 is a driver of proliferation in BMPR2-silenced PAH-derived cells [32]. Seralutinib showed a 13- to 20-fold greater potency at inhibiting proliferation in human PASMCs and HLFs compared to imatinib. Furthermore, seralutinib was more potent than imatinib against CSF1R and c-KIT kinases. A limitation of the current data is the absence of compound profiling in patient-derived cells. PAH-derived PASMCs and HLFs display altered metabolism and functional signalling compared to healthy cells [33, 34]. Future studies using PAH patient cells could provide additional insights into the effects of these compounds.
Two animal models of PAH were used to examine the efficacy of inhaled seralutinib: the SU5416/H model and the MCTPN model. The SU5416/H model reproduces significant features of human PAH, including angio-obliterative lesions and vascular remodelling [35]. The MCTPN model is associated with increased inflammation, fibrosis, increased pulmonary arterial pressure and obstructive neointimal lesions (a feature not observed in the MCT-only model) [36, 37]. While it is recognised that the results of drug studies performed in animal models of PAH do not necessarily translate to human disease, the models we studied replicate key features and different aspects of human PAH. Furthermore, the experiments were designed to demonstrate a therapeutic effect after pulmonary hypertension was established rather than a preventive strategy.
Seralutinib prevented PAH progression in the MCTPN model and reversed pulmonary hypertension in the SU5416/H model in a dose-responsive manner. Haemodynamic improvements were accompanied by reverse pulmonary vascular remodelling, a reduction in NT-proBNP, an increase in pulmonary BMPR2 and an improvement in inflammatory biomarkers. The pathways targeted directly or indirectly by seralutinib stand out as key regulatory nodes in the pathological remodelling associated with PAH (figure 8). In our head-to-head preclinical study, both seralutinib and imatinib decreased mPAP, RVSP, PVRI and NT-proBNP compared to vehicle; however, the effects of seralutinib were more statistically robust. In addition, seralutinib had a greater effect in restoring small pulmonary artery muscularisation towards normal compared to imatinib. Interestingly, BMPR2 was restored to normal levels in the seralutinib-treated group, but not in the imatinib-treated group. Furthermore, while seralutinib decreased MCP-1 (CCL2), imatinib did not. Differences in compound potency, kinase selectivity and downstream signalling profiles as well as target coverage in vivo could be contributing to the observed differences between seralutinib and imatinib.
Seralutinib is a more potent PDGFRβ inhibitor than imatinib. Because signalling through PDGFRα and PDGFRβ may mediate different effects important in pathological pulmonary vascular remodelling, potent inhibition of both kinases may lead to improved efficacy in vivo. Seralutinib is also a strikingly more potent inhibitor of CSF1R than imatinib, potentially contributing to reduced inflammation and reverse remodelling. In seralutinib-treated animals in the MCTPN study, inhibition of both PDGFR and CSF1R signalling pathways may be contributing to the observed reduction in perivascular fibrosis. Although we cannot rule out that down-modulation of inflammatory markers observed in the current study may be an indirect outcome of seralutinib's reverse remodelling effects, MCP-1 modulation has been directly linked to CSF1R signal transduction in human macrophages [38, 39], and would therefore be indicative of seralutinib target engagement. Future studies to evaluate the potential anti-inflammatory and anti-fibrotic properties of seralutinib would be of interest.
Loss of BMPR2 plays a pivotal role in the pathogenesis of PAH, and crosstalk between PDGFR signalling and BMPR2 expression has been reported [9]. It is known that miRNAs can mediate crosstalk between PDGFR signalling and BMPR2, directly by repressing BMPR2 expression or indirectly by repressing other targets that alter BMPR2 [40–42]. We identified six miRNAs predicted to suppress both rat and human BMPR2 that were differentially expressed in SU5416/H rats treated with seralutinib. Of these, miR-135a-5p and miR-146a-5p were decreased in seralutinib-treated lungs, consistent with the observed BMPR2 increase. Of note, miR-135a has previously been implicated in human pulmonary hypertension [42, 43] and linked to BMPR2-specific expression in animal models [41, 44]. For example, in the mouse ovalbumin-urban particulate matter (OVA-PM) model of PAH, treatment with Antago-miR-135a restored BMPR2 to levels observed in healthy lungs [41]. A limitation of our study is that miR-135a-5p expression was only detected in one out of four animals treated with imatinib, which suggests this miRNA may not be the sole contributor to the observed changes in BMPR2 in the seralutinib group (given that BMPR2 in the imatinib group was unchanged). Expression of miR-146a-5p, which decreased with seralutinib in our study, was increased in serum from PAH patients relative to healthy controls, and has been shown to promote proliferation in HPAECs [45]. Although miR-376b is reportedly regulated by PDGF-BB, we did not find a significant regulation of this miRNA in our model [9]. Several additional predicted BMPR2-regulating miRNAs (i.e. predicted to reduce BMPR2 protein expression) were elevated following treatment with seralutinib. For example, miR-381-3p was strongly upregulated in the seralutinib and imatinib groups compared to vehicle. This miRNA is predicted to weakly repress BMPR2 but also functions as a tumour suppressor, blocking proliferation in cancer cell lines [46]. Furthermore, increased miR-381-3p has been shown to repress TGF-β and inhibit proliferation of human bronchial smooth muscle cells [47]. The net effect on BMPR2 expression of these miRNAs as an ensemble has not been characterised and is difficult to predict. Future studies could shed light on the contribution of each miRNA to seralutinib's mechanism of action. Regardless of mechanism, the increase in BMPR2 following seralutinib treatment could lead to synergistic effects in combination with therapeutic approaches specifically targeting the activin/TGF-β pathway.
Seralutinib is also a potent c-KIT inhibitor and decreased SCF-induced autophosphorylation of KIT in HPAECs. Hypoxia has been shown to increase c-KIT expression on pulmonary endothelial cells, enhancing the angiogenic response to SCF and contributing to pulmonary vascular pathology in the SU5416/H rat model [26]. Infiltration of c-KIT+ cells (endothelial progenitor cells and mast cells) was also reported in pulmonary arterial plexiform lesions in PAH lungs [8, 23, 27, 48]. Lung-targeted delivery of seralutinib may mitigate risks associated with systemic c-KIT inhibition by limiting inhibition to the disease site.
Quantitative IHC demonstrated increased integrated intensity of PDGFRα, PDGFRβ, CSF1R and c-KIT in human PAH lungs compared to controls. Our findings are consistent with previous reports of increased expression of PDGFRα, PDGFRβ and c-KIT in human PAH lungs [11, 23]. To our knowledge, this is the first report of increased CSF1R expression in human PAH. These findings support the relevance of targeting CSF1R in addition to PDGFRs and c-KIT in PAH. IHC of PDGFRα/β and CSF1R in both the rat MCTPN and SU5416/H models showed patterns similar to those seen in human PAH.
In conclusion, seralutinib delivered as an inhaled dry powder was effective in two preclinical models of PAH. Because these animal models of PAH replicate different features of the human disease, the fact that seralutinib demonstrated robust efficacy in both models increases the likelihood of seralutinib's efficacy as a treatment in human PAH. The improvement in BMPR2 levels observed with seralutinib is consistent with the reverse remodelling of small pulmonary arteries in PAH. Current standard-of-care treatments in PAH function primarily as vasodilators, with limited effects on neointimal proliferation and pulmonary vascular remodelling. Our studies indicate that seralutinib has a direct ameliorative impact on pulmonary vascular remodelling that results in improved cardiopulmonary haemodynamic parameters. The design of these studies ensured that seralutinib was initiated under fully established disease conditions, thus demonstrating the potential for efficacy in a therapeutic setting. Observed reverse remodelling of the small pulmonary arteries and restoration of lung BMPR2 expression in the rat PAH models suggest that seralutinib may have an impact on underlying causes of PAH. Seralutinib is currently in clinical development for patients with PAH (NCT04456998).
Supplementary material
Supplementary Material
Please note: supplementary material is not edited by the Editorial Office, and is uploaded as it has been supplied by the author.
Supplementary material ERJ-02356-2021.Supplement
Supplementary figures ERJ-02356-2021.Figures
Supplementary table S2 ERJ-02356-2021.Table_S2
Supplementary table S3 ERJ-02356-2021.Table_S3
Shareable PDF
Supplementary Material
This one-page PDF can be shared freely online.
Shareable PDF ERJ-02356-2021.Shareable
Acknowledgements
The authors gratefully acknowledge ITR Laboratories (Canada) for in-life pharmacokinetic and pharmacodynamics studies; IPS Therapeutique (Canada) for in vivo efficacy, Study 3; Joanna Peng (Q-Q PK Consulting LLC, USA) for pharmacokinetic modelling imatinib dose selection, in vivo studies. PHBI was the source of human lung tissue used for immunohistochemistry.
Footnotes
Selected data previously presented as follows: Galkin A, Clemons B, Garcia E, et al. GB002, a novel inhaled PDGFR kinase inhibitor, demonstrates efficacy in the Su5416 hypoxia rat model of pulmonary arterial hypertension. Circulation 2019; 140: A11102. Sitapara R, Slee D, Salter-Cid L, et al. In vivo efficacy of a novel, inhaled PDGFRα/β inhibitor, GB002, in the rat monocrotaline and pneumonectomy model of pulmonary arterial hypertension. Circulation 2019; 140: A12947. Galkin A, Sitapara R, Clemons B, et al. Pharmacologic characterization of GB002, a novel inhaled PDGFR kinase inhibitor in development for pulmonary arterial hypertension. Eur Respir J 2020; 56: Suppl. 64, 3550.
Author contributions: A. Galkin and R. Sitapara contributed equally as first authors in the generation and interpretation of data and development of content for this manuscript. All authors made substantial contributions to the conception or design of the work, or the acquisition, analysis or interpretation of data for the work; drafted the work or revised it critically for important intellectual content; and gave final approval of the version submitted for publication. All authors agree to be accountable for all aspects of the work in ensuring that questions related to the accuracy or integrity of any part of the work are appropriately investigated and resolved.
Conflict of interest: A. Galkin, R. Sitapara, B. Clemons, E. Garcia, M. Kennedy, D. Guimond, L.L. Carter, A. Douthitt, R. Osterhout, D. Slee, L. Salter-Cid and L.S. Zisman are employees of and hold stock options in Gossamer Bio, Inc. A. Gandjeva reports support for the present work from Gossamer Bio, Inc. (rat tissue slides for analysis provided to institution) and consulting fees from Gossamer Bio, Inc., outside the submitted work. R.M. Tuder reports grants P01HL152961 and R24HL123767 from NIH and stock options from Pulmokine, outside the submitted work. L.S. Zisman reports employment at Pulmokine, Inc., grants from NIH (HL102946) and patents for non-selective kinase inhibitors and spray dry formulations, outside the submitted work.
Support statement: This work was supported by Gossamer Bio, Inc. Work at Pulmokine, Inc. was supported by NIH grant HL102946 to L.S. Zisman. R.M. Tuder was supported by the following NIH grants: P01HL152961 and R24HL123767. Funding information for this article has been deposited with the Crossref Funder Registry.
- Received August 27, 2021.
- Accepted May 20, 2022.
- Copyright ©The authors 2022.
This version is distributed under the terms of the Creative Commons Attribution Non-Commercial Licence 4.0. For commercial reproduction rights and permissions contact permissions{at}ersnet.org