key: cord-0754609-20g0xr2p
authors: Hamed, Maaweya E.; Naeem, Asif; Alkadi, Haitham; Alamri, Aref A.; AlYami, Ahmad S.; AlJuryyan, Abdullah; Alturaiki, Wael; Enani, Mushira; Al-Shouli, Samia T.; Assiri, Abdullah M.; Alosaimi, Bandar
title: Elevated Expression Levels of Lung Complement Anaphylatoxin, Neutrophil Chemoattractant Chemokine IL-8, and RANTES in MERS-CoV-Infected Patients: Predictive Biomarkers for Disease Severity and Mortality
date: 2021-07-07
journal: J Clin Immunol
DOI: 10.1007/s10875-021-01061-z
sha: 22df7d8854432235423e6d1a687a973f7a8f004e
doc_id: 754609
cord_uid: 20g0xr2p

The complement system, a network of highly-regulated proteins, represents a vital part of the innate immune response. Over-activation of the complement system plays an important role in inflammation, tissue damage, and infectious disease severity. The prevalence of MERS-CoV in Saudi Arabia remains significant and cases are still being reported. The role of complement in Middle East Respiratory Syndrome coronavirus (MERS-CoV) pathogenesis and complement-modulating treatment strategies has received limited attention, and studies involving MERS-CoV-infected patients have not been reported. This study offers the first insight into the pulmonary expression profile including seven complement proteins, complement regulatory factors, IL-8, and RANTES in MERS-CoV infected patients without underlying chronic medical conditions. Our results significantly indicate high expression levels of complement anaphylatoxins (C3a and C5a), IL-8, and RANTES in the lungs of MERS-CoV-infected patients. The upregulation of lung complement anaphylatoxins, C5a, and C3a was positively correlated with IL-8, RANTES, and the fatality rate. Our results also showed upregulation of the positive regulatory complement factor P, suggesting positive regulation of the complement during MERS-CoV infection. High levels of lung C5a, C3a, factor P, IL-8, and RANTES may contribute to the immunopathology, disease severity, ARDS development, and a higher fatality rate in MERS-CoV-infected patients. These findings highlight the potential prognostic utility of C5a, C3a, IL-8, and RANTES as biomarkers for MERS-CoV disease severity and mortality. To further explore the prediction of functional partners (proteins) of highly expressed proteins (C5a, C3a, factor P, IL-8, and RANTES), the computational protein–protein interaction (PPI) network was constructed, and six proteins (hub nodes) were identified. [Image: see text] SUPPLEMENTARY INFORMATION: The online version contains supplementary material available at 10.1007/s10875-021-01061-z.

The COVID-19 pandemic caused by severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) has gained significant attention in the medical and scientific communities. The Middle East Respiratory Syndrome coronavirus (MERS-CoV) has caused considerable medical and health issues in many countries, particularly in Saudi Arabia. The prevalence of MERS-CoV in the Kingdom of Saudi Arabia (KSA) remains significant. MERS-CoV cases are still being reported in Saudi Arabia, and a high prevalence of MERS-CoV in dromedary camels and direct contact with infected camels have been linked to human infections [1] [2] [3] [4] [5] . MERS-CoV is a single-stranded RNA virus of the Betacoronavirus genus. It was first reported in the KSA (Jeddah City) in 2012. As of December 27, 2020, 2564 laboratory-confirmed cases and 881 associated deaths (case-fatality ratio, 34.4%) were reported in 27 countries worldwide, of which 2121 cases (82.7%) were reported in Saudi Arabia. The majority of the fatalities (37.1%, 788 deaths) also occurred in Saudi Arabia [4] . An excessive inflammatory response is a prominent phenotype associated with MERS-CoV infection, which leads to lung immunopathology, disease progression, and poor clinical outcome. MERS-CoV infections are characterized by dysregulation in both the innate and adaptive immune systems [5, 6] . Several inflammatory cytokines and chemokines (IL-1β, IL-2, IL-6, IL-7, IL-8, IL-10, G-CSF, GM-CSF, IP-10, MCP-1, MIP-1α, IFN-γ, TNF-α, CCL2, and CCL3) are significantly associated with severe MERS-CoV infection and higher fatality rates [5, 7, 8] . Elevated inflammatory cytokine and chemokine levels during SARS-CoV-1, MERS-CoV, and SARS-CoV-2 infections are significantly associated with massive infiltration of immune cells into the lungs and poor disease outcome [5, [8] [9] [10] . The complement system consists of a multiprotein network belonging to both the innate and adaptive immune systems [11] . Depending on the manner of activation, the complement cascade operates by three pathways: the classical pathway, the lectin pathway, and the alternative pathway [12, 13] . Cross-talk between the complement and coagulation systems plays a crucial role in vascular endothelial damage and thromboinflammation [14] . A number of viral infections are associated with complement activation and coagulation dysfunction [11, 15, 16] . Over-activation of pulmonary and systemic complement plays a key role in inflammation, endothelial cell damage, thrombus formation, and intravascular coagulation, which results in multiple organ failure and eventually death [12, 15, 17] . This over-stimulation leads to the formation of the complement anaphylatoxins, C3a and C5a. C5a is a chemoattractant for neutrophils, monocytes, eosinophils, and T cells [15, 18] .

Following infection, complement anaphylatoxins stimulate phagocytic cells and enhance the production of TNF-α, IL-1β, IL-6, IL-8, granular enzymes, and free radicals. These mediators promote vascular dysfunction, fibrinolysis, and microvascular thrombosis formation [11, 12, 14, 15, 17, 18] . C5a also plays an important role in stimulating the expression of P-selectin, intercellular adhesion molecule-1, fibronectin, and fibrinogen. The upregulation of adhesion molecules activates different cell signaling and pro-inflammatory pathways [15, 16] .

The role of complement in MERS-CoV disease immunopathology and complement-modulating treatment strategies during MERS-CoV infection has received limited attention. There are many important unanswered questions regarding complement, MERS-CoV interactions, and disease outcome. In addition, little is known regarding pulmonary complement activation during MERS-CoV infection, the manner in which complement activation affects disease severity or the association of complement response with viral load and mortality.

In this study, we performed a comprehensive investigation of the pulmonary complement proteins, IL-8 (CXCL8) and RANTES (CCL5) expression in MERS-CoV-infected patients in addition to viral load determination. We also assessed the correlation between these factors and the fatality rate. To our knowledge, this is the first study demonstrating a relationship between lung complement proteins and complement regulatory factors in MERS-CoV-infected patients.

A total of 31 MERS-CoV-positive patients and 15 MERS-CoV non-infected group were enrolled in this study. Lower respiratory samples (bronchoalveolar lavage (BAL) or tracheal aspirate (TA)) were collected. The mean time from the onset of symptoms to hospital arrival, seeking medical attention, and hospital admission was 4.3 days. All respiratory samples were collected in less than one week after symptom onset (Early phase of infection) within 24 h of hospital admission. Although healthy control individuals in this study presented with respiratory symptoms, their MERS-CoV RT-PCR test was negative and were considered as the healthy non-infected control group. In this study, we used the remaining volume of MERS-CoV non-infected subject samples that had been collected for clinical diagnosis. To exclude the effects of antiviral therapy on the expression of complement proteins, IL-8 and RANTES, all samples were collected before the administration of any antiviral treatment. Samples were centrifuged at 1000 rpm at 4 °C for 5-10 min. The cell-free supernatants were used for the analysis of complement proteins, inflammatory chemokines, RANTES, and MERS-CoV viral load. The exclusion criteria were as follows: (1) patients coinfected with other respiratory pathogens, (2) immunocompromised patients, (3) patients under treatment with anti-inflammatory and/ or immunosuppressive drugs, (4) patients with chronic diseases, and (5) patients with preexisting autoimmune diseases. These exclusion criteria were selected to exclude any possible effects on the expression of the clinicopathological factors listed above. This study was reviewed and approved by the Institutional Review Board at King Fahad Medical City (IRB register number 019-053).

The MERS-CoV viral loads of the lower respiratory samples were detected by real-time RT-PCR after viral RNA was extracted using QIAamp Mini kit (Qiagen) according to the manufacturer′s instructions. The viral open reading frame regions (orf1a) gene was detected with a commercial kit according to the manufacturer's instructions (Real-Star® MERS-CoV RT-PCR Kit 1.0). The RT-PCR analysis was performed using an ABI Prism® 7500 (Applied Biosystems).

Pulmonary levels of human complement C3 and C5 fragments, as well as C3b, C1q, and C2, were measured using ELISA kits (HCA39-K01-Eagle Biosciences, Inc., Columbia, USA; ab193695, Abcam, Cambridge, UK; ab195461, Abcam, Cambridge, UK; ab170246, Abcam, Cambridge, UK; ab154132, Abcam, Cambridge, UK) following the manufacturer's instructions. The concentrations were calculated using standard curves.

The concentrations of four human complement regulatory factors, factors P (properdin), I, C4-binding protein (C4-BP), and H, were quantified in the lung using ELISA kits (ab222864, Abcam, Cambridge, UK; ab195460, Abcam, Cambridge, UK; ab222866, Abcam, Cambridge, UK; HK342 Hycult Biotech, Uden, Netherlands). The ELISAs were done following the manufacturer's instructions. The concentrations of each factor were calculated using standard curves.

We determined the local RANTES chemokine levels in MERS-CoV-infected patients (n = 30) and MERS-CoV noninfected individuals (n = 18). Lung RANTES levels were quantified using the human RANTES ELISA Kit (R&D Systems, Minneapolis, USA) following the manufacturer's protocol. RANTES concentrations were calculated using standard curves, and the results were expressed as pg/ml.

The concentrations of major human pro-inflammatory cytokines and chemokines were measured in the respiratory samples of 30 MERS-CoV-infected patients and 18 MERS-CoV non-infected individuals using the multi-analyte ELISArray (Qiagen, Germantown, MD, USA) following the manufacturer's protocol. The absorbance of the ELISArray was measured at 450 nm. The concentrations were calculated using a standard curve. Cytokine/chemokine levels were expressed as pg/ml.

To further explore the potential interplay among the differentially expressed proteins (C3a, C5a, factor P, IL-8, and RANTES) in the lung of MERS-CoV infected patients with the potential interactors. Protein-protein interaction networks were constructed using bioinformatics resources of the Search Tool for the Retrieval of Interacting Genes/ Proteins database (STRING version 11.0). This bioinformatics resource provides known and predicted protein-protein interaction networks. We used multiple proteins (C3a, C5a, factor P, IL-8, and RANTES) as an input (seed proteins). Active interaction sources include; databases, co-occurrence of genes, homology of proteins, experiments (biochemical/ genetic data), co-expression of gene and text mining as well as species limited to "Homo sapiens", confidence score > 0.4 and maximum interactors (= 20) were used to construct the STRING networks. The STRING resource is available online at https:// string-db. org/. The constructed STRING PPI network was exported to Cytoscape software (version 3.8.2 http:// apps. cytos cape. org/ apps/ mcode) for visualization and additional analysis of functional protein-protein interaction.

Statistical analyses were performed using the GraphPad 5.0 software (GraphPad Software, San Diego, CA, USA). Data were assessed using a t-test. The correlations between complement proteins, inflammatory factors, and chemokines were assessed using Pearson's correlation test. The results were presented as means ± standard deviation (SD) unless otherwise specified. A P-value of < 0.05 was considered statistically significant.

A total of 31 MERS-CoV-infected patients (22 males and 9 females) and 15 MERS-CoV non-infected group without underlying diseases/pre-existing conditions (9 males and 6 females) were included in this study ( Table 1 ). The ages ranged from 30 to 100 years. The majority of MERS-COVinfected patients were 60-75 years old. The overall mean and median ages were 68.26 ± 16.04 and 73 years, respectively. The mean ages in the non-survival and survival patients were 74.5 ± 11.3 and 53 ± 15.8 years, respectively. Twenty-two (70.97%) patients died, 9 recovered (29.03%), and 25 (80.6%) required intensive care unit (ICU) admission (Fig. 1) . The age is one of factors that could cause physiologic changes within the immune system, and may affect both the innate and adaptive immune arms of immune system, particularly T cell immunity [19, 20] . However, we did not observe any significant modulation or differences in complement inflammatory mediators and cytokines/ chemokines expression levels between aged MERS-CoV infected patients and younger MERS-CoV infected patients, but this finding requires further evaluation as the exact picture and details about immune physiologic changes with aging is still emerging. In a study of small numbers of MERS-CoV-infected patients, a similar MERS-CoV-specific cellular immune response was observed among all age groups [21] .

In this study, most deaths occurred in elderly patients aged > 70 years (68%) followed by 60-70 years (22%), 50-60 years (4.5%) and 40-50 years (4.5%). We found that the increased age was associated with mortality in MERS-CoV infected patients. As with COVID-19, we observed that with increased age (60-70 and > 70 years old), case fatality was increased from 22 to 68%, suggesting that older peoples are at high risk for death. The mean MERS-CoV viral load, ± SD and (median) were 25.7 ± 5 (26), respectively (Table 1 ). We also found that the mean viral load was significantly higher in male patients (24.5) than in female patients (28.7) (P-value 0.032) ( Table 1) .

Over-activation of the complement system is associated with immunopathology and tissue damage. Therefore, we hypothesized that the elevated lung complement protein levels occurring during MERS-CoV infection are involved in the massive infiltration of immune cells into the lungs and result in poor disease outcomes. To assess whether lung complement anaphylatoxins (C3a and C5a) were increased in MERS-CoV-infected patients, we examined complement components in lower respiratory lung samples using ELISA. As shown in (Fig. 2) , the levels of complement anaphylatoxins (C3a and C5a) and C1q were significantly higher in the lungs of MERS-CoV-infected patients compared with MERS-CoV non-infected group ( Fig. 2A , 2B, and 2G). Together, these results show that the high levels of complement anaphylatoxins in the lungs of MERS-CoV-infected patients are significantly increased, suggesting a significant pulmonary complement activation. In addition, the elevated levels of lung complement anaphylatoxins suggest a role of these factors in lung tissue damage, immunopathology, ARDS development, and mortality of MERS-CoV-infected patients.

Elevated levels of complement anaphylatoxins prompted us to evaluate the changes in other immunoregulatory proteins. Complement regulatory proteins function by inhibiting complement over-activation to avoid inflammation and tissue damage. We quantified factor P (properdin) levels in the lung of MERS-CoV-infected patients. As shown in (Fig. 2C ), the levels of positive regulatory factor P were significantly higher in the MERS-CoV-infected patients compared with the MERS-CoV non-infected group, suggesting that the levels of factor P may enhance complement activation during MERS-CoV infection. Factor P measurement in serum may provide evidence for the involvement of the alternative complement pathway since factor P represents an important factor in the activation of the alternative pathway.

The measurement of negative regulatory proteins in the lung of MERS-CoV-infected patients may provide evidence for complement system regulation. The quantification of several complement negative regulatory factors (factor I, C4-BP, and factor H) revealed that the levels of factors I and H were increased in the lower lung respiratory samples ( Fig. 2D and 2E). These negative regulatory proteins play an important role in complement system regulation. In contrast, the levels of C4-BP were unchanged, and there was no statistical significance between the levels in the MERS-CoV-infected patients compared with MERS-CoV non-infected group (Fig. 2F ). This result indicates that MERS-CoV may suppress and inhibit the function of C4-B. The measurement of negative regulatory proteins in the lung of MERS-CoV-infected patients may provide evidence for complement system regulation. The quantification of several complement negative regulatory factors (factor I, C4-BP, and factor H) revealed that the levels of factors I and H were increased in the lower lung respiratory samples ( Fig. 2D and 2E ). These negative regulatory proteins play an important role in complement system regulation. In contrast, the levels of C4-BP were unchanged, and there was no statistical significance between the levels in the MERS-CoV-infected patients compared with MERS-CoV non-infected group (Fig. 2F ). This result indicates that MERS-CoV may suppress and inhibit the function of C4-B.

The measurement of negative regulatory proteins in the lung of MERS-CoV-infected patients may provide evidence for complement system regulation. The quantification of several complement negative regulatory factors (factor I, C4-BP, and factor H) revealed that the levels of factors I and H were increased in the lower lung respiratory samples ( Fig. 2D and 2E ). These negative regulatory proteins play an important role in complement system regulation. In contrast, the levels of C4-BP were unchanged, and there was no statistical significance between the levels in the MERS-CoV-infected patients compared with MERS-CoV noninfected group (Fig. 2F ). This result indicates that MERS-CoV may suppress and inhibit the function of C4-B.

To examine the levels of chemokines in the lung during MERS-CoV infection, we quantified IL-8 and RANTES in the lower respiratory tract of MERS-CoV-infected patients and the MERS-CoV non-infected group. As shown in Fig. 2 , IL-8 and RANTES levels were significantly higher in the lungs of MERS-CoV-infected patients compared with that in the MERS-CoV non-infected group ( Fig. 2H and 2I ).

Twenty-two MERS-CoV-infected patients died during hospitalization. The C3a (4525 ± 920.4, P = 0.0008), (Fig. 3A, 3B, 3C , and 3F). The levels of C4BP were significantly higher in the surviving group compared with that in the non-surviving group (Fig. 3D ).

The Pearson correlation analysis revealed a significant association of C3a, C5a, IL-8, and RANTES with ARDS development and a higher fatality rate ( Table 2 ). Higher levels of these mediators were significantly positively correlated with ARDS and a higher fatality rate. These immune mediators increase the risk of developing ARDS and mortality in MERS-CoV-infected patients. Elevation of lung C3a, C5a, IL-8, and RANTES may represent biomarkers for ARDS development and a predictor for in-hospital mortality.

We further examined whether there were correlations between lung complement anaphylatoxins (C3a and C5a), factor P, IL-8, and RANTES. The results indicated that lung complement C5a was positively correlated with factor P, IL-8, and RANTES, whereas complement C3a was positively correlated with IL-8 and RANTES (Table 2) . A positive correlation between RANTES, IL-8, and complement factor P was also observed (Table 2) . Similarly, IL-8 was positively correlated with complement factor P ( Table 3) .

To understand the protein-protein interaction between the complement proteins and cytokines/chemokines and predicted interactors, we performed data mining and curation to construct and map the network of protein-protein interactions using the STRING databases. C3a, C5a, factor P, IL-8 and RANTES were used as seeds for network analysis. The PPI network showed 20 proteins that have the highest interaction scores with C3a, C5a, factor P, IL-8, and RANTES (Supplemental Fig.4 ). For C3a, C5a, IL-8, and RANTES, individual protein-protein interaction was also created (Supplemental Figs.5 , 6, and 7) . The names of proteins, predicted functional partners, and actions are shown in (Supplementary Table1 ). This network comprises several types of interactions including; gene neighborhood, gene fusions, co-occurrence, coexpression, text-mining, protein homology, and experiments (biochemical/genetic data). The physical (direct) or functional (indirect) interactions were also shown. The constructed network contained 25 nodes, 149 edges, average node degree 11.9 and the PPI enrichment P-value was < 1.0e-16. Cytoscape analysis was shown in (Supplementary Table 2 ). CytoHubba analysis identified the top 6 proteins (hub nodes) based on Betweenness, Closeness, Degree, EcCentricity, EPC, MCC, and MNC calculation methods (Supplementary Tables 3 and 4 ). These hub nodes are involved in the inflammatory response and molecular binding interaction as well as ligand-receptor interaction. These results indicate that predicted proteins (interactors) and hub proteins may also have a role in MERS-CoV disease severity.

An excessive inflammatory response is a major characteristic of MERS-CoV infections and results in disease progression and poor clinical outcomes. MERS-CoV infections are characterized by dysregulation of the innate and adaptive immunity systems. Several inflammatory cytokines/ chemokines and over-activation of complement proteins are significantly associated with severe MERS-CoV infections and a higher fatality rate [5, 6, 8] . In this study, we sought to determine the levels of pulmonary complement proteins, neutrophil chemoattractant chemokine IL-8, and RANTES, as well as viral load, in MERS-CoV-infected patients and assessed their association with mortality. This study is the first to evaluate the pulmonary complement protein expression profile in MERS-CoV infected patients without chronic diseases. The results showed high levels of complement anaphylatoxins (C3a and C5a), positive complement regulatory proteins, neutrophil chemoattractant chemokine IL-8, RANTES, and viral load in MERS-CoV-infected patients.

A number of studies have found that high viral load, duration of viral shedding, and direct cytopathic effects were associated with severe complications during SARS-CoV-1,

RNA levels [27] . In this study, 70% of the MERS-CoVinfected patients developed pneumonia and required ICU admission.

Over-activation of the immune response, including the complement system, is believed to be an important factor for the high fatality rate of the 1918 influenza pandemic; H1N1, H5N1, and H7N9; SARS-CoV-1, MERS-CoV; Ebola infection; and, most recently, COVID-19 (SARS-CoV-2) infection [5, 10, [28] [29] [30] [31] [32] [33] [34] [35] . Complement activation leads to the production of several effector pro-inflammatory molecules, including anaphylatoxins C3a and C5a. Overstimulation of the complement system or inadequate inhibition causes tissue damage [36] and the formation of high levels of anaphylatoxins. C5a and C3a also play important roles in inflammatory cascades [37, 38] . Following infection, complement anaphylatoxins stimulate phagocytic cells and the production of high levels of inflammatory cytokines (cytokine storm), granular enzymes, and free radicals. These mediators may eventually contribute to vascular dysfunction, fibrinolysis, microvascular thrombosis formation, or tissue damage [11, 12, 14, 15, 17, 18] . In this study, the expression levels of the pulmonary neutrophil chemoattractant chemokine, IL-8, C5a, and C3a were increased in MERS-CoV-infected patients and associated with a higher fatality rate. Our results are consistent with previous findings [39, 40] showing excessive complement activation in mouse models, particularly anaphylatoxins C3a, C5a, and C5b-9, during MERS-CoV and SARS-CoV-1 infection, which, in turn, contribute to lung tissue damage, a hyper-inflammatory response, and severe complications from the infection. Furthermore, several studies have revealed that C5a was associated with acute lung diseases, severe pneumonia, and immunopathology during highly pathogenic viral infection with H1N1, H5N1, H7N9, and SARS-CoV-1 [34, 35, 39, 41] . Similar to SARS-CoV-1 and MERS-CoV, patients with COVID-19 (SARS-CoV-2) are characterized by complement activation with high levels of complement protein [11, 29, 42, 43] . A rapid elevation of C3a variants (C3a, C3b, iC3b, C3c, C3d) was observed in mice infected with SARS-CoV-1, which contributed to the systemic inflammatory response and lung injury [39] . C3 activation has also been shown to be elevated in cells infected with SARS-CoV-2 [44] . In addition, in vitro and in vivo experiments on human respiratory syncytial viral infections showed complementmediated lung damage induced by high levels of C3a [45] . These findings clearly demonstrate that C5a and C3a recruit and activate inflammatory immune cells and play a central role in lung injury and immunopathology during respiratory viral infection. In contrast, complement C5a and C3a are involved in ARDS pathogenesis, neutrophil recruitment and activation, and lung endothelial and epithelial injuries [38, 46] . Recent data from COVID-19 patients showed that systemic complement activation is associated with inflammation and respiratory failure, as well as increased odds for oxygen therapy [47] . Moreover, MERS-CoV infection is associated with more severe pneumonia compared with SARS-CoV-1 infection [48] . ARDS was shown to be the main cause of mortality among patients infected with MERS-CoV, SARS-CoV-1, and highly pathogenic influenza virus [10, 49, 50] . In this study, we observed that almost all of the MERS-CoV-infected patients rapidly developed ARDS and required ICU admission. Therefore, we hypothesize that complement-induced ARDS may contribute to the disease severity and high mortality rate of MERS-CoVinfected patients observed in this study. We observed that the expression levels of pulmonary IL-8 (CXCL8) and C5a were significantly higher in MERS-CoV-infected patients compared with the MERS-CoV noninfected group. C5a contributes to the formation of neutrophil extracellular traps (NETosis) and inflammatory cytokine induction. IL-8 and C5a are important chemoattractants for neutrophil recruitment, activation, and neutrophil accumulation, and both induce NETosis. Excess NETosis contributes to inflammation, pathological cellular damage, and acute lung injury in mice infected by the influenza virus [51] [52] [53] . Similarly, high numbers of neutrophils and NETs were induced by C5a and contributed to the immunopathology, alveolar damage, and acute lung injury during influenza A H1N1 infection [51] . A number of in vitro and in vivo studies have found that C5a was associated with macrophage and endothelial cell activation, endothelial damage, NETosis, and increases in alveolar-capillary barrier permeability, as well as vascular leakage [37, 54] . The complement and tissue factors are contributing to the NETosis in COVID-19 immunothrombosis, suggesting the role of complement activation in the development of coagulopathy in COVID-19 patients [55] . Also, NETosis is associated with more severe COVID-19 disease [56] . Furthermore, SARS-CoV-2 infection induced high levels of IL-8 and markers linked with neutrophil activation which is associated with higher case fatality among COVID-19 patients [57, 58] . Thus, we hypothesize that high C5a, C3a, and IL-8 levels may play a vital role in lung tissue damage, immunopathology, ARDS development, ICU admission, and mortality in MERS-CoVinfected patients.

During SARS-CoV-1 infection, C5a induced several proinflammatory cytokines and chemokines including IL-8 [59] . C5a can also establish a positive feedback loop consisting of IL-8 induction, which results in further IL-8 production. Thus, a loop of continued IL-8 production may result in further inflammatory cell recruitment to the lung and subsequently contribute to lung damage and pathological changes [60] . We found that high levels of the lung complement anaphylatoxins, C5a and C3a, were closely associated with the overexpression of pulmonary IL-8 in MERS-CoV-infected patients. There was a significant correlation between C5a, C3a, and IL-8. The overproduction of C5a and IL-8 may be responsible for more damage to the host tissue compared with MERS-CoV. Previous studies have also shown that the levels of IL-8 significantly correlate with neutrophil numbers and airway inflammation, as well as lung dysfunction, in patients with chronic obstructive pulmonary disease and asthma [18, 61] . Therefore, we conclude that the high levels of C5a might be a direct mediator of neutrophil chemoattraction or an indirect inducer of IL-8 production during MERS-CoV infection.

C5a is also known to activate inflammatory cells to release reactive oxygen species (ROS). ROS overproduction leads to oxidative stress that subsequently contributes to airway and lung damage [62] [63] [64] . A previous in vivo study demonstrated that ROS is strongly associated with lung damage and pneumonia in mice infected with the influenza virus [65] . Mice treated with an antioxidant resulted in significantly reduced mortality, lung damage, and pathogenesis following influenza virus infection [66] . Several studies have observed that anti-C5a and a C5aR receptor antagonist significantly blocked and inhibited neutrophil oxidative burst formation [18, 67, 68] . These studies suggest a critical role of the C5a/C5aR/ROS axis in lung pathology and virusinduced immunopathology. We hypothesize that high levels of C5a induce ROS, which results in a more severe MERS-CoV infection, ARDS, and immunopathology.

Several studies have shown that targeted therapy with C5a and C5aR represents a significant anti-inflammatory approach to control inflammatory cell recruitment, immunopathology, and acute lung damage induced by highly pathogenic viral infections [34, 69, 70] . One study showed that the blockade of the C5a-C5aR axis in mice infected with MERS-CoV markedly reduced pathological changes in lung and spleen tissues, viral load, lymphopenia, and systemic and pulmonary inflammatory responses [40] . Another study showed that complement-deficient mice infected with SARS-CoV-1 were associated with decreased lung neutrophilia, a pro-inflammatory response, and viral replication [39] . Blocking and targeting C5a/C5aR and C3a/C3aR during respiratory viral infections significantly reduced and controlled pathology, lung damage, and mortality and inhibited inflammatory cell infiltration in the lung, T-lymphocyte apoptosis, and NETosis [34, 71] .

A recent study demonstrated that severe COVID-19 cases are associated with high levels of plasma C5a and soluble membrane attack complex (sC5b-9), signifying the C5a blockade as a potential intervention strategy [72, 73] . Several randomized controlled trials showed that anti-C5 therapy increased survival in severe COVID-19 cases and significantly reduced inflammatory marker production [72, [74] [75] [76] . These studies confirmed that the inhibition of an over-activated complement response and its signaling pathways significantly affected immunopathology, respiratory disease severity, and viral replication. Accordingly, it is reasonable to speculate that targeting the C5a/C5aR and C3a/C3aR axes may be effective at controlling MERS-CoV infection-induced immunopathology as MERS-CoV infection similarly leads to acute lung injury.

Over-activation of the complement system is controlled by a series of proteins known as the regulators of complement activation. These proteins play a key role in preventing complement-mediated tissue and cell damage and dysregulation of one or more of the complement regulatory proteins, which results in tissue injury, immunopathology, and inflammation-associated disease [77, 78] . The complement system is negatively regulated by several complement proteins, including factor I, C1-inhibitor (CI-INH), factor H, and C4-BP [79] [80] [81] [82] . In contrast, factor P is a positive regulatory complement protein. In this study, the levels of positive regulatory factor P were significantly higher in the lungs of MERS-CoV-infected patients compared with MERS-CoV non-infected group, suggesting that the levels of factor P may positively regulate complement activation during MERS-CoV infection [80] . Factor P has been associated with complement-mediated organ injuries in various human diseases. Therapy targeting factor P showed beneficial outcomes and prevented complement-mediated tissue damage [83] [84] [85] [86] [87] [88] [89] . The measurement of factor P may provide evidence for the involvement of the alternative complement pathway since factor P is an important factor in alternative pathway activation [90] . A recent study demonstrated that SARS-CoV-2 can directly activate the alternative complement pathway [73] . In contrast, the levels of negative regulatory proteins, factor I and C4-BP, were decreased in the lung of MERS-CoV-infected patients when compared with MERS-CoV non-infected group. These negative regulatory proteins play an important role in regulating the complement system. The low levels of factor I and C4-BP suggest that patients with MERS-CoV have a reduced capacity to control and regulate complement activation. These results indicate that MERS-CoV somehow suppressed and inhibited negative regulatory complement proteins during infection [47, 79, 80, 91] . A number of viral infection-mediated chronic inflammatory and autoimmunity diseases are associated with complement regulatory protein dysfunction [78, 80, 92, 93] . Over-activation of pulmonary and systemic complement plays a key role in inflammation, endothelial cell damage, thrombus formation, and intravascular coagulation and ultimately leads to multiple-organ failure and death [12, 18] . In this study, high levels of pulmonary complement mediators, disease severity, and increased mortality appear to be linked to the degree of complement activation against MERS-CoV. Complement C3a and C5a may be an independent risk factor for death in MERS-CoV-infected patients.

RANTES is a key proinflammatory chemokine produced during respiratory viral infection. Virus-infected lung and epithelial cells secret a high amount of RANTES. RANTES has a critical role in the platelet activation and initiation of the coagulation cascade [94] . In this study, we detected high levels of RANTES, this inflammatory chemokine was significantly correlated with death and ARDS among MERS-CoV-infected patients. In an in vitro experiment, infection of human monocyte-derived macrophages (MDMs) and dendritic cells (MDDCs) with MERS-CoV showed a high level and upregulation of RANTES and other inflammatory chemokines such as MIP-1α, IP-10, and IL-8 [95] . Recent studies showed that the severe and mild COVID-19 patients had elevated levels of RANTES [95] [96] [97] . Recent data from SARAS-CoV studies suggested targeting CCR5 could be a therapeutic strategy for COVID-19 [97] [98] [99] . Previous studies also showed increased levels of RANTES contributed to the exacerbation of allergic airway inflammation and severe human respiratory syncytial infection [100] [101] [102] .

Studying the protein-protein interaction networks and the predicted protein interactors provides significant data to explore the functions of proteins [103, 104] . In PPI networks, proteins that have direct interaction with several other proteins are called hub proteins (hub nodes). Proteins with more interaction partners may become targets for follow-up investigation [105] . In this study, the constructed PPI network (25 nodes and 149 edges) demonstrated that C3, C5, CCL5, CR1, CXCL8, IL10, IL-4 and CXCR1 were the hub proteins (nodes). Most of these hub proteins are involved in the inflammatory response and molecular binding interaction as well as receptor-ligand interactions. These results indicate that predicted proteins (interactors) may also have a role in MERS-CoV disease severity. The function and the exact role of hub proteins identified in our PPI network in MERS-CoV infection require further investigation.

Here, we propose a mechanism to explain the role of pulmonary complement anaphylatoxins (C3a and C5a), IL-8, and RANTES in severe MERS-CoV infection. High levels of complement anaphylatoxins C5a and IL-8 recruit and activate neutrophils. Subsequently, activated neutrophils undergo NETosis and ROS production, which results in oxidative stress. Increased levels of C5a and IL-8 may cause an inflammatory loop that contributes to extensive cellular damage and pathological changes. Also, the RANTES recruit and activate macrophages, and the elevation of complement anaphylatoxins C5a and C3a may induce cytokine storm and inflammatory cascades. On the other hand, RANTES recruit and activate macrophages while, C3a recruit, active, and degranulate mast cells and eosinophils which results in airway smooth muscle contraction. These meditators eventually contribute to airway and lung damage, more severe MERS-CoV infection, ARDS, and immunopathology. The overexpression of lung C5a during MERS-CoV infection may establish an amplification loop of IL-8 induction. Thus, a loop of continued IL-8 production leads to increased inflammatory cell activation and recruitment to the lung, subsequently contributing to the lung pathological features. Our results and hypothesis may explain the events of complement activation and its causal relation to the lung tissue damage during MERS-CoV infection.

The main limitation of this study is that we measured complement proteins, IL-8, RANTES levels and viral load at a single time point; measuring this mediator expression levels and viral load at different time points to create a kinetic profile might provide additional information. Also, we did not analyze the cellular components of the bronchoalveolar lavage samples. Future studies to close these gaps are needed.

We conclude that the high levels of complement anaphylatoxins, C5a and C3a; positive regulatory complement protein (factor P); IL-8; and CCL5 in the lower respiratory tracts of MERS-CoV-infected patients are associated with immunopathology, higher fatality rates, more severe disease, and ARDS development. High levels of complement mediators, disease severity, and increased mortality appear to be linked to the degree of complement activation against MERS-CoV. Furthermore, the levels of C3a, C5a, IL-8, and CCL5 in the lung may be useful biomarkers to predict a more severe MERS-CoV infection and mortality. Targeting any of these mediators may offer an effective treatment for MERS-CoV infection. As such, future large studies characterizing components of the complement system at different stages of MERS-CoV infection may offer an effective immunotherapeutic strategy.

The online version contains supplementary material available at https:// doi. org/ 10. 1007/ s10875-021-01061-z.

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The authors thank the Deanship of Scientific Research and RSSU at King Saud University for their technical support.Funding The authors thank the Research Center at King Fahad Medical City for funding this study (Grant No 019-053).

The datasets generated and/or analyzed during the current study are available from the corresponding author on reasonable request.

Ethics Approval and Consent to Participate This study was reviewed and approved by the Institutional Review Board at King Fahad Medical City (IRB register number 019-053). The study procedures were in accordance with the 1964 Helsinki Declaration and later versions.

The authors declare no competing interests.