key: cord-0698759-ah0qum3e
authors: Cherubini, Fabio; Cristiano, Antonio; Valentini, Alessandra; Bernardini, Sergio; Nuccetelli, Marzia
title: Correction to: Circulating calprotectin as a supporting inflammatory marker in discriminating SARS-CoV-2 infection: an observational study
date: 2021-11-18
journal: Inflamm Res
DOI: 10.1007/s00011-021-01512-8
sha: 92f224719faac57a839aef6e2db6dadcc3dd710a
doc_id: 698759
cord_uid: ah0qum3e

nan

Calprotectin (CLP) is a calcium and zinc-finger heterodimer (36.5 kDa) formed by proteins S1008 and S1009. It belongs to S100 calcium binding protein family comprising small acidic proteins with high solubility in 100% ammonium sulfate solution, thus the name S100 [1] . CLP has different synonyms. It was first called leukocyte protein L1 [2] ; current names are myeloid-related-proteins-8 and -9 (MRP8, MRP9) owing to its abundance in neutrophils, monocytes and early-differentiated macrophages [3] , where it represents 5% of the total proteins and 60% of the cytosolic proteins, respectively, and calgranulin (A and B) linked to distinctive calcium-binding properties in granulocytes [4] .

CLP is a potent antimicrobial protein: an initial proinflammatory stimulus triggers its production via Toll-Like Receptor 4 (TLR4) expressed on granulocytes [5] . CLP release prevents bacterial growth by impairment of zincdependent enzymes upon zinc (Zn) sequestration. Indeed, mounting evidence proves the effect of CLP against several bacterial species such as Escherichia coli and Staphylococcus aureus among others, along with fungistatic function [6, 7] .

CLP involvement in inflammatory process is broadly known: first, granulocytes increase CLP expression and secretion upon inflammatory stimuli, then CLP acts as a cytokine-like protein by binding surface receptors and triggering pathways engaged in mounting immune response. Conversely, CLP exerts an immune-regulatory role by chelation of Zn divalent cations, thus resulting in zinc-dependent metalloproteinases inhibition, responsible for activation of pro-inflammatory cytokines such as tumor necrosis factor (TNF) [8] . Furthermore, CLP drives several cellular processes via calcium homeostasis regulation, such as rearrangement of cytoskeletal components, cell cycle progression, proliferation, migration and survival. Collective data agree with the idea of CLP as a smart molecule in which its function outcome depends on concentration and intra-or extracellular localization [9] .

CLP is found in various body fluids such as serum and synovial liquid in proportion to the severity of any existing inflammation. Indeed, serum levels are usually reported below 1 μg/ml in healthy subjects, but during inflammation they may increase by 100 times [10] . Besides, healthy subjects' concentration in feces is about six times that of normal plasma [11] . Therefore, CLP promptly became a reliable biomarker in inflammatory diseases including inflammatory bowel diseases (IBDs), rheumatoid arthritis, cystic fibrosis, chronic bronchitis, many types of cancers and neurodegenerative disorders, such as Alzheimer [12] [13] [14] . Accordingly, stool levels in IBDs are routinely measured, thus representing the gold standard to assess inflammation status in patients and providing important hints for clinical examinations to be made in the follow-up (e.g., colonoscopy) [15] .

To our knowledge, few studies on circulating CLP have been published in the context of SARS-CoV-2 infection and most of them report serum analysis [16] [17] [18] . However, data show that CLP yields on ethylene-diamine-tetra-acetic acid (EDTA) plasma are lower than on serum, due to EDTA inhibitory effect on CLP release from neutrophils in vitro [19] . Furthermore, as the release of CLP is strongly accelerated during blood clotting, EDTA plasma is preferable to obtain levels closer to baseline [20] .

Currently, inflammatory status assessment relies mainly on few classical tests like C-reactive protein (CRP) and erythrocyte sedimentation rate (ESR). In this scenario, an inflammatory marker algorithm which grants information about the expected detrimental effects and retains the prognostic value in most of the diseases is desirable. CLP feasibility as a standard test in laboratory repertoire is supported by evidence of sustained employment in gastrointestinal inflammation and consistent reports of plasma dosage in autoimmune diseases such as rheumatoid arthritis [10] . Therefore, CLP can be considered as a candidate biomarker in the laboratory analysis for the evaluation of the inflammation status, thus also providing insights about improving risk stratification strategies in the plethora of inflammationdriven diseases.

Under these circumstances, SARS-CoV-2 pandemic raised the need to have a battery of preliminary serological tests that can be prognostic for positivity to nasopharyngeal swab regardless of the severity of symptoms. Indeed, in situations where is not possible to perform swab tests, the score provided by reliable analytes can improve the management of patients and may indicate subsequent diagnostic investigation. In this retrospective observational study, we detected circulating calprotectin (cCLP) levels in patients with confirmed positive nasopharyngeal swab RT-PCR compared to patients with confirmed negative nasopharyngeal swab RT-PCR, as well as healthy controls, to evaluate the clinical outcome predictivity, thus suggesting CLP-positive correlation with COVID-19 onset. 

Nasopharyngeal swabs were tested for SARS-CoV-2 infection with Seegene AllplexTM2019-nCoV Assay (Seegene, Seoul, South Korea), according to the manufacturer's protocols. Automated RNA extraction and PCR setup were carried out using Seegene NIMBUS, a liquid handling workstation. RT-PCR was run on a CFX96TMDx platform (Bio-Rad Laboratories, Inc., CA, USA) and subsequently interpreted by Seegene's Viewer Software. The Seegene All-plexTM2019-nCoV Assay identifies the virus by multiplex real-time PCR targeting of three viral genes (E, RdRP and N), thus complying with the international validated testing protocols.

The "QUANTA Flash Calprotectin" kit (INOVA Diagnostics Inc., San Diego, CA, USA) is a chemiluminescent immunoassay for the quantitative calprotectin determination in human samples, performed on the fully automated BIO-FLASH Instrument (INOVA Diagnostics Inc., San Diego, CA, USA), at 37 °C. The principle of the test is a "sandwich immunoassay" where calprotectin-specific capture antibodies are coated on paramagnetic beads. An aliquot of patient sample, antibody-coupled beads and assay buffer are combined in a cuvette. The beads are then magnetized, washed several times until isoluminol-conjugated anti-calprotectin antibodies are added, developing a luminescent reaction when "trigger" reagents are mixed to the cuvette. The light produced from this reaction is measured as relative light units (RLUs) by the BIO-FLASH optical system. RLU values are proportional to the amount of bound isoluminol conjugate, which in turn is proportional to the amount of calprotectin captured on the surface of the beads. By running three calibrators, an instrument-specific working curve is created, which is used by the software to calculate ng/ml values from the RLU obtained for each sample. Considering the 1:23 pre-dilution factor performed by the BIO-FLASH Instrument on the samples measured with "QUANTA Flash Calprotectin" kit, all the calprotectin concentration values must be multiplied for a k factor of 0.023 to obtain µg/ml.

High-sensitivity C-reactive protein (hsCRP) was determined in serum by a latex immunoassay for quantitative immunoturbidimetric detection with a commercial kit performed on the Architect c16000 analyzer ("CRP Vario" assay, Abbott Laboratories, Chicago, USA). The hsCRP levels were reported in mg/l (reference range 0-5 mg/l). Fibrinogen quantitative determinations in human citrated plasma samples were performed on the ACL Top 550 CTS Coagulation analyzer (IL-Instrumentation Laboratory, Bedford, USA), using the Clauss method based on the fibrinogen ability to form fibrin clot after being exposed to a high concentration of purified thrombin and by comparing sample thrombin clotting time against a plasma standard (reference range 238-498 mg/dl).

Erythrocyte sedimentation rate (ESR) measurements were performed by capillary photometric-kinetic technology on the fully automated Test 1 SDL analyzer (Alifax S.p.A., Padova, Italy). Whole blood samples are delivered into a capillary tube where they are accelerated via a "stoppedflow" circuit, which causes sedimentation of erythrocytes. Results are transformed to Westergren values (reference range males 2-25 mm/h, females 2-30 mm/h).

IL-6 levels (reference range 0-50 pg/ml) were measured by an automated chemiluminescent assay on the Immulite 2000 instrument (Siemens, Milan, Italy). TNF-α levels (reference range 0-12.4 pg/ml) were detected by an automated enzyme-linked immunosorbent assay (ELISA) performed on the Immunomat analyzer (Institut Virion/Serion, Wurzburg, Germany).

White blood cell (WBC) count was determined by an automated hematological analyzer (Dasit-Sysmex, Milan, Italy). We also determined the neutrophil-to-lymphocyte ratio (NLR) as a marker of systemic inflammation.

Results were calculated by Mann-Whitney test. Statistical significance was defined as p < 0.05. Specificity and sensitivity were calculated by receiver operating characteristic curves (ROC curve). All data were analyzed using GraphPad Prism Software 8.0.1 (San Diego, California, USA). The investigators were blinded to the group allocation during the experiment.

To evaluate cCLP as a reliable marker of inflammation in the context of SARS-CoV-2 infection, we initially compared hospitalized COVID-19 patients to healthcare workers screened negative to nasopharyngeal swab for SARS-CoV-2, by analyzing cCLP levels in serum. As expected, our cohort shows a statistically significant difference between the two groups, thus confirming the increase of calprotectin median concentration in the serum of patients with COVID-19 (292.7 ng/ml; range 19.13-3642 ng/ml) vs negative RT-PCR control group (143.9 ng/ml; range 13.91-508.4 ng/ml) ( Table 1 ; Fig. 1 ).

Later on, considering that cCLP stability is established by evaluation on plasma, we took advantage of samples collected from patients' first access to the emergency department with positive or negative results to nasopharyngeal swab RT-PCR for SARS-CoV-2, exploiting as control group healthcare workers and outpatient users from Tor Vergata Hospital with negative inflammation markers (i.e., CRP < 0.1 mg/l, ESR < 2 mm/h).

Statistical analysis on calprotectin values provided interesting significant differences among the groups: overall median results confirmed cCLP increase in plasma of patients who tested positive for nasopharyngeal swab (222.7 ng/ml; range 48.35-1621 ng/ml) with respect to patients with negative swab (104.8 ng/ml; range 32.17-1022 ng/ml) and to the control group (32.87 ng/ml; range 14.00-152.20 ng/ml) (Table 1; Fig. 2 ).

Based on this excellent evidence, we calculated the specificity and sensitivity using receiver operating characteristic curves (ROC curves). On comparing controls and patients with negative RT-PCR, an area under curve (AUC) value of 0.8872 was achieved, with a sensitivity of 83.05% and a specificity of 80.28% at a cutoff value of 76.45 ng/ml. Intriguingly, matching controls with the positive RT-PCR group, we obtained an AUC value of 0.9684, with a sensitivity of 92.31% and specificity of 94.37% at a cutoff value of 93.04 ng/ml. Finally, the ROC curve resulting from negative and positive RT-PCR group comparison shows an AUC value of 0.7257 with a specificity of 70.77% and a sensitivity of 69.49% at a cutoff value of 131.3 ng/ml, thus suggesting that cCLP can be considered as an inflammation marker able to discriminate between negative and positive patients to SARS-CoV-2 infection, with the best fit cutoff that emerged from our data analysis Fig. 3 ). All the calprotectin concentration values must be multiplied for a k factor of 0.023 to obtain µg/ml. Since cCLP has been suggested as a reliable biomarker of inflammation in several diseases, we first tested the correlation with two parameters frequently increased in most of COVID-19 longitudinal studies, such as CRP and fibrinogen (FBG) by means of Pearson's test. Accordingly, cCLP correlates positively with CRP and FBG (r = 0.69: r = 0.7, respectively) in negative swab patients; the correlation is maintained in positive swab patients, though to a lesser extent (r = 0.366; r = 0.378).

We also retrospectively analyzed IL-6 and TNF-α levels, known to be involved in the "cytokine storm". Based on the tests requested by the clinicians at the same time as the assessment of calprotectin levels, we found results only in 35 out of 65 positive RT-PCR patients and no data on negative RT-PCR patients: IL-6 levels were over threshold in 19 patients (median 57.2 pg/ml; range 2.42-5000 pg/ml); TNF-α levels were over threshold in 13 patients (median 7.55 pg/ml; range 1.78-142 pg/ml) and only 10 out of 35 patients were positive for both IL-6 and TNF-α.

Moreover, since calprotectin represents 60% of neutrophils' granule content, we could reasonably suggest that the calprotectin analyzed in the plasma was of neutrophil derivation. To this end, we retrospectively analyzed the neutrophil and lymphocyte counts. As expected, our cohort showed a significant increase in median neutrophil count in positive RT-PCR patients (8.35 × 10 3 /µl; range 2.3-43.69 × 10 3 / µl) compared to negative RT-PCR patients (5.69 × 10 3 /µl; range 0.66-24.2); p value = 0.0123. Conversely, median lymphocyte count showed higher values in negative RT-PCR patients (1.16 × 10 3 /µl; range 0.37-9.49 × 10 3 /µl) than positive RT-PCR patients (0.91 × 10 3 /µl; range 0.06-2.96 × 10 3 / µl); p value p = 0.0224. In addition, our data showed an increased neutrophil-to-lymphocyte ratio in positive RT-PCR patients compared to negative RT-PCR patients (9.17 vs 4.9, respectively; p value = 0.0002), corroborating other studies in which NLR is considered a systemic inflammatory biomarker as well as a prognostic factor in SARS-CoV-2 infection [21, 22] .

In the last 20 years, considerable evidence has developed that supports the use of fecal calprotectin as a marker of intestinal inflammation. However, several studies have reported that circulating calprotectin proves to be an excellent marker capable of providing relevant information about subclinical inflammation in patients suffering from diseases such as rheumatoid arthritis and cystic fibrosis [10, 14] . SARS-CoV-2 pandemic in 2020 has put a strain on the health systems in several countries with profound repercussions on the global economy and societies. In this scenario, an urgent need arises for fast, reliable tests and markers that can support and guide diagnostic responses, giving first important clinical information in SARS-CoV-2-positive patients.

In this observational study, we sought to investigate the efficacy of circulating calprotectin as a marker of inflammation in the context of SARS-CoV-2 infection, using blood samples from patients taken at Tor Vergata Hospital COVID Center of Rome. Serum analysis of COVID-19 hospitalized patients showed that circulating calprotectin median levels were significantly higher than that of the control population (143.9 ng/ml vs 292.7 ng/ml, respectively; p value < 0.0001), confirming that calprotectin could be routinely used to discriminate well between healthy and pathological patients.

Subsequent studies were focused on circulating calprotectin in plasma of patients who accessed the emergency department of Tor Vergata Hospital for suspected SARS-CoV-2 infection. Notably, plasma employment for calprotectin dosage is recommended, as the presence of EDTA prevents massive calprotectin release by granulocytes, thus ensuring lower concentrations but closer to real values of circulating protein. As expected, plasma calprotectin has higher median levels in patients with suspected SARS-CoV-2 infection, but negative to RT-PCR, when compared to the control group (104.8 ng/ml vs 32.87 ng/ml respectively; p value < 0.0001). Noteworthy, these differences are significantly increased in case of confirmed RT-PCR positivity, showing overall higher median calprotectin values (222.7 ng/ml; p value < 0.0001). All the calprotectin concentration values must be multiplied for a k factor of 0.023 to obtain µg/ml.

Calprotectin could therefore be a marker capable of distinguishing clearly between COVID-19-positive and -negative patients. Furthermore, ROC curve results explored the discrimination ability of circulating plasma calprotectin. The comparison between positive RT-PCR patients and negative control group shows that circulating calprotectin is a good inflammatory marker as it affords high percentages of sensitivity and specificity (92.31%, 94.37%; respectively) with an AUC = 0.9684, considering a best fit cutoff value > 93.04 ng/ml. However, the application of this cCLP concentration does not allow differentiating between patients with confirmed SARS-CoV-2 infection from patients with negative swab tests. Therefore, taking for comparison only samples from patients with suspicion of infection grouped by certified RT-PCR positivity/ negativity, we obtained a best fit cutoff value > 131.3 ng/ ml, which allows to better distinguish patients infected by SARS-CoV-2. Accordingly, the lowering in sensitivity and specificity (70.77%, 69.49%; respectively) is due to the comparison performed on a patient control group with somewhat ascertained inflammatory status that does not reflect the general population.

Since calprotectin is mainly released from neutrophils' granules content and neutrophils are the first responders to many infections, we also analyzed the neutrophil and lymphocyte counts according to evidence of their recruitment in the immune response triggered by SARS-CoV-2 [23] [24] [25] . Our data showed a higher median neutrophil count in positive RT-PCR patients compared to negative RT-PCR patients, in contrast with a lower median lymphocyte count in positive RT-PCR patients compared to negative RT-PCR patients.

In addition, we found an increased NLR in positive RT-PCR patients compared to negative RT-PCR patients, supporting the results in recent literature proposing increased neutrophil counts and lymphocytopenia as typical clinical features in COVID-19 patients and confirming the same trend for the circulating calprotectin levels [26] .

Furthermore, it is well known that toll-like receptor (TLR) can be stimulated by calprotectin leading to release of pro-inflammatory cytokines and the so-called "cytokine storm" can develop in severe cases of COVID-19, which exacerbates the damage caused by the infection [5, 27] . In this line, we found IL-6 and TNF-α levels over threshold in 19 and 13 positive RT-PCR patients, respectively. Since, peripheral blood calprotectin is mainly neutrophil derived and circulating calprotectin can stimulate TLR, leading to expression and release of pro-inflammatory cytokines, it could presumably be considered as an early and more informative marker in the inflammation context compared to the "cytokine storm" [5, 28] .

Finally, correlation analysis was positive for C-reactive protein and fibrinogen, thus demonstrating that circulating calprotectin acts as an excellent marker in the inflammatory setting.

Moreover, several studies propose circulating calprotectin in the prognosis of different inflammation-elicited diseases, as well as assessing subclinical inflammation in patients [29] ; therefore, cCLP should be definitely considered in a panel of markers aimed at investigating the inflammation state.

Summing up, this study is strengthened by a relatively large sample size compared to other research about circulating calprotectin detection in the context of SARS-CoV-2 infection and is the first to our knowledge that explores calprotectin performance using plasma, as well as serum samples, from infected patients.

All these add up to other remarkable insights proposing circulating calprotectin as a new, quantitative and convenient marker in the assessment of inflammatory diseases.

Besides, since CLP assessment is currently mostly applied to inflammatory bowel diseases, it could be relevant to investigate the relationship between fecal and circulating CLP in COVID-19 patients with gastrointestinal manifestations for further important evidence of its diagnostic value as a promising marker in COVID-19.

Unfortunately, our work has some limitations. The population of the study was chosen on the basis of available samples collected on the same day of the first access to the emergency department. As a consequence, we had no information regarding the presence of concomitant diseases. Therefore, in light of the aim of the study, RT-PCR positivity/negativity outcome was the only inclusion/ exclusion criterion considered.

Furthermore, according to hospital data access policy, we cannot provide any further information on medical records and on the clinical status of the patients, except for laboratory medicine department results.

In conclusion, our data suggest that circulating calprotectin along with being of interest as a generic inflammatory marker may provide important indications in the context of SARS-CoV-2 infection.

Of course, additional studies are required to confirm circulating plasma calprotectin assay as a support for the diagnosis of SARS-CoV-2 infection by larger samples size, taking advantage of longitudinal and retrospective studies.

A soluble protein characteristic of the nervous system

A radioimmunoassay for a granulocyte protein as a marker in studies on the turnover of such cells

MRP-8 and MRP-14, two abundant Ca(2+)-binding proteins of neutrophils and monocytes

Identification of p8,14 as a highly abundant heterodimeric calcium binding protein complex of myeloid cells

Phagocyte-derived S100 proteins in autoinflammation: putative role in pathogenesis and usefulness as biomarkers

Nickel Sequestration by the host-defense protein human calprotectin

Nutrient metal sequestration by calprotectin inhibits bacterial superoxide defense, enhancing neutrophil killing of Staphylococcus aureus

Mrp8 and Mrp14 are endogenous activators of Toll-like receptor 4, promoting lethal, endotoxin-induced shock

Calprotectin (S100A8/S100A9): a key protein between inflammation and cancer

Calprotectin in rheumatic diseases: a review

Calprotectin as a diagnostic tool for inflammatory bowel diseases

Mechanism of apoptosis induced by S100A8/A9 in colon cancer cell lines: the role of ROS and the effect of metal ions

Emerging role of calprotectin in gastroenterology

Calprotectin in cystic fibrosis

Assessment of the neutrophil dominating protein calprotectin in feces: a methodologic study

Circulating levels of GDF-15 and calprotectin for prediction of in-hospital mortality in COVID-19 patients: a case series

Neutrophil calprotectin identifies severe pulmonary disease in COVID-19

Elevated serum levels of S100A8/A9 and HMGB1 at hospital admission are correlated with inferior clinical outcomes in COVID-19 patients

Calprotectin (S100A8/A9) should preferably be measured in EDTA-plasma

results from a longitudinal study of patients with rheumatoid arthritis

Plasma calprotectin is superior to serum calprotectin as a biomarker of intestinal inflammation in ulcerative Colitis

Neutrophil-tolymphocyte ratio predicts critical illness patients with 2019 coronavirus disease in the early stage

Neutrophilto-lymphocyte ratio as an independent risk factor for mortality in hospitalized patients with COVID-19

Cytokine storm and leukocyte changes in mild versus severe SARS-CoV-2 infection: Review of 3939 COVID-19 patients in China and emerging pathogenesis and therapy concepts

A meta-analysis of SARS-CoV-2 patients identifies the combinatorial significance of D-dimer, C-reactive protein, lymphocyte, and neutrophil values as a predictor of disease severity

Continuous tracking of COVID-19 patients' immune status. Int Immunopharmacol

Neutrophils and COVID-19: the road so far

The cytokine storm and COVID-19

The expression of calprotectin and factors in TLR4/NF-κB/MyD88 pathway in patients with idiopathic acute anterior uveitis

Calprotectin in rheumatic diseases

The original article can be found online at https:// doi. org/ 10. 1007/ s00011-021-01465-y.

The authors would like to thank the Clinical Biochemistry Laboratory staff of Tor Vergata Hospital, for their support; INOVA Diagnostics Inc. and Werfen Instrumentation Laboratory SpA, for kindly having provided kits and instrument for this study.