key: cord-0895338-6gpzxqcl
authors: Ortillon, Marine; Coudereau, Remy; Cour, Martin; Rimmelé, Thomas; Godignon, Marine; Gossez, Morgane; Yonis, Hodane; Argaud, Laurent; Lukaszewicz, Anne‐Claire; Venet, Fabienne; Monneret, Guillaume
title: Monocyte CD169 expression in COVID‐19 patients upon intensive care unit admission
date: 2021-02-05
journal: Cytometry A
DOI: 10.1002/cyto.a.24315
sha: 52135805751daaaf033f029fc7c6daffb8744381
doc_id: 895338
cord_uid: 6gpzxqcl

During the second surge of COVID‐19 in France (fall 2020), we assessed the expression of monocyte CD169 (i.e., Siglec‐1, one of the numerous IFN‐stimulated genes) upon admission to intensive care units of 45 patients with RT‐PCR‐confirmed SARS‐CoV2 pulmonary infection. Overall, CD169 expression was strongly induced on circulating monocytes of COVID‐19 patients compared with healthy donors and patients with bacterial sepsis. Beyond its contribution at the emergency department, CD169 testing may be also helpful for patients' triage at the ICU to rapidly reinforce suspicion of COVID‐19 etiology in patients with acute respiratory failure awaiting for PCR results for definitive diagnosis.

The appearance of severe acute respiratory coronavirus-2 (SARS-CoV-2) has led to a rapidly spreading pandemic. 1 Since the first cases of coronavirus disease-19 (COVID-19), more than 73 million cases and 1.6 million deaths have been reported worldwide (by December, 16 -Johns Hopkins University). In areas particularly affected by virus spread, the tremendous number of patients coming to hospital threatened to overwhelm emergency departments (ED) and intensive care units (ICU) resources. Thus a crucial issue lied in the local capacity to rapidly test patients in order to confirm or rule out COVID-19 diagnosis and consequently optimize patients' triage. Diagnosis of COVID-19 was routinely achieved by detection of SARS-CoV-2 RNA in nasopharyngeal swabs via RT-PCR.

In response to viral infection, host cells immediately produce cytokines as a first alarm bell. 2, 3 Among these, type-I interferons (IFN-I) are crucial components of innate immune system against viruses.

IFN-I have, by themselves, antiviral properties but they also induce the expression of hundreds of IFN-stimulated genes (ISG) turning cells into antiviral status that limits virus spread. 2 Among various effects, IFN-I induce sharp rise in CD169 (also known as Siglec-1) expression on monocytes (mCD169) whereas this molecule is not expressed (or at very low levels) under baseline conditions. 4 Such overexpression is consequently easily detectable by flow cytometry. Therefore, increased mCD169 has been proposed, by itself, as a potential host marker of viral infections (e.g., HIV, influenza). Moreover, in conjunction with concomitant assessment of neutrophil CD64 (nCD64) expression, mCD169 was used to differentiate viral from bacterial infections. 5 Recently, along with increased plasma IFN-I concentration, mCD169 overexpression was observed in COVID-19 patients. 6 Within a pandemic context, this highlighted the interest of mCD169 as a rapid marker for the triage of patients with suspected COVID-19.

As this first work in COVID-19 reported on patients admitted to the ED, we investigated in prospective observational study whether CD169 overexpression would also be present in critically ill COVID-19 patients upon ICU admission.

Critically-ill patients admitted to ICUs from university hospitals (Hospices Civils de Lyon, Lyon, France) who presented with pulmonary infection with SARS-CoV2 confirmed by RT-PCR testing were prospectively included in the study. This study was part of an ongoing prospective observational clinical study (RICO, REA-IMMUNO-COVID) 7 and was registered at ClinicalTrials.gov (NCT04392401).

This study was approved by ethics committee (Comité de Protection des Personnes Ile de France 1-N IRB/IORG #: IORG0009918) under agreement number 2020-A01079-30. The committee waived the need for written informed consent because the study was observational. Nevertheless, oral information and non-opposition to inclusion in the study were mandatory and were systematically obtained before any blood sample was drawn and recorded in patients' clinical files. If a patient was unable to consent directly, non-opposition was obtained from the patient's legally authorized representative and reconfirmed from the patient at the earliest opportunity. Inclusion criteria were: patients aged >18 years, diagnosis of COVID-19 confirmed by RT-PCR testing in one respiratory sample. Exclusion criteria were pregnancy, institutionalized patients, inability to obtain informed consent.

As controls, patients with septic shock (bacterial infection) from the cohort IMMUNOSEPSIS 8 were included as well as healthy donors from Etablissement Francais du Sang (Lyon, F).

EDTA-whole blood samples were processed by flow cytometry according to a newly described one-step procedure (no wash, no centrifuge protocol). 9 For each blood sample tested, 500 μl of Versalyse In addition, to fit with results from multi-parametric paper in COVID-19, 10 results were also expressed as % of positive cells (positivity threshold was based on lack of CD169 expression on neutrophils).

Neutrophil CD64 results were expressed as MFI.

During the second surge of COVID-19 pandemic in France, between October 8th and December 8th, 2020, we enrolled 45 critically ill patients with positive SARS-CoV-2 RT-PCR. During the same period, we also included 2 ICU patients with septic shock and 12 healthy controls. Main demographic and characteristics are presented in Table 1 .

We observed a strong mCD169 overexpression in COVID-19 ICU patients and clear differences with septic shock or healthy donors with results expressed as MFI, percentages or ratio ( Figure 2 ). Original data for the measurements in the three patients groups are listed in Table S1 . When expressed as percentages of CD169+ monocytes, all COVID-19 patients except two expressed higher mCD169 than healthy donors and septic shock patients. Notably, in more than half of COVID-19 patients, almost all circulating monocytes expressed CD169. Regarding results as ratio, when applying the threshold recently proposed by Bedin et al. (i.e., 3.5), 6 77% of COVID-19 ICU patients presented with elevated results whereas all controls and septic patients were <3.5. Of note, although nCD64 values measured in COVID-19 patients were not as high as observed in septic shock patients, they were nevertheless elevated above healthy controls (data not shown). This might be due to putative co-infections as reported in COVID-19 patients arriving at the ICU. 11 

In areas particularly affected by the virus spread, the tremendous number of patients coming to hospital overwhelmed hospital resources. 12 As a consequence, the local capacity to rapidly test patients in order to confirm or rule out COVID-19 diagnosis and consequently optimize patients' triage has appeared as a major factor in the fight against COVID-19 pandemic. Due to the surge of patients, resources to address the diagnosis (routinely achieved by detection of SARS-CoV-2 RNA in nasopharyngeal swabs via RT-PCR) in a timely F I G U R E 1 Gating strategy (illustrative examples). Monocytes are first gated out from other cells on the basis of on SSC (side-scatter) / HLA-DR histogram (blue circle, left histogram) and CD169 is then measured on their surface (monoparametric histogram, right panel) as mean of fluorescence related to the entire monocyte population or as % of positive cells (positivity threshold, red cursor, was based on lack of CD169 expression on neutrophils). In addition, CD169 MFI was also determined on total lymphocyte population gated on SSC / FSC (forward-scatter) histogram (not shown) in order to provide results CD169 ratio (i.e., mCD169 MFI/lymphocyte CD169 MFI). One illustrative example of each group is depicted (healthy controls, septic shock, COVID-19) manner have been overwhelmed. Rapid antigen detection tests have been developed to identify active infection but, in their first generation, they lack sensitivity. Consequently, measurement of host marker reflecting viral infection has appeared as a sound approach. Unfortunately, IFN-I are produced at very low concentrations and most usual ELISA technologies are not able to quantify such low amount of cytokines (concentrations in fg/ml range). Only ultrasensitive digital Elisa (SIMOA) allows for the accurate IFN-I measurements but this technique is usually not available on a routine basis. The detection of ISG mRNA levels by molecular approach, although possible within the non-urgent context of auto-immunity, is not suitable to COVID-19 emergency due to extended time-to-results. 13, 14 Alternatively, overexpression of mCD169 (siglec-1, one of ISG) by whole blood flow cytometry has been recently proposed as a sensitive and specific surrogate marker of viral infection within the context of early COVID-19. 6 This marker was previously described as a tool, in conjunction with nCD64 expression, to discriminate bacterial from viral infections at emergency room. 5, 15 Specific kinetics of mCD169 expression in response to IFN-I has been described in vitro. 4 The main result of the present study is to show that, upon ICU admission, critically ill COVID-19 patients presented with strong mCD169 overexpression. Although altered IFN-I production is known to undoubtedly concur to the most severe forms of COVID-19, [16] [17] [18] mCD169 overexpression was still observed in this cohort. According to Bedin's threshold, almost 80% of patients were correctly identified as virally infected. Thus, in more severe patients, the present work reinforces the seminal description by Bedin et al. 6 It also extends the interest of mCD169 testing to larger cohorts of patients, especially those directly admitted to ICU for acute respiratory failure after sudden pulmonary worsening and without definitive diagnosis. Thus elevated mCD169 could help for patients triage in the ICU by reinforcing suspicion of COVID-19 etiology while awaiting for PCR results. mCD169 protocol is a one-step whole blood method that enables a streamlined flow cytometry sample preparation protocol. The simplified phenotyping procedure reduces training requirements and overcomes logistic constraints inherent to many flow cytometry applications (in particular due to the absence of compensation).

Reagents costs are limited (<5 €/test) and results may be provided in less than 45 min. Consequently, mCD169 may contribute to preserving hospital medical capacities by accelerating patients' triage.

By nature, this preliminary work, conducted during the second wave of pandemic in France presents with limitations. First, a larger cohort of ICU COVID-19 patients would be desirable to confirm these results. In addition, before drawing definitive conclusion, the inclusion of a cohort of mixed ICU patients with different etiologies (surgery, trauma, sepsis, burns) needs to be tested for mCD169 to precisely 

The authors certify that this manuscript reports original clinical research data. Individual data that underlie the results reported in this article are available from the corresponding author following publication, including the study report and study protocol. Additional data are available upon reasonable request.

This study was part of an ongoing prospective observational clinical study (RICO, REA-IMMUNO-COVID) and was registered at ClinicalTrials.gov (NCT04392401). This study was approved by ethics committee (Comité de Protection des Personnes Ile de France 1-N IRB/ IORG #: IORG0009918) under agreement number 2020-A01079-30. The committee waived the need for written informed consent because the study was observational. Nevertheless, oral information and nonopposition to inclusion in the study were mandatory and were systematically obtained before any blood sample was drawn and recorded in patients' clinical files. If a patient was unable to consent directly, non-opposition was obtained from the patient's legally authorized representative and reconfirmed from the patient at the earliest opportunity.

https://orcid.org/0000-0002-9961-5739

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SUPPORTING INFORMATION Additional supporting information may be found online in the Supporting Information section at the end of this article