key: cord-0728573-df5zpd4e
authors: Perez-Zsolt, Daniel; Muñoz-Basagoiti, Jordana; Rodon, Jordi; Elosua-Bayes, Marc; Raïch-Regué, Dàlia; Risco, Cristina; Sachse, Martin; Pino, Maria; Gumber, Sanjeev; Paiardini, Mirko; Chojnacki, Jakub; Erkizia, Itziar; Muñiz-Trabudua, Xabier; Ballana, Ester; Riveira-Muñoz, Eva; Noguera-Julian, Marc; Paredes, Roger; Trinité, Benjamin; Tarrés-Freixas, Ferran; Blanco, Ignacio; Guallar, Victor; Carrillo, Jorge; Blanco, Julià; Telenti, Amalio; Heyn, Holger; Segalés, Joaquim; Clotet, Bonaventura; Martinez-Picado, Javier; Vergara-Alert, Júlia; Izquierdo-Useros, Nuria
title: SARS-CoV-2 interaction with Siglec-1 mediates trans-infection by dendritic cells
date: 2021-11-15
journal: Cell Mol Immunol
DOI: 10.1038/s41423-021-00794-6
sha: 764291a72bbf537c31caf2d9a263c0f67c8751a5
doc_id: 728573
cord_uid: df5zpd4e

nan

infection but still contribute to viral pathogenesis. Lectins such as sialic acid-binding Ig-like lectin 1 (Siglec-1/CD169) mediate the attachment of viruses to APCs. Here, we show that APCs effectively capture SARS-CoV-2 within compartments via recognition of Siglec-1. This receptor interacts with sialylated gangliosides on membranes of SARS-CoV-2 variants, as previously shown for retroviruses or filoviruses [1] . Blockage of Siglec-1 on monocyte-derived dendritic cells (MDDCs) decreased SARS-CoV-2 viral transfer or trans-infection to bystander target cells. However, monocyte-derived macrophages (MDMs) capturing SARS-CoV-2 via Siglec-1 did not transmit infectious particles. The presence of pulmonary APCs co-expressing Siglec-1 and SARS-CoV-2 corroborated these findings in vivo.

We used the methodology described in the Supplementary Methods to dissect the contribution of Siglec-1 to SARS-CoV-2 pathogenesis. Siglec-1 expression is induced on APCs upon IFN-α or LPS exposure and increased in myeloid cells of COVID-19 patients [2] . Here, we tested whether this lectin could bind SARS-CoV-2 via recognition of sialylated gangliosides on viral membranes. APCs captured incoming SARS-CoV-2 in cellular compartments, eventually leading to viral degradation (Supplementary Fig. 1,2 ). Raji B cell lines transfected with different lectins ( Supplementary Fig. 3A ) were pulsed with SARS-CoV-2, washed and assessed by ELISA to measure cell-associated viral nucleocapsid content (Fig. 1A) . While Raji cells trasnfected with wild-type Siglec-1 captured SARS-CoV-2, cells transfected with DC-SIGN, Siglec-5, Siglec-7 or devoid of these lectins did not (Fig. 1A) . Viral uptake via Siglec-1 relied on the recognition of sialylated ligands, as observed with Raji cells transfected with the Siglec-1 mutant R116A, which lacks sialic acid recognition capacity and did not trap SARS-CoV-2 (Fig. 1A) . Raji cells pretreated with the α-Siglec-1 monoclonal antibody (mAb) 7-239 reduced SARS-CoV-2 uptake ( Supplementary Fig. 3B ). SARS-CoV-2 variants were equally trapped via Siglec-1 but not by the mutated Siglec-1 R116A, indicating that sialic acid recognition is critical (Fig. 1B) . Superresolution microscopy of SARS-CoV-2 confirmed that GM1, one of the sialyllactose-containing gangliosides interacting with Siglec-1 [1] , was detectable on 74% of virus particles (Fig. 1C ). MDMs and MDDCs treated with IFN-α to induce Siglec-1 expression displayed higher SARS-CoV-2 uptake than nonactivated cells (Fig. 1D) , and uptake was blocked by the α-Siglec-1 mAb 7-239 (Fig. 1E ). These complementary approaches identified Siglec-1 as a central molecule mediating SARS-CoV-2 uptake via sialic acid recognition.

Once Siglec-1 binds to HIV-1 or Ebola viruses, receptors polarize and engulf particles within viral-containing compartments (VCCs) that are continuous with the plasma membrane and connected to the extracellular space [1] . To elucidate whether Siglec-1 also recruits SARS-CoV-2 to VCCs, we used confocal and electron microscopy and found Siglec-1-positive VCCs containing viral particles on activated MDDCs (Fig. 1F , G and Movie 1). Siglec-1 has a dual role in enhancing infectivity, either facilitating fusion on APCs, as is the case for the Ebola virus, or mediating transmission to other target cells in trans, as is the case for retroviruses [1] . Since SARS-CoV-2 fusion on APCs is limited ( Supplementary  Fig. 1B) , we explored the relevance of viral trans-infection. Raji cells were exposed to SARS-CoV-2, washed and cocultured with targets expressing or not expressing ACE2 (Fig. 1H ). Raji Siglec-1 cells cocultured with ACE2-expressing cells released higher amounts of SARS-CoV-2 than cells expressing the R116A mutant (Fig. 1H) . A minimal viral amount was detected in cocultures with cells lacking ACE2, excluding SARS-CoV-2 replication on Raji cells or the release of initially trapped viruses (Fig. 1H ). IFN-α-treated MDDCs cocultured with ACE2-and TMPRSS2-expressing target cells released higher amounts of SARS-CoV-2 than MDMs (Fig. 1I) . Experiments with nonreplicative HIV-1 pseudotyped with SARS-CoV-2 spike confirmed Siglec-1 transmission of SARS-CoV-2 via ACE2-dependent fusion on target cells (Supplementary Fig. 4) . Hence, SARS-CoV-2 retention on MDDCs via Siglec-1 allows trans-infection. Lung immunohistochemistry analysis from a SARS-CoV-2infected rhesus macaque used in a previous study [3] confirmed the codetection of Siglec-1 and viral nucleocapsid in cells with myeloid morphology (Fig. 1J ). Single-cell RNA sequencing data previously collected in African green monkeys (AGMs) allowed us to focus on pulmonary APCs ( Supplementary Fig. 5) , where SARS-CoV-2 infection upregulated SIGLEC1 expression 3 days postinoculation (dpi) (Supplementary Fig. 6A ). Viral RNA was detected in high numbers at 3 dpi, but the levels decreased at 10 dpi ( Supplementary Fig. 6B) , consistent with the resolution of infection in this mild COVID-19 model. When we compared the expression of SIGLEC1 on APCs without or with associated viral RNA, only alveolar and interstitial macrophages containing viral RNA significantly increased SIGLEC1 expression (Fig. 1K) . Thus, infection triggers SIGLEC1 expression on all APCs, but this phenomenon is not linked to the detection of cell-associated viral RNA. We next analyzed the most detailed single-cell atlas [4] of human lungs of COVID-19 patients with advanced disease and controls (Supplementary Fig. 7A-B) . Here, APCs were enriched for viral RNA but lacked ACE2 and TMPRSS2 viral entry receptors ( Supplementary  Fig. 7C ). Pulmonary myeloid cells were enriched in COVID-19 patients as compared to those in controls ( Fig. 1L ; Supplementary  Fig. 8A-E) , and SIGLEC1-expressing APCs were also enriched ( Fig. 1M; Supplementary Fig. 8F ). Twenty percent of pulmonary APCs expressing viral RNA also coexpressed SIGLEC1, whereas none coexpressed other lectins or viral receptors (Fig. 1N) . These results corroborated the presence of the Siglec-1 receptor or transcripts on APCs containing SARS-CoV-2 in vivo. Targeting Siglec-1 or trans-infection [5] could offer cross-protection against SARS-CoV-2 and other enveloped viruses that exploit APCs for viral dissemination and lead to the development of new broadspectrum antivirals for future outbreaks.

When dendritic cells go viral: the role of siglec-1 in host defense and dissemination of enveloped viruses

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Baricitinib treatment resolves lower-airway macrophage inflammation and neutrophil recruitment in SARS-CoV-2-infected rhesus macaques

COVID-19 tissue atlases reveal SARS-CoV-2 pathology and cellular targets

Lectins enhance SARS-CoV-2 infection and influence neutralizing antibodies

We acknowledge J. Díaz from the CMCiB for his constant help at the BSL3 facility. We thank C. Esteban from the microbiology department of HUGTiP for identifying two different variants used in this study. We also thank M. Parera from IrsiCaixa for her outstanding help in sequencing viral variants. We are grateful to E. Rebollo from the Molecular Imaging Platform, IBMB-CSIC. We would like to thank the Advanced Light Microscopy Unit at the Centre for Genomic Regulation (CRG), Barcelona (Spain), for access to the Leica STED microscope. The research of the CBIG consortium (constituted by IRTA 

Correspondence and requests for materials should be addressed to Javier Martinez-Picado, Júlia Vergara-Alert or Nuria Izquierdo-Useros.

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