key: cord-0896207-y4oeeelf
authors: Picchianti-Diamanti, Andrea; Aiello, Alessandra; Laganà, Bruno; Agrati, Chiara; Castilletti, Concetta; Meschi, Silvia; Farroni, Chiara; Lapa, Daniele; Najafi Fard, Saeid; Cuzzi, Gilda; Cimini, Eleonora; Grassi, Germana; Vanini, Valentina; Di Rosa, Roberta; Salemi, Simonetta; Nalli, Gabriele; Salmi, Andrea; Repele, Federica; Altera, Anna Maria Gerarda; Maffongelli, Gaetano; Palazzolo, Claudia; Vita, Serena; Leone, Sara; Puro, Vincenzo; Capobianchi, Maria Rosaria; Ippolito, Giuseppe; Nicastri, Emanuele; Goletti, Delia
title: ImmunosuppressiveTherapies Differently Modulate Humoral- and T-Cell-Specific Responses to COVID-19 mRNA Vaccine in Rheumatoid Arthritis Patients
date: 2021-09-14
journal: Front Immunol
DOI: 10.3389/fimmu.2021.740249
sha: 6ae4cbb824cde25ca7dff140974635e0abef3ff2
doc_id: 896207
cord_uid: y4oeeelf

OBJECTIVE: To assess in rheumatoid arthritis (RA) patients, treated with different immunosuppressive therapies, the induction of SARS-CoV-2-specific immune response after vaccination in terms of anti-region-binding-domain (RBD)-antibody- and T-cell-specific responses against spike, and the vaccine safety in terms of clinical impact on disease activity. METHODS: Health care workers (HCWs) and RA patients, having completed the BNT162b2-mRNA vaccination in the last 2 weeks, were enrolled. Serological response was evaluated by quantifying anti-RBD antibodies, while the cell-mediated response was evaluated by a whole-blood test quantifying the interferon (IFN)-γ-response to spike peptides. FACS analysis was performed to identify the cells responding to spike stimulation. RA disease activity was evaluated by clinical examination through the DAS28crp, and local and/or systemic clinical adverse events were registered. In RA patients, the ongoing therapeutic regimen was modified during the vaccination period according to the American College of Rheumatology indications. RESULTS: We prospectively enrolled 167 HCWs and 35 RA patients. Anti-RBD-antibodies were detected in almost all patients (34/35, 97%), although the titer was significantly reduced in patients under CTLA-4-inhibitors (median: 465 BAU/mL, IQR: 103-1189, p<0.001) or IL-6-inhibitors (median: 492 BAU/mL, IQR: 161-1007, p<0.001) compared to HCWs (median: 2351 BAU/mL, IQR: 1389-3748). T-cell-specific response scored positive in most of RA patients [24/35, (69%)] with significantly lower IFN-γ levels in patients under biological therapy such as IL-6-inhibitors (median: 33.2 pg/mL, IQR: 6.1-73.9, p<0.001), CTLA-4-inhibitors (median: 10.9 pg/mL, IQR: 3.7-36.7, p<0.001), and TNF-α-inhibitors (median: 89.6 pg/mL, IQR: 17.8-224, p=0.002) compared to HCWs (median: 343 pg/mL, IQR: 188-756). A significant correlation between the anti-RBD-antibody titer and spike-IFN-γ-specific T-cell response was found in RA patients (rho=0.432, p=0.009). IFN-γ T-cell response was mediated by CD4(+) and CD8(+) T cells. Finally, no significant increase in disease activity was found in RA patients following vaccination. CONCLUSION: This study showed for the first time that antibody-specific and whole-blood spike-specific T-cell responses induced by the COVID-19 mRNA-vaccine were present in the majority of RA patients, who underwent a strategy of temporary suspension of immunosuppressive treatment during vaccine administration. However, the magnitude of specific responses was dependent on the immunosuppressive therapy administered. In RA patients, BNT162b2 vaccine was safe and disease activity remained stable.

reduced in patients under CTLA-4-inhibitors (median: 465 BAU/mL, IQR: 103-1189, p<0.001) or IL-6-inhibitors (median: 492 BAU/mL, IQR: 161-1007, p<0.001) compared to HCWs (median: 2351 BAU/mL, IQR: 1389-3748). T-cell-specific response scored positive in most of RA patients [24/35, (69%) ] with significantly lower IFN-g levels in patients under biological therapy such as IL-6-inhibitors (median: 33.2 pg/mL, IQR: 6.1-73.9, p<0.001), CTLA-4-inhibitors (median: 10.9 pg/mL, IQR: 3.7-36.7, p<0.001), and TNF-ainhibitors (median: 89.6 pg/mL, IQR: 17.8-224, p=0.002) compared to HCWs (median: 343 pg/mL, IQR: 188-756). A significant correlation between the anti-RBD-antibody titer and spike-IFN-g-specific T-cell response was found in RA patients (rho=0.432, p=0.009). IFN-g T-cell response was mediated by CD4 + and CD8 + T cells. Finally, no significant increase in disease activity was found in RA patients following vaccination.

The COronaVIrus Disease-2019 (COVID-19) pandemic caused by the Severe Acute Respiratory Syndrome CoronaVirus 2 (SARS-CoV-2) has recently emerged as a new human-tohuman transmissible disease with a serious global health impact and still difficult clinical management (1) (2) (3) .

Mass vaccination is the single most effective public health measure for controlling the COVID-19 pandemic, and a global effort to develop and distribute an effective vaccine produced important containment results. Several data are currently available about efficacy of mRNA platform vaccines, namely BNT162b2 and mRNA-1273 vaccines, in inducing strong antibody and cell-mediated immune responses in naïve healthy individuals (4) (5) (6) . The ability to elicit a coordinated induction of both humoral-and cell-mediated arms is fundamental for a more effective fighting of SARS-CoV-2 infection (7, 8) .

Currently available data suggest that patients with autoimmune inflammatory rheumatic diseases have a slightly higher prevalence of SARS-CoV-2 infections, risk of hospitalization, and death from COVID-19 than the general population, and they have been considered a priority target group for vaccine administration (9, 10) . However, considering the immunologic dysregulation and the immunosuppressive treatments frequently adopted in these patients, some concerns have arisen regarding vaccine efficacy and safety.

Recently, some encouraging data on mRNA vaccination in rheumatoid arthritis (RA) patients have emerged from few small and one large prospective observational multicenter study evaluating the immunogenicity and safety of the BNT162b2 mRNA vaccine compared to control subjects without rheumatic diseases (11) (12) (13) . Overall, these studies show that the antibody response to BNT162b2 vaccine is immunogenic in the majority of patients with RA (86-100%), but delayed and reduced compared to controls. Although the results on the impact of the immunosuppressive therapy on vaccine immunogenicity are not homogenous, most of studies suggest that rituximab followed by abatacept, mycophenolate mofetil, corticosteroids (CCS), and methotrexate (MTX) can induce a significant reduction of seropositive rate and antibody levels (14) . These data are crucial to optimize the management of RA patients and to improve vaccine safety and effectiveness, but they need to be confirmed and supplemented by additional real-world studies and by the evaluation of the T-cellspecific response.

This study aimed to assess in RA patients treated with different immunosuppressive therapies the induction of a specific immune response after SARS-CoV-2 vaccination in terms of anti-region-binding-domain (RBD)-antibody-and Tcell-specific responses against spike, and the safety of vaccination in terms of clinical impact on disease activity. A cohort of health care workers (HCWs) was used as a healthy control group.

Participants were enrolled from two parallel prospective studies conducted at the National Institute for Infectious Diseases (INMI) Lazzaro Spallanzani and approved by the INMI Ethical Committee. The approved studies evaluated the immune response to SARS-CoV-2 vaccination in both HCWs enrolled at INMI (approval number 297/2021) and in rheumatologic patients enrolled at Sant'Andrea Hospital in Rome (approval number 318/2021). All HCWs and rheumatologic patients received the BNT162b2-mRNA vaccine. Inclusion criteria for the enrollment of rheumatologic patients were: a diagnosis of RA according to the European League Against Rheumatism/ American College of Rheumatology (EULAR/ACR) 2010 criteria (15) , having completed the two-dose schedule of the mRNA vaccine in the last 2 weeks, being on treatment with a biological drug (except anti-CD20) with or without MTX or other disease modifying anti-rheumatic drugs (DMARD), with only DMARD, with anti-Janus kinase (JAK) or low dosage of CCS (prednisone <7.5 mg/day or methylprednisolone <6 mg/ day). Written, informed consent was required to consecutively enroll patients and controls.

Clinical, demographic data and the use of medication were collected at the time of enrollment (T0) and after 2 weeks from the second dose (T1) ( Table 1) . RA disease activity was evaluated by clinical examination at T0 and T1 through the DAS28crp. At T1, blood samples were collected and local and/or systemic clinical adverse events were registered.

RA patients were stratified according to drug treatments in four groups: TNF-a-inhibitors with or without DMARD, IL-6inhibitors with or without DMARD/CCS, CTLA-4-inhibitors with or without DMARD/CCS, and DMARD with or without CCS. The lymphocyte count of the RA patients was performed within one week from the samples' collection taken for the immune-based assays.

A convenient sample of 167 individuals was included as healthy controls from the cohort of vaccinated HCWs at INMI L. Spallanzani (4, 16) .

Whole-blood (600 µL) was stimulated with a pool of peptides covering the sequence of SARS−CoV−2 spike protein (SARS−CoV−2 PepTivator ® Prot_S1, Prot_S, and Prot_S+, Miltenyi Biotec, Germany) in a 48-well flat-bottom plate (17) . The PepTivator ® Peptide Pools used were constituted by peptides of 15 amino acid length with an 11 amino acid overlap. After 20-24 hours of incubation at 37°C (5% CO 2 ), plasma was harvested and stored at -80°C until use. IFN-g levels were quantified in the plasma samples using an automatic ELISA (ELLA, protein simple). IFN-g values of the stimulated samples were subtracted from the unstimulated-control value. The detection limit of this assay was 0.17 pg/mL.

PBMCs, isolated from HCWs (n=7) and RA patients (n=15), were thawed, counted, assessed for viability, and rested for 2-4 hours at 37°C in RPMI supplemented with 1% L-glutamine, 1% penicillin/ streptomycin (Euroclone S.p.A, Italy), and 10% heat-inactivated FBS. For antigen-specific T-cell stimulation, PBMCs were seeded at a concentration of 2.5 × 10 6 cells/mL in a final volume of 200 µL in a 96-multiwell flat-bottom plate (COSTAR, Sigma Aldrich), and stimulated with spike peptide pool at 1 µg/mL or Staphylococcal Enterotoxin B (SEB) at 200 ng/mL, used as a positive control. We added anti-CD28 and anti-CD49d monoclonal antibodies (BD Biosciences San Jose, USA) to co-stimulate cells at a final concentration of 1 µg/mL each. After 1h of incubation at 37°C (5% CO 2 ), a Golgi plug (BD Biosciences) at 1 µL/mL was added to cell cultures to inhibit cytokine secretion and to allow intracellular molecule detection by flow cytometry. After 16-24 h, cells were stained as described in the following.

Stimulated PBMCs were stained with fluorochrome-conjugated antibodies prepared in Brilliant Stain Buffer (BD Biosciences) (see Supplementary Figure S1 for gating strategy). The Cytofix/ Cytoperm solution kit (BD Biosciences) was used for the intracellular IFN-g staining, according to the manufacturer's instructions (see Supplementary Table S1 for the list of antibodies and reagents used). Dead cells were excluded from the analysis by side/forward scatter gating and then by Fixable Viability stain 700 (BD Biosciences). At least 100,000 lymphocytes from each sample were gated (except for three samples, two from the unstimulated conditions and one from the SEB condition which were gated with 80,000 events). Samples were acquired on a BD Lyric (BD Biosciences) cytometer and data were analyzed by the FlowJo software (version 10, Tree Star). IFN-g-mediated T-cell response was considered positive when: i) the frequency of the SARS-COV-2 peptide-stimulated PBMCs was at least twofold higher compared to the unstimulated control; and ii) at least 10 events were present within the IFN-g gate (18) .

The humoral response to vaccination was assessed by quantifying the anti-Nucleoprotein-IgG and the anti-RBD-IgG (Architect ® i2000sr Abbott Diagnostics, Chicago, IL). Anti-N-IgG were expressed as arbitrary units (AU)/mL and values were considered positive when ≥ 1.4. Anti-RBD-IgG were expressed as binding arbitrary units (BAU)/mL and values were considered positive when ≥ 7.1.

Data were analyzed using GraphPad (GraphPad Prism 8 XML ProjecT). Categorical variables were reported as count and proportion, whereas continuous variables, including IFN-g levels and anti-RBD titers, were reported as median and interquartile range (IQR). Results were evaluated by non-parametric statistical inference tests. The comparisons among groups were evaluated using the Kruskal-Wallis test, whereas the Mann-Whitney U-test with Bonferroni correction was used for pairwise comparisons. The Chi-squared test was used for categorical variables. Correlations of demographic, clinical, and laboratory variables with antibody and S-specific T-cell response, as well as betweenassay correlations, were assessed by non-parametric Spearman's Rank test. Spearman's r ho >0.7 was considered high correlation, 0.7 <r ho >0.5 moderate correlation, and r ho <0.5 low correlation. Twotailed p-values were considered significant if <0.05, except for subgroup analyses by type of rheumatologic-specific treatment, where a correction for multiplicity was applied according to the Bonferroni method, yielding to a significant two-tailed p-value threshold of 0.0125 (a/4).

We prospectively enrolled 202 vaccinated subjects from whom 35 were RA patients and 167 were HCWs. Significant differences were found with respect to age (p<0.0001) and origin (p=0.005), but not for sex between the two groups ( Table 1) .

The RA cohort consisted of 7 patients under treatment with TNF-a-inhibitors with or without DMARD, 8 treated with IL-6-inhibitors with or without DMARD/CCS, 13 under CTLA-4-inhibitors with or without DMARD/CCS, and 7 under only DMARD (5 patients were receiving MTX, 1 salazopyrin, and 1 hydroxychloroquine) with or without CCS. At vaccination, the median treatment duration for TNF-a-inhibitors with or without DMARD was 2.9 years (IQR: 1.3-11), for IL-6-inhibitors with or without DMARD/CCS 6.1 years (IQR: 4.9-7.6), for CTLA-4-inhibitors with or without DMARD/CCS 6 years (IQR: 1.9-10), and for DMARD with or without CCS 2.2 years (IQR: 1.9-4.9).

In RA patients, the ongoing therapeutic regimen was modified during the vaccination period according to the ACR indications (19) . In particular, MTX and JAK-inhibitors were stopped for one week after the first and second dose, whereas abatacept, the CTLA-4 inhibitor, was stopped one week before and after the first dose only.

No significant increase of disease activity was found at T1 compared with baseline values [T0: median 2.9, IQR (2.4-3.5) vs T1: median 3.1, IQR (2.0-3.5), p=0.759]. No severe adverse reactions were observed in vaccinated patients. Mild, transient, systemic, and local side effects, mainly pain at the injection location, mild fever, arthromyalgia, and fatigue, were reported by 18 patients (46%).

Humoral response was evaluated by measuring the anti-RBD antibodies, while the natural infection was excluded by the detection of anti-N-antibodies. Both HCWs and RA patients were naïve for SARS-CoV-2 infection, as confirmed by the undetectable levels of anti-N antibodies (data not shown). A detectable anti-RBD antibody response was observed in all HCWs (100%) and in all RA patients, except for one individual (97.1%). However, the magnitude of the HCWs response was significantly higher than that of RA patients under CTLA-4 and IL-6 inhibitors with or without DMARD/ CCS (p<0.0001 in both groups). Differently, no significant differences were found for the anti-RBD antibody response of patients under TNF-a-inhibitors with or without DMARD (p=0.273) and DMARD with or without CCS (p=0.421) ( Figure 1A) . The response to vaccination can naturally wane with age. Older age may have an impact on the magnitude of the humoral response (19) . Therefore, among the HCWs we selected a group (n=50) who were age-matched [age median: 56, IQR (53-61)] with the RA cohort. We confirmed the results described in Figure 1A and we suggest that, more than the age, the RA related-therapies are likely responsible for the reduced specificantibody response (Supplementary Figure S2A) .

All HCWs showed an IFN-g-S-specific T-cell response, evaluated by the whole blood platform (3, 10) . Contrarily, significant different proportions of responders were found in RA patients under both CTLA-4 and IL-6-inhibitors with or without DMARD/CCS therapy, compared to HCWs (p=0.0018 and p<0.0001, respectively) ( Table 2) . Moreover, the quantitative responses were significantly different among groups (p<0.0001) ( Figure 1B) . In particular, the IFN-g-S-specific levels were significantly lower in RA patients under TNF-a-inhibitors with or without DMARD, IL-6-inhibitors with or without DMARD/ CCS, and CTLA-4-inhibitors with or without DMARD/CCS therapy than those in HCWs (p=0.0020, p<0.0001, p<0.0001, respectively). In contrast, no significant difference was found between the IFN-g-S-specific response of patients treated with DMARD with or without CCS compared to that of HCWs (p=0.016), albeit the IFN-g levels were lower than those of HCWs. These data were confirmed comparing the S-specific T-cell response of RA patients with that of age-matched HCWs (n=50) [age median: 56, IQR (53-61)] (Supplementary Figure S2B ).

We then focused on the correlation between the two arms of the immune response. A significant correlation between anti-RBDantibody titer and SARS-CoV-2-S-specific IFN-g T-cell response was found in HCWs (3) . Similarly, a significant moderate correlation was observed in RA patients (rho=0.432, p=0.009) ( Figure 1C) . Differently, there was no correlation between the lymphocyte number and anti-RBD antibody titer (rho=0.325, p=0.069) or T-specific response (rho=0.151, p=0.409) (data not shown). Further, we analyzed in the RA cohort the impact of age, gender, or years of therapy to identify potential factors affecting the qualitative and quantitative immune responses. None of these variables showed a significant impact on the humoral-or T-cell-specific responses (Supplementary Tables S2, S3) .

To assess which T-cell subset among CD4 + or CD8 + T cells was responsible for the SARS-CoV-2-S-specific response, the IFN-g-Sspecific T-cell frequency was analyzed by flow cytometry after stimulation of the PBMCs with the spike peptide pool. To this aim, we used PBMCs isolated from 7 HCWs and 15 RA patients. Among the RA subjects, we selected those characterized by good specific antibody and T-cell responses ( Figure 2 ). In particular, we selected 5 RA patients under TNF-a-inhibitors with or without DMARD, 3 patients under CTLA-4-inhibitors with or without DMARD/CCS, 3 patients under IL-6-inhibitors with or without DMARD/CCS, and 4 DMARD with or without CCStreated patients. We show that the IFN-g response is mediated by CD4 + T cells following in vitro stimulation with spike peptide pool compared to the unstimulated control, both in HCWs and in RA patients (Figures 2A, B) . The CD4 + T-cell response was scored positive in all HCWs (7/7, 100%) ( Figure 2E ) and in most RA patients (12/15, 80%) ( Figure 2E) . The IFN-g response was mediated also by CD8 + T cells in most HCWs (5/7, 71%) and in a portion of the RA patients tested (3/15, 20%) ( Figures 2C, D) . In the HCWs, the magnitude of the specific response was higher in CD4 + T cells (median: 0.28%, IQR: 0.19-0.42) ( Figure 2E ) compared to CD8 + T cells (median: 0.058%, IQR: 0.00-0.14) ( Figure 2E) . Similarly, in RA patients the CD4 + T cells showed a higher specific response (median: 0.17%, IQR: 0.05-0.24) ( Figure 2E ) compared to the CD8 + T cells (median: 0.00%, IQR: 0.00-0.00) ( Figure 2E ). All HCWs and RA patients responded to SEB, used as a positive control, confirming the absence of an impairment of the cytokine production (Supplementary Figures  S3A, B) . Interestingly, in the RA cohort, the CD8 + T-cell mediated response to SEB was significantly higher compared to that observed in HCWs (p=0.001) (Supplementary Figure S3B ).

Mass vaccination is a crucial public health measure for limiting COVID-19 pandemic especially in fragile populations such as RA patients. Here, we show the results of the immune response to BNT162b2 vaccine in RA patients that were vaccinated based on the ACR indications (20) with an interruption of MTX and JAKinhibitors 1 week after the first and second vaccine dose, or with an interruption of abatacept for 1 week before and after the first dose. In RA patients, BNT162b2 vaccine showed a good safety profile and disease activity remained stable with no patient experiencing a disease relapse. The vaccine induced an antibody-specific response in almost all patients (97%), although the titer was significantly reduced in those under CTLA-4inhibitors (abatacept) or IL-6-inhibitors compared to HCWs. Concomitantly, spike-specific T-cell response was evaluated and scored positive in 69% of RA patients vs. 100% of HCWs with significantly lower levels in those under a biological therapy compared to HCWs, particularly in patients under CTLA-4inhibitors or IL-6-inhibitors. The response to vaccination may decrease with age. However, the present finding was confirmed when comparing the results of a group of age-matched HCWs with the RA cohort suggesting that the lower magnitude of both RBD-antibody and T-cell responses was not due to the older age of patients but likely to the RA-treatment. Based on these results, we confirm that COVID-19 vaccination is immunogenic and safe, also in patients under immunosuppressive therapies, although the specific immune responses were present at a lower magnitude compared to the healthy population.

Recently, it has been shown that individuals with immunemediated inflammatory diseases treated with MTX have up to a 62% rate of specific-immune response to BNT162b2 mRNA vaccine (14) , whereas those under cytokine-inhibitors have levels similar to those of healthy controls (greater than 90%) (11, 13, 14) . The different results reported here on the impact of immunosuppressant drugs on the humoral response may be associated with the therapeutic strategy adopted to optimize vaccine immunogenicity. Indeed, as already seen for seasonal influenza vaccination (21), the 1-week interruption of MTX after the first and second vaccine dose may have reduced the negative impact on antibody production previously shown (11, 14) . This strategy was useful also for those under CTLA-4-inhibitors, as demonstrated by the reassuring proportion of patients mounting an anti-RBD-specific response rate, 92% here vs. 62% of previous reports (11, 14) , although with a significant decreased antibody titer compared to that observed in the HCWs. Furthermore, notably, this brief "window of therapy interruption" did not affect the RA disease activity, as shown by the DAS28crp that remained stable throughout the vaccination period.

On the other hand, the strategy of interrupting abatacept administration limited to the first dose was not satisfactory to provide the induction of the T-cell-specific response, which is known to be impaired by the drug itself (22) , as shown here by the 46% positive responder rate. Based on these results and considering that abatacept blocks the T-cell activation by binding with high-affinity CD80/CD86 molecules thus interfering with the co-stimulation signals delivered through the antigen presenting cells (23) , it may be reasonable to extend its interruption also at the second vaccine dose. This approach may improve the induction of a specific immune response especially at the T-cell level.

Interestingly, IL-6-inhibitors had a higher negative impact on the magnitude of antibody-and T-cell-specific Responses compared to TNF-a-inhibitors. This is likely due to the important effect of IL-6 in controlling the survival, population expansion, and maturation of B cells and plasmablasts acting on the follicular helper T cells, a specialized subset of CD4 + T cells that localize to B cell follicles, where they promote B cell proliferation and immunoglobulin class switching (24, 25) . IL-6 is also important for the T-cell memory response (24, 26) .

Flow cytometry analysis showed that the in vitro T-cell response to SARS-CoV-2 spike peptides is mediated by CD4 + and CD8 + T cells in both HCWs and RA patients. Notably, CD4 + T-cell frequency was higher compared to that observed for the CD8 + T cells. These data agree with the results from the HCWs cohorts (5, (27) (28) (29) (30) (31) and the COVID-19 convalescent subjects (17, 32) . Remarkably, CD8 + T-cell response was lower in the RA cohort compared to that observed in the HCWs. Due to the small sample size of samples included in the flow cytometry analysis, we cannot associate the low frequency of the CD8 + T cell response observed in RA patients to the different therapeutic regimens.

Some limitations of this study need to be considered. First, it was a single center study with a low number of recruited patients that may limit the impact of the study, especially for the comparison of the effects of vaccination among different immunosuppressive therapies. However, the enrolled patients are representative of RA patients under different therapies, and they were well characterized, both clinically and immunologically. Second, the evaluation of the immune responses was performed at a single time point post-vaccination, and the assay used to detect the T-cell response was based on the measurement of a single cytokine (IFN-g) differently from published studies assessing additional T-helper 1 cytokines (4). However, it was shown that the IFN-g-specific T-cell response correlates with RBD-antibody titers (4); therefore this cytokine may be considered as a robust parameter to detect T-cell-specific response induced after vaccination.

Importantly, one of the strengths of this study is the more accurate assessment of the humoral immune response using specific anti-RBD-IgG against the total spike protein compared to the previous published work, where IgG antibody titers against only S1 were evaluated (14) . In addition, we characterized the Tcell response in terms of CD4 + or CD8 + T-cell involvement. The assays used in the present study to detect SARS-CoV-2 specific response are easy and highly reproducible (17, (33) (34) (35) (36) (37) (38) , and therefore are compatible with the routine monitoring of vaccinated individuals (4, 5, 16) . Indeed, the T-cell response was detected by a whole blood assay, whose platform is similar to current tests measuring T-cell-specific responses against M. tuberculosis in both immune-competent and immunesuppressed subjects (39) (40) (41) (42) .

To the best of our knowledge, this is the first study evaluating both humoral and cellular immune responses to BNT162b2 vaccine in RA patients, who underwent a temporary suspension of immunosuppressive treatment during vaccine administration. For the optimal management of RA patients, clinicians need to consider both the risk of disease relapse and that of a decreased vaccine immunogenicity. These findings suggest that holding treatment with MTX and abatacept at the first and second vaccine dose can be considered a useful practice in clinically stable patients. To draw definite conclusions, these results need to be confirmed in a larger population adopting a similar therapeutic strategy suspension, and future studies are needed to further evaluate the longevity of humoral and T-cell responses following vaccination.

The raw data generated and/or analyzed within the present study are available in our institutional repository (rawdata.inmi.it), subject to registration. The data can be found by selecting the article of interest from a list of articles ordered by year of publication. No charge for granting access to data is required. In the event of a malfunction of the application, the request can be sent directly by e-mail to the Library (biblioteca@inmi.it).

The studies involving human participants were reviewed and approved by the Ethical Committee of the National Institute of Infectious Diseases "Lazzaro Spallanzani" IRCCS (approval numbers 297/2021 and 318/2021). The patients/participants provided their written informed consent to participate in this study. The funders were not involved in the study design, collection, analysis, and interpretation of data, the writing of this article, or the decision to submit it for publication.

Immune Therapy, or Antiviral Therapy, or Both for COVID-19: A Systematic Review

Baricitinib Therapy in Covid-19 Pneumonia -An Unmet Need Fulfilled

Cytokine Release Syndrome in COVID-19 Patients, A New Scenario for an Old Concern: The Fragile Balance Between Infections and Autoimmunity

Coordinate Induction of Humoral and Spike Specific T-Cell Response in a Cohort of Italian Health Care Workers Receiving BNT162b2 mRNA

T-Cell and Antibody Responses to First BNT162b2 Vaccine Dose in Previously SARS-CoV-2-Infected and Infection-Naive UK Healthcare Workers: A Multicentre, Prospective

Efficacy and Safety of the mRNA-1273 SARS-CoV-2 Vaccine

Antigen-Specific Adaptive Immunity to SARS-CoV-2 in Acute COVID-19 and Associations With Age and Disease Severity

Immunological Memory to SARS-CoV-2 Assessed for Up to 8 Months After Infection

EULAR Provisional Recommendations for the Management of Rheumatic and Musculoskeletal Diseases in the Context of SARS-CoV-2

Direct and Indirect Impact of COVID-19 for Patients With Immune-Mediated Inflammatory Diseases: A Retrospective Cohort Study

Immunogenicity and Safety of the BNT162b2 mRNA COVID-19 Vaccine in Adult Patients With Autoimmune Inflammatory Rheumatic Diseases and in the General Population: A Multicentre Study

Immunogenicity and Safety of Anti-SARS-CoV-2 mRNA Vaccines in Patients With Chronic Inflammatory Conditions and Immunosuppressive Therapy in a Monocentric Cohort

SARS-CoV-2 Vaccination Responses in Untreated, Conventionally Treated and Anticytokine-Treated Patients With Immune-Mediated Inflammatory Diseases

Methotrexate Hampers Immunogenicity to BNT162b2 mRNA COVID-19

Vaccine in Immune-Mediated Inflammatory Disease. medRxiv

Rheumatoid Arthritis Classification Criteria: An American College of Rheumatology/European League Against Rheumatism Collaborative Initiative

Impact of Prior Influenza and Pneumoccocal Vaccines on Humoral and Cellular Response to SARS-CoV-2 BNT162b2 Vaccination. Vaccines (Basel) (2021) 9

Spike is the Most Recognized Antigen in the Whole-Blood Platform in Both Acute and Convalescent COVID-19 Patients

How Many Events is Enough? Are You Positive?

Delayed Antibody and T-Cell Response to BNT162b2 Vaccination in the Elderly

American College of Rheumatology Guidance for COVID-19 Vaccination in Patients With Rheumatic and Musculoskeletal Diseases: Version 2

Impact of Temporary Methotrexate Discontinuation for 2 Weeks on Immunogenicity of Seasonal Influenza Vaccination in Patients With Rheumatoid Arthritis: A Randomised Clinical Trial

Cytotoxic T Lymphocyte Antigen 4-Immunoglobulin)

Improves B Cell Function and Regulatory T Cell Inhibitory Capacity in Rheumatoid Arthritis Patients non-Responding to Anti-Tumour Necrosis Factor-a Agents

IL-6 as a Keystone Cytokine in Health and Disease

The Origins, Function, and Regulation of T Follicular Helper Cells

Interleukin-6 is Crucial for Recall of Influenza-Specific Memory CD4 T Cells

mRNA Vaccine-Induced T Cells Respond Identically to SARS-CoV-2 Variants of Concern But Differ in Longevity and Homing Properties Depending on Prior Infection Status

Immune Responses Against SARS-CoV-2 Variants After Heterologous and Homologous ChAdOx1 Ncov-19/BNT162b2 Vaccination

SARS-CoV-2 Spike Glycoprotein-Reactive T Cells can be Readily Expanded From COVID-19 Vaccinated Donors

The Potential Clinical Utility of Measuring Severe Acute Respiratory Syndrome Coronavirus 2-Specific T-Cell Responses

SARS-CoV-2 Specific T-Cell Immunity in COVID-19 Convalescent Patients and Unexposed Controls Measured by Ex Vivo ELISpot Assay

Interferon-Gamma Release Assay for Accurate Detection of SARS-CoV-2 T Cell Response

A Whole Blood Test to Measure SARS-CoV-2-Specific Response

In-Vitro Evaluation of the Immunomodulatory Effects of Baricitinib: Implication for COVID-19 Therapy

Coinfection of Tuberculosis and COVID-19 Limits the Ability to In Vitro Respond to SARS-CoV-2

Exploratory Analysis to Identify the Best Antigen and the Best Immune Biomarkers to Study SARS-CoV-2 Infection

Optimization and Interpretation of Serial QuantiFERON Testing to Measure Acquisition of Mycobacterium Tuberculosis Infection

Latent Tuberculosis Infection Screening in Persons Newly-Diagnosed With HIV Infection in Italy: A Multicentre Study Promoted by the Italian Society of Infectious and Tropical Diseases

Characterization of QuantiFERON-TB-Plus Results in Latent Tuberculosis Infected Patients With or Without Immune-Mediated Inflammatory Diseases

Effect of HIV-Infection on QuantiFERON-Plus Accuracy in Patients With Active Tuberculosis and Latent Infection

Immunosuppressive Therapies Differently Modulate Humoral-and T-Cell-Specific Responses to COVID-19 mRNA Vaccine in Rheumatoid Arthritis Patients

This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited

COVID-19-Vaccine Response in Rheumatoid Arthritis

The authors gratefully acknowledge the Collaborators Members of the National Institute for Infectious Diseases (INMI) COVID-

The Supplementary Material for this article can be found online at: https://www.frontiersin.org/articles/10.3389/fimmu.2021. 740249/full#supplementary-material