key: cord-0949222-o89qzvll authors: Strengert, Monika; Becker, Matthias; Ramos, Gema Morillas; Dulovic, Alex; Gruber, Jens; Juengling, Jennifer; Lürken, Karsten; Beigel, Andrea; Wrenger, Eike; Lonnemann, Gerhard; Cossmann, Anne; Stankov, Metodi V.; Dopfer-Jablonka, Alexandra; Kaiser, Philipp D.; Traenkle, Bjoern; Rothbauer, Ulrich; Krause, Gérard; Schneiderhan-Marra, Nicole; Behrens, Georg M.N. title: Cellular and humoral immunogenicity of a SARS-CoV-2 mRNA vaccine in patients on haemodialysis date: 2021-08-12 journal: EBioMedicine DOI: 10.1016/j.ebiom.2021.103524 sha: e0b286242957d7e9bbbffd6be4b4b23aad972fe5 doc_id: 949222 cord_uid: o89qzvll BACKGROUND: Patients with chronic renal insufficiency on maintenance haemodialysis face an increased risk of COVID-19 induced mortality and impaired vaccine responses. To date, only a few studies have addressed SARS-CoV-2 vaccine elicited immunity in this immunocompromised population. METHODS: We assessed immunogenicity of the mRNA vaccine BNT162b2 in at-risk dialysis patients and characterised systemic cellular and humoral immune responses in serum and saliva using interferon γ release assay and multiplex-based cytokine and immunoglobulin measurements. We further compared binding capacity and neutralization efficacy of vaccination-induced immunoglobulins against emerging SARS-CoV-2 variants Alpha, Beta, Epsilon and Cluster 5 by ACE2-RBD competition assay. FINDINGS: Patients on maintenance haemodialysis exhibit detectable but variable cellular and humoral immune responses against SARS-CoV-2 and variants of concern after a two-dose regimen of BNT162b2. Although vaccination-induced immunoglobulins were detectable in saliva and plasma, both anti-SARS-CoV-2 IgG and neutralization efficacy was reduced compared to a vaccinated non-dialysed control population. Similarly, T-cell mediated interferon γ release after stimulation with SARS-CoV-2 spike peptides was significantly diminished. INTERPRETATION: Quantifiable humoral and cellular immune responses after BNT162b2 vaccination in individuals on maintenance haemodialysis are encouraging, but urge for longitudinal follow-up to assess longevity of immunity. Diminished virus neutralization and interferon γ responses in the face of emerging variants of concern may favour this at-risk population for re-vaccination using modified vaccines at the earliest opportunity. FUNDING: Initiative and Networking Fund of the Helmholtz Association of German Research Centres, EU Horizon 2020 research and innovation program, State Ministry of Baden-Württemberg for Economic Affairs, Labour and Tourism. Since its emergence in late 2019, SARS-CoV-2 has become a global pandemic with more than 166 million confirmed cases and 3¢46 million deaths (as of 24 .05.21) [1] . Vulnerable populations such as the elderly, immunocompromised or those suffering from chronic conditions or requiring continual medical intervention such as dialysis are at-risk of severe COVID-19 disease and associated death [2] . Although a series of vaccines have been developed, tested and approved at unprecedented speed, only one vaccine study for NVX CoV2373 has enrolled patients with chronic diseases such as chronic kidney disease to assess efficacy and safety of SARS-CoV-2 vaccination within this vulnerable population [3] . Patients on maintenance haemodialysis are a particularly high-risk group, as renal disease has been identified as a key risk factor for severe COVID-19 [4] [5] [6] [7] , while at the same time their regular need for therapy does not allow them to self-isolate and reduce contacts to avoid infection. A recent study also suggested that seroreversion following natural SARS-CoV-2 infection is faster in dialysis patients compared to the general population further increasing the risk of re-infection [8] . Other studies have also demonstrated an impaired humoral immune response in dialysis patients, as seen by the attenuation of antibody titres following vaccination with SARS-CoV-2 vaccines [9] [10] [11] [12] [13] [14] [15] . Both, COVID-19 and BNT162b2-induced effective immunity appear to result from functional T-follicular helper (TfH) cell responses and Th1 cytokines [16, 17] . In contrast, end-stage kidney failure is associated with proinflammatory markers (including IFNg, TNFa, IL-8, CCL-2, and others), exhausted T-cell phenotype, and perturbed TfH-cells [18] . Additional data on the efficiency of SARS-CoV-2 vaccination is urgently needed not only for risk mitigation but also to assess whether additional protective measures during therapy must be put in place as seen by the impaired infection and vaccination-induced responses for influenza A and hepatitis B [19] [20] [21] . While antibody titres have already been characterised within vaccinated dialysis patients, little is known about the ensuing cellular immune response [22] or about the neutralization potential of vaccine-induced antibodies [23] , particularly in light of the increasingly appearing SARS-CoV-2 variants of concern (VoC) which threaten the success of vaccination programs [24] . To assess efficacy of SARS-CoV-2 vaccination in dialysis patients, we characterised cellular and humoral immune responses in serum and saliva of dialysed and non-dialysed individuals after vaccination with the mRNA vaccine BNT162b2. Considering the increasing presence of mutated SARS-CoV-2 strains, we further compared binding capacity and neutralization efficacy of vaccination-induced immunoglobulins against emerging variants of concern such as B.1.1.7 (Alpha), B.1.351 (Beta), B.1.429 (Epsilon) and Cluster 5 (Mink). Following written informed consent, heparinized blood samples from haemodialysis patients (n=81) were taken before start of dialysis using a vascular access which was either an arterio-venous fistula or a central venous catheter or by venipuncture from health care workers (n=34), who served as non-dialysed control population. Participants had to be over the age of 18 and able to give written informed consent. All study participants were either patients or worked at the dialysis centre Eickenhof and received the vaccine on the same occasion. 10 of the 81 dialysis patients were on immunosuppressive medication such as prednisolone, tacrolimus, mycophenolatmofetil, hydrocortisone, or a combination. Four of those patients had received a kidney transplant, and one of them additionally a liver transplant. Other reasons for immunosuppressive therapy included polymyositis, polyarthritis, vasculitis and chronic obstructive pulmonary disease. Further details about the study population can be found in Table 1, Table S2 and S3. One haemodialysis patient had previously been tested positive for SARS-CoV-2 by routine PCR screening. As subsequent antibody testing was negative for SARS-CoV-2 IgG, this patient received BNT162b2 and was not excluded from the study. All participants received the standard two-dose regimen of BNT162b2 21 days apart, followed by blood collection for analysis 21 days after the second dose. Plasma was obtained from lithium heparin blood (S-Monovette Plasma, Sarstedt, Germany). Whole blood samples were used immediately for interferon g release assay (IGRA). For saliva collection, all individuals spat directly into a collection tube. To Evidence before this study Patients on dialysis tend to have a reduced immune response to both infection and vaccination. We searched PubMed and medRxiv for studies including search terms such as "COVID-19", "vaccine", and "dialysis" but no peer-reviewed studies to date simultaneously assessed both SARS-CoV-2 specific B-and T-cell responses, mucosal immunoglobulins, and considered the impact of SARS-CoV-2 variants of concern in this at-risk population. We provide a comprehensive functional characterisation of both T-and B-cell responses following a two-dose regimen of BNT162b2 in at-risk patients on maintenance haemodialysis. More importantly, to the best of our knowledge, we assess for the first time binding and neutralization capacity of vaccination-induced circulation and mucosal antibodies towards emerging SARS-CoV-2 variants of concern in an immunocompromised population. Patients on maintenance haemodialysis develop a substantial cellular and humoral immune response following the BNT162b2 vaccine. These findings should encourage patients on maintenance haemodialysis to receive the vaccine. However, we suggest continuing additional protection measures against variants of concern in this at-risk population until longevity of the vaccine response is fully evaluated. inactivate replication-competent SARS-CoV-2 virus particles potentially present in saliva samples, Tri(n-butyl) phosphate (TnBP) and Triton X-100 were added to final concentrations of 0¢3% and 1%, respectively [25] . Both plasma and saliva samples were frozen and stored at À80°C until further use. Ethical approval of the study was obtained from the relevant authority -the Internal Review Board of Hannover Medical School (MHH, approval number 8973_BO-K_2020, amendment Dec. 2020). Written informed consent was obtained from all participants prior to starting the study. Coupling of antigens to spectrally distinct MagPlex beads (Cat #MC10XXX-01, Luminex Corporation, USA) was done by EDC/s-NHS coupling for all standard MULTICOV-AB antigens [26] . Receptor-binding domains (RBD)s from VoC were coupled using Anteo coupling (Cat #A-LMPAKMM-10, Anteo Tech Reagents, Australia) following the manufacturer's instructions [27] . Antibody titres and binding was analysed using MULTICOV-AB, a multiplex immunoassay which simultaneously analyses 20 antigens, as previously described [26] . The full list of antigens included in this study can be found in Table S1 . Plasma samples were diluted 1:400, while saliva samples were diluted 1:12 [27] . Briefly, antigens were immobilised on spectrally distinct populations of MagPlex beads (as above) and combined into a single bead mix. Samples were combined with the bead mix, incubated for 2 h at 21°C and then washed using a microplate washer to remove unbound antibodies. Bound antibodies were detected following a 45 min incubation at 21°C with R-phycoerythrin labeled goat-anti-human IgG (Jackson ImmunoResearch Labs, United Kingdom, Cat #109-116-098, Lot #148837, RRID: AB_2337678, used at 3 mg/mL) or IgA (Jackson ImmunoResearch Labs, Cat #109-115-011, Lot #143454, RRID: AB_2337674, used at 5 mg/mL) as secondary antibodies. Following another washing step, beads were re-suspended and then measured using a FLEXMAP 3D instrument (Luminex Corporation, Texas, USA) using the following settings: Timeout 80 sec, Gate: 7500-15000, Reporter Gain: Standard PMT, 40 events. Each sample was measured once. Three quality control (QC) samples were included on each plate to monitor MULTI-COV-AB assay performance. Raw median fluorescence intensity (MFI) values or normalised values (MFI/MFI of QC samples [27] ) are reported. To determine neutralization, an ACE2-RBD competition assay was carried out as previously described [27] . Briefly, biotinylated ACE2 was added to the assay buffer to a final concentration of 500 ng/mL for all samples. Samples were then mixed with MULTICOV-AB bead mix (see above) and incubated for 2 h at 21°C, 750 rpm. After washing, ACE2 was detected using Streptavidin-PE (2 mg/mL, Cat #SAPE-001, Moss, Maryland, US) by incubating the sample for 45 min at 750 rpm. After an additional wash step and resuspension, samples were measured on a FLEXMAP 3D instrument (same settings as MUL-TICOV-AB). As control, 500 ng/mL ACE2 was used. For analysis, MFI values were normalised against the control wells. All samples were measured once. To further validate plasma IgG levels measured by MULTICOV-AB, samples were further analysed using the Anti-SARS-CoV-2-Quanti-Vac-ELISA IgG (Cat #EI 2606-9601-10G, Euroimmun, Germany) according to the manufacturer's instructions. Plasma samples were diluted 1:400 to achieve assay linearity. SARS-CoV-2-specific T-cell responses were determined by measuring IFNg production upon SARS-CoV-2 antigen stimulation using the SARS-CoV-2 Interferon Gamma Release Assay (Cat #ET-2606-3003, Euroimmun, Germany). Briefly, 0¢5 mL of full blood was stimulated with peptides of the SARS-CoV-2 S1 domain of the Spike protein for a period of 20-24 h. Negative and positive controls were carried out according to the manufacturer's instruction. Following stimulation, supernatants were isolated through centrifugation and IFNg measured using ELISA (Cat #EQ-6841-9601, Euroimmun, Germany). The remaining supernatant was stored at -80°C. Background signals from negative controls were subtracted and final results calculated in mIU/mL using standard curves. IFNg concentrations >200 mIU/mL were considered as reactive. The upper limit of reactivity was 2000 mIU/mL. Supernatants of SARS-CoV-2 antigen stimulated blood cells were prepared and isolated as explained for the detection of IFNg by SARS-CoV-2 Interferon Gamma Release Assay and analysed by LEGENDplex TM using the Human Essential Immune Response Panel (Cat #740930, Bio Legend, California, US) for L-4, IL-2, CXCL-10 (IP-10), IL-1b, TNFa, CCL-2 (MCP-1), IL-17A, IL-6, IL-10, IFNg, IL-12p70, CXCL-8 (IL-8), TGFb1) according to manufacturer's instructions. Analysis was performed using an LSR II flow cytometer (Becton Dickinson, Germany) and data analysed using the LEGENDplex TM Data Analysis Software Suite. RStudio (Version 1.2.5001), with R (version 3.6.1) was used for data analysis and figure generation. Additionally, the R add-on package "beeswarm" was utilised to visualise data as stripcharts with overlaying boxplots and to create non-overlaying data points. A second R add-on package "RcolorBrewer" was used to generate specific colours for plots. The type of statistical analysis performed (when appropriate) is listed in the figure legends. Figures were exported from Rstudio and then edited using Inkscape (Inkscape 0.92.4). Spearman's rho coefficient was calculated in order to determine correlation between IGRA results and antibody responses or neutralization using the "cor" function from R's "stats" library. Mann-Whitney-U test was used to determine difference between signal distributions between dialysed and non-dialysed groups using the "wilcox.test" function from R's "stats" library. To assess differences in the study population, Pearson's Chi-squared test with Yates' continuity correction was used for categorical characteristics using the "chisq.test" function from R's "stats" library and Mann-Whitney-U test as above was used for difference in age. Pre-processing of data such as matching sample metadata and collecting results from multiple assay platforms was performed in Excel 2016. This work was financially supported by the Initiative and Networking Fund of the Helmholtz Association of German Research Centres (grant number SO-96), the EU Horizon 2020 research and innovation program (grant agreement number 101003480 -COR-ESMA) and the State Ministry of Baden-W€ urttemberg for Economic Affairs, Labour and Tourism (grant numbers FKZ 3-4332.62-NMI-67 and FKZ 3-4332.62-NMI-68). The funders had no role in study design, data collection, data analysis, interpretation, writing or submission of the manuscript. All authors had complete access to the data and hold responsibility for the decision to submit for publication. To characterise the vaccination response in patients on maintenance haemodialysis, we measured immunoglobulin levels 21 days after the second dose of Pfizer BNT162b2 using MULTICOV-AB, a multiplex immunoassay containing antigens from Spike and Nucleocapsid proteins of both SARS-CoV-2 and the endemic human coronaviruses (hCoVs) [26] . As a control group, 34 samples from healthcare workers vaccinated at the same time points as the 81 patients on haemodialysis were used. (Detailed information on the study population can be found in Table 1, Table S2 and S3). As indicated by the lack of a significant anti-Nucleocapsid (N) IgG or IgA response at the time of blood draw 21 days after the second vaccination, none of the study participants had been previously infected or seroconverted after a SARS-CoV-2 infection (data not shown). IgG responses towards the original B.1 isolate in vaccinated dialysis patients were significantly reduced (p<0¢0001, Mann-Whitney-U test) and more variable (Fig. 1a) than in the control group, which reached the upper limit of detection of the assay, as seen previously [27] . Interestingly, plasma IgA responses in the dialysis group were comparable to the control group (Fig. 1b, p=0¢38 , Mann-Whitney-U test). While all participants in the control group seroconverted, within our dialysis population, four from 81 vaccinated individuals (4¢92%) were classified as serologic non-responders with antibody titres below the cut-off. As an additional control, S1 IgG titres were measured using a commercial assay (Fig. S2) , which identified the same pattern of a significantly diminished antibody response in dialysed patients (272¢3 RU/mL) compared to non-dialysed individuals (456¢8 RU/mL, p<0¢0001, Mann-Whitney-U test). Due to the small sample size, we were unable to confidently identify factors associated with reduced humoral immunity by analysis of variance. Dialysis patients receiving immunosuppressive therapy tended to have lower anti-spike IgG levels (median 65¢68 RU/mL, IQR 285¢14) compared to the remaining dialysis patients (median 112.3 RU/mL, IQR 323.6, p=0¢09, Mann-Whitney-U test), which is consistent with a recent report [28] . As SARS-CoV-2 is a mucosal-targeted virus, we also collected saliva from our vaccination cohort and assessed IgG and IgA levels using MULTICOV-AB. When examining antibody titres found in saliva, dialysed individuals had significantly lower IgG titres (p=0¢0007), but similar IgA titres (p=0¢70) to the control group ( Fig. 1c and Neutralization capacity is displayed as ratio where 1 indicates maximum neutralization and 0 no neutralization (e). Saliva (c, d) was collected from 33 controls (red circles), 65 individuals on maintenance haemodialysis (blue circles) and from 9 individuals on maintenance haemodialysis and immunosuppressive medication (yellow circles). Boxes represent the median, 25th and 75th percentiles, whiskers show the largest and smallest non-outlier values. Outliers were determined by 1¢5 times IQR. Statistical significance was calculated by Mann-Whitney-U (two-sided). Significance was defined as *<0¢01, **<0¢001, ***<0¢0001 or n.s.>0¢01. binding towards B.1.1.7 in both dialysed and non-dialysed individuals was comparable to B.1 (original isolate), while binding was clearly reduced for B.1.351 (Fig. 1a) . Antibody binding for Cluster 5 and B.1.429 was similar to the B.1 isolate for both groups (Fig. S1 ). As part of the MULTICOV-AB antigen panel, we also analysed the humoral response towards endemic CoV S1 and N protein, but found no general significant differences between control group and dialysis patients (Fig. S3 ). To assess neutralizing potency of plasma towards both the original B.1 isolate and VoC RBDs, we used a previously described ACE2-RBD competition assay [27] . Neutralization across both wild-type and all VoCs measured was significantly reduced in dialysed compared to non-dialysed individuals (all p<0¢0001, Mann-Whitney-U test) (Fig. 1e, Fig. S4 ). As expected, there were differences between the VoCs themselves, with B.1.351 having the lowest neutralization for both control and dialysed individuals. However, responses were comparably low for all VoCs tested for patients on maintenance haemodialysis and additional immunosuppressive medication in the dialysis group further reduced neutralizing potency with the majority of samples located in the 25th quartile (Fig. 1e) . As clinical studies have suggested that both cellular and humoral response can confer protection from a SARS-CoV-2 infection [29] , we also assessed vaccination-induced T-cell responses by IFNg release assay and characterised cytokine and chemokine responses after stimulation with a Spike S1-derived peptide pool by multiplex Whole blood from vaccinated controls (red circles, n=34), individuals on maintenance haemodialysis (blue circles, n=71) and haemodialysed individuals on immunosuppressive medication (yellow circles, n=10) 21 days post second vaccination was ex vivo stimulated using a SARS-CoV-2 Spike S1-specific peptide pool. Supernatant fractions were analysed by interferon g release assay (IGRA, a) or bead-based multiplex-cytokine assay for CCL-2 (b), IL-8 (c), TNFa (d), IL-2 (e) and IL-1b (f). Data is shown in mIU/mL for IGRA or pg/mL for the multiplex-cytokine assay. T-cells were classified as reactive if IFNg was >200 mIU/mL. IGRA (a) was carried out with samples from all study participants. Bead based-cytokine measurements (b-f) were performed with samples from 29 control, 42 haemodialysed and 8 haemodialysed individuals on immunosuppressive medication. Samples that were classified as above upper or below the lower limit of detection of the cytokine assay or the IGRA are shown at the respective limit. Boxes represent the median, 25th and 75th percentiles, whiskers show the largest and smallest non-outlier values. Outliers were determined by 1¢5 times IQR. Statistical significance was calculated by Mann-Whitney-U (two-sided). Significance was defined as *<0¢01, **<0¢001, ***<0¢0001 or n.s.>0¢01. cytokine measurements. Consistent with reduced anti-Spike S1 IgG and anti-RBD IgG levels (Fig. 1a, Fig. S2 ), IGRA showed significantly lower levels of IFNg released in the supernatants of stimulated T-cells from vaccinated patients on maintenance haemodialysis (p<0¢0001, Fig. 2a ). In addition, all but one individual within the control group (97¢1%) was classified as reactive by IGRA whereas only 71¢6 % were within the haemodialysed group. Of the 12 analysed cytokines beyond IFNg, only IL-8 and CCL-2 (both p<0¢0001, Mann-Whitney-U test) were significantly different between the two immunised groups, whereas no other Th1 type cytokines such as TNFa or IL-2 accompanied the IFNg response ( Fig. 2b-f, Fig. S5 ). At this moment, there are no defined correlates of protection against a SARS-CoV-2 infection and the relative importance of cellular versus humoral response is equally undefined [30, 31] . To shed light on this, we correlated B-and T-cell responses within our vaccination cohort. Comparable to other studies examining vaccination responses of BNT162b2 in a similar setting [32] , we observed a moderate correlation between T-cell responses (measured by IGRA) and B-cell responses (determined by RBD B.1-specific IgG levels (Spearman's rho=0¢56, Fig. 3a ) or RBD B.1 IgG-neutralizing potency (Spearman's rho=0¢56, Fig. 3b) ). In addition, we observed a skew towards increased B-cell reactivity in both control group and individuals on haemodialysis. To control the ongoing COVID-19 pandemic, efficient vaccination to create herd immunity without the infection-induced mortality will be key. We initiated this study to further increase information, including neutralization and response to VoCs, on vaccinationinduced immune responses in at-risk immunocompromised populations such as renal dialysis patients. Similar to other groups, we found robust antibody responses following vaccination within dialysed patients [9, 13] , confirming that our results are comparable to other studies. Overall, 95% of our dialysis patients showed a humoral immune response to vaccination, higher than what other studies with similar time points had found [10] [11] [12] 14, 32] . We can only speculate about potential reasons for those discrepancies such as differences in renal replacement therapies, composition of the patient cohort or co-morbidities. It should be noted that titres were significantly reduced in dialysis patients compared to control individuals, which could result in reduced vaccine efficacy within this group. We also observed differences in humoral IgG and cellular T-cell response in our dialysis group, with four (4¢92%) non-humoral responders and 23 (28¢4%) non-T-cell responders, respectively. Overall, it is apparent from our data that in both groups vaccination response was skewed towards secretory immunity. This is in line with exploratory studies using BNT161b1 and other mRNA vaccines, which induce a B-cell response peak around two weeks after the boosting dose to then decline before reaching a memory plateau phase [33, 34] . Future studies will be needed to determine the longevity and relative contribution of both T-and B-cell responses towards vaccination-induced protection. We found no significant differences in vaccinationinduced IgA levels in both saliva and plasma between our study groups. Although several studies reported lower protective IgG titres over time following hepatitis B, influenza A or SARS-CoV-2 vaccinations, IgA levels were not analysed to determine if IgA vaccination responses are in general less affected in dialysis patients [9] [10] [11] [12] [13] [14] [19] [20] [21] . Interestingly, a monoclonal IgA antibody capable of recognizing both the SARS-CoV-1 and SARS-CoV-2 spike proteins and blocking ACE2 receptor interaction combined with an increased neutralization ability over its IgG equivalent has been described [35] . . Some studies even report a higher neutralizing capacity of purified serum IgA monomers from early convalescent sera compared to IgG and increased saliva IgA titres and neutralization versus IgG in recovered hospitalised COVID-19 patients [36] . We identified a clearly reduced neutralizing capacity towards all VoC RBDs tested in our dialysed individuals compared to controls. Taking into account that SARS-CoV-2 infections were increased in vaccinated dialysis patients compared to vaccinated control individuals [11] , further monitoring is urgently needed to determine if vaccine-induced protection prevents infection with increasingly circulating and diverse SARS-CoV-2 mutant strains, or if additional protection measures still need to be put in place throughout therapy session despite a completed vaccination scheme. Individuals with kidney failure are at increased risk of infections and malignancies, with the uremic milieu potentially triggering a chronic inflammatory state, which promotes T-cell exhaustion and suppression of IFNg production [37, 38] . Indeed, patients with endstage kidney disease (ESKD) are reported to have elevated serum levels of cytokines such as IFNg, TNFa, IL-8, and CCL-2 compared to healthy controls. After mitogen stimulation, both CD4 + and CD8 + T- cells in ESKD group demonstrated a pro-inflammatory phenotype, more exhausted and anergic CD4 + and CD8 + T-cells and a reduced frequency of follicular helper T-cells, which are important for humoral immunity [18] . In light of these immunological changes, our results about diminished SARS-CoV-2 specific T-cell responses and increased proinflammatory cytokine release may account in part for impaired vaccine-induced IgG responses in these patients. Specifically, CCL-2 and IL-8, which both were increased following restimulation with SARS-CoV-2 peptides in dialysis patients, could reflect a more pronounced innate immune response released by monocytes and acting on neutrophils and endothelial cells. We speculate these responses to be secondary to mechanisms triggered by spike-specific T-cells and their cytokines. Which mechanisms critically trigger and facilitate such cytokine patterns in dialysis patients and whether constitutively disturbed cytokine responses in dialysis patients are contributing to hamper humoral or cellular immunity after BNT161b2 vaccination remains to be studied with more careful approaches. Our study has several limitations. While we have a reasonable sample size (81 dialysis patients), which is similar or even larger compared to several other studies [12, 13, 32] , our control group is not age-and gender-matched. Since others have described that both factors have independent influence on the immunogenicity of COVID-19 vaccines [39À42], our observed differences are likely to be influenced by age and sex to some extent. In addition, we evaluated only one of the currently approved SARS-CoV-2 vaccines with samples from a single dialysis centre and did not perform in-depth immune phenotyping or assessment of SARS-CoV-2 responsive T-cell frequencies. Thus, we cannot extrapolate that other COVID-19 vaccines or vaccine schedules will lead to reduced immune responses in dialysis patients as described here. We also lack paired saliva and plasma samples pre and post first dose to characterise B-and T-cell response kinetics or assess potential cross-reactivity of endemic CoV antibodies in immunocompromised individuals across the dosing scheme. However, all of our samples were collected at the same time with an identical dosing regimen which allows us to make a direct comparison between our two groups of interest (dialysed versus non-dialysed). Additionally, the lack of previously infected samples within our study groups limits us to only study vaccine-induced responses. Several groups independently report high antibody titres and neutralization activity after the first dose of Pfizer or Moderna RNA vaccine in individuals who already had SARS-CoV-2 infections [43] . This effect is likely to be repeated in dialysis patients with a single vaccination post COVID-19. Taken together, we provide robust evidence that a completed two-dose regimen of BNT162b2 elicits both antibody and T-cell responses in patients on maintenance haemodialysis towards the SARS-CoV-2 B.1 isolate. Future studies are needed to assess the lifespan and long-term kinetics of the vaccination response. As neutralization is reduced in dialysed patients towards all VoCs examined, our data also highlights the need to monitor if infection with SARS-CoV-2 VoC occur more frequently in this vulnerable population compared to vaccinated healthy individuals. NSM was a speaker at Luminex user meetings in the past. The Natural and Medical Sciences Institute at the University of T€ ubingen is involved in applied research projects as a fee for services with the Luminex Corporation. The other authors declare no competing interest. COVID-19) Dashboard, Accessed 24th Factors associated with COVID-19-related death using OpenSAFELY COVID-19 vaccines and kidney disease COVID-19 and survival in maintenance dialysis Chronic kidney disease is a key risk factor for severe COVID-19: a call to action by the ERA-EDTA COVID-19 among US dialysis patients: risk factors and outcomes from a national dialysis provider COVID-19 antibodies and outcomes among outpatient maintenance hemodialysis patients. Kid-ney360 A longitudinal, 3-Month serologic assessment of SARS-CoV-2 infections in a belgian hemodialysis facility Antibody response to COVID-19 vaccination in patients receiving dialysis Immunogenicity of SARS-CoV-2 vaccine in dialysis Experience with SARS-CoV-2 BNT162b2 mRNA vaccine in dialysis patients Haemodialysis patients show a highly diminished antibody response after COVID-19 mRNA vaccination compared to healthy controls. Nephrology, dialysis, transplantation: official publication of the European Dialysis and Transplant Association Humoral response to the Pfizer BNT162b2 vaccine in patients undergoing maintenance hemodialysis Antibody response to mRNA SARS-CoV-2 vaccine among dialysis patients -a prospectivecohort study High immunogenicity of a messenger RNA based vaccine against SARS-CoV-2 in chronic dialysis patients Immunological memory to SARS-CoV-2 assessed for up to 8 months after infection SARS-CoV-2 mRNA vaccines foster potent antigen-specific germinal center responses associated with neutralizing antibody generation Kidney failure associates with T cell exhaustion and imbalanced follicular helper T cells Efficacy of influenza A H1N1/2009 vaccine in hemodialysis and kidney transplant patients Immunogenicity of a standard trivalent influenza vaccine in patients on longterm hemodialysis: an open-label trial Hepatitis B virus vaccine immune response and mortality in dialysis patients: a meta-analysis Antibody and T cell response to SARS-CoV-2 messenger RNA BNT162b2 vaccine in kidney transplant recipients and hemodialysis patients Early humoral responses of hemodialysis patients after COVID-19 vaccination with BNT162b2 Immunity to SARS-CoV-2 variants of concern SARS-coronavirus (SARS-CoV) and the safety of a solvent/detergent (S/D) treated immunoglobulin preparation Exploring beyond clinical routine SARS-CoV-2 serology using MultiCoV-Ab to evaluate endemic coronavirus cross-reactivity Immune response to SARS-CoV-2 variants of concern in vaccinated individuals Glucocorticoids and B cell depleting agents substantially impair immunogenicity of mRNA vaccines to SARS-CoV-2. medRxiv : the preprint server for health sciences COVID-19 vaccines: where we stand and challenges ahead Correlates of protection from SARS-CoV-2 infection Potential SARS-CoV-2 immune correlates of protection in infection and vaccine immunization Immunogenicity of COVID-19 Tozinameran vaccination in patients on chronic dialysis mRNA vaccines against H10N8 and H7N9 influenza viruses of pandemic potential are immunogenic and well tolerated in healthy adults in phase 1 randomized clinical trials COVID-19 vaccine BNT162b1 elicits human antibody and TH1 T cell responses Enhanced SARS-CoV-2 neutralization by dimeric IgA IgA dominates the early neutralizing antibody response to SARS-CoV-2 Interleukin-18, interleukin-18 binding protein and impaired production of interferon-gamma in chronic renal failure Low-flux hemodialysis suppresses interferon-gamma production: the possible role of beta2-microglobulin Age-related immune response heterogeneity to SARS-CoV-2 vaccine BNT162b2 Confounding factors influencing the kinetics and magnitude of serological response following administration of BNT162b2 Impact of age, ethnicity, sex and prior infection status on immunogenicity following a single dose of the BNT162b2 mRNA COVID-19 vaccine: real-world evidence from healthcare workers Initial observations on age, gender, BMI and hypertension in antibody responses to SARS-CoV-2 BNT162b2 vaccine SARS-CoV-2 vaccines for all but a single dose for COVID-19 survivors We sincerely thank all patients for their contribution and willingness to participate in this study. We also thank the clinical staff for their additional efforts to make this study possible. Data relating to the findings of this study are available from the corresponding authors upon request. Supplementary material associated with this article can be found in the online version at doi:10.1016/j.ebiom.2021.103524.