TO THE EDITOR:
Patients with hematological malignancies have been excluded from the new zoonotic coronavirus (severe acute respiratory syndrome coronavirus 2 [SARS-CoV-2]) vaccine trials,1,2 despite being at higher risk for SARS-CoV-2 disease (COVID-19)–related mortality.3-5 However, most health authorities worldwide have designated these patients as a priority for COVID-19 vaccination,6-12 even in the absence of efficacy data in these highly immunosuppressed patients. In addition, on 12 August 2021, the US Food and Drug Administration amended the emergency use authorizations for the Pfizer-BioNTech and Moderna COVID-19 vaccines to allow for the use of an additional dose in immunocompromised individuals, such as solid organ transplant recipients or equivalently immunosuppressed patients. This emergency use authorization prompted the American Society of Hematology to consider a third dose in immunocompromised patients with hematological malignancies who were being actively treated or were receiving high-dose corticosteroids at vaccination and/or agents causing prolonged B-cell lymphopenia within 12 months before vaccination, those with chronic lymphocytic leukemia, and recipients of chimeric antigen receptor T cells or a hematopoietic stem cell transplant (within 2 years).13 Again, the lack of prospective randomized clinical trials in immunosuppressed patients with hematological malignancies exploring the safety and efficacy of SARS-CoV-2 vaccines urge studies aimed at identifying which patients may or may not require a third vaccine dose before studying the potential benefit of this third booster dose.
To provide some rationale for these 2 pressing questions, we report a case-control analysis of the probabilities of exhibiting detectable SARS-CoV-2–reactive immunoglobulin G antibodies (SCoV2-R-A) at 3 weeks after a full vaccination schedule in a large series of patients with hematological malignancies and a history of SARS-CoV-2 infection (as defined by molecular or serological tests for SARS-CoV-2) before the first vaccine dose. The SCoV2-R-A detection rate in this cohort was compared with that observed in a control cohort of patients without evidence of prior SARS-CoV-2 infection at the time of vaccination. The latter included patients with hematological malignancies without prior polymerase chain reaction (PCR)-confirmed SARS-CoV-2 infection and a negative SCoV2-R-A serology test within 2 weeks of the first vaccine dose. The next step was to exclude patients with hematological malignancies and/or procedures not represented in the study group.
Both cohorts came from the Spanish Hematopoietic Stem Cell Transplantation and Cell Therapy Group multicenter prospective registry, which included 1568 consecutive patients with hematological malignancies who received a full vaccination schedule with any of the available compounds between 30 December 2020 and 30 June 2021 and who had available serological results performed 3 weeks after full vaccination. The algorithm selection of both cohorts is shown in supplemental Figure 1. All patients included in this registry gave their signed informed consent according to the Declaration of Helsinki. The local ethics committee of the Hospital Clinic Universitario of Valencia approved the registry and study protocol (reference code 35.21).
The presence of SCoV2-R-A was determined at each center using serological enzyme-linked immunosorbent assays or chemiluminescence immunoassays, following the manufacturers’ instructions, and based on their availability at the microbiology services of each participating center. The techniques used are shown in supplemental Table 1. For this study, we defined antibody detection or seropositivity when SCoV2-R-A were detected at any level above the lower limit level of detection for each of the tests used. The primary end points were to compare the rate of postvaccination seropositivity for SCoV2-R-A between cohorts, to identify the main factors associated with seropositivity, and to describe the characteristics of SCoV2-R-A detection in patients with prior SARS-CoV-2 infection as a model of a somewhat more natural immunological booster.
Overall, this series included 461 patients with hematological malignancies. The first cohort included 99 patients with prior SARS-CoV-2 infection, whereas the control cohort included 362 patients without prior COVID-19 history and a negative SCoV2-R-A serological test before the first vaccine dose. The clinical characteristics of both cohorts are detailed in Table 1. Eighty-two of 99 patients (82%) had prior PCR-confirmed COVID-19, whereas 17 (17%) were diagnosed at the time of SCoV2-R-A serological testing within 2 weeks of the first vaccine dose. Fifty-one of 82 patients with PCR-confirmed COVID-19 (62%) had prevaccination serological test results available. Of them, 33 (65%) were SCoV2-R-A positive and 18 (35%) were SCoV2-R-A negative. Differences between these cohorts included a higher rate of messenger RNA (mRNA)-1273 (or Moderna) vaccine administration and a higher frequency of recipients of allogeneic stem cells, whereas patients with prior SARS-CoV-2 infection had lower rates of baseline disease in complete remission, lower rates of patients treated >1 year before vaccination, and higher rates of tyrosine kinase inhibitor therapy. In terms of safety, self-reported adverse events were more common in patients with prior SARS-CoV-2 infection (14%) than in patients without (5%; P = .003) (supplemental Table 2). The SCoV2-R-A detection rate in patients with prior SARS-CoV-2 infection was 93% compared with 78% in those without (P < .0001). Of note, 15 of 18 patients (83%) with prior COVID-19 and negative SCoV2-R-A serostatus before vaccination mounted a SCoV2-R-A serological response at 3 weeks after full vaccination. Univariate and multivariate logistic regression analyses of factors associated with the detection of SCoV2-R-A at 3 weeks after full vaccination are shown in Table 2. Multivariate analysis confirmed that prior COVID-19 was the main factor associated with detectable SCoV2-R-A after vaccination (odds ratio, P = .001), whereas diagnosis of B-cell non-Hodgkin lymphoma (NHL), corticosteroid use, and lymphopenia (<1 × 109 lymphocytes per milliliter) at vaccination were associated with lower rates of SCoV2-R-A detection. Prior exposure to anti-CD20 therapy was also significantly associated with a lower response rate when we removed B-cell NHL from the multivariate analysis model (see footnote “‡” in Table 2).
Our findings indicate that patients with hematological malignancies with prior history of SARS-CoV-2 infection before vaccination achieve a high SCoV2-R-A detection rate (93%), similar to that reported in clinical trials of healthy subjects with mRNA vaccines.1,2 The most important limitation of this study is the use of several serological tests that may differ with regard to their detection range, sensitivity, and specificity. Thus, further confirmation of our findings using World Health Organization standardized tests is a priority for future research. Our finding indicates that these patients may not require an immediate SARS-CoV-2 vaccine booster dose, irrespective of current or past treatments, type and status of disease, or the absolute lymphocyte count at the time of vaccination. Furthermore, SARS-CoV-2 full-dose vaccination was able to reach seroconversion in 83% of patients with prior negative SCoV2-R-A, despite prior COVID-19. These data suggest that a booster dose in these highly immunosuppressed patients could likely elicit a humoral response similar to that observed in the healthy population and likely higher than prior experiences with mRNA SARS-CoV-2 vaccine booster doses in recipients of solid organ transplants, where the additional dose increased the seroconversion rate from 40% to 68%.14,15 Although the SARS-CoV-2 antibody detection rate in patients with hematological malignancies and prior SARS-CoV-2 infection is similar to that in the general population, and an up-front third dose could be questionable, it remains to be determined whether the duration of such a response is similar to the general population’s because immunocompromised patients may have more rapidly decreasing antibody titers, especially those who have undergone allogeneic stem cell transplantation or those in active treatment. If such a serological behavior is confirmed, a third dose could be advisable in this scenario. In line with early studies, we report that B-cell NHL6,11 (or treatment with anti-CD20 monoclonal antibodies), lymphopenia (<1 × 109 lymphocytes per milliliter),8 and corticosteroid therapy16 were associated with a lower probability of mounting SCoV2-R-A. After removing patients with B-cell NHL from the multivariate analysis, the significant effect of anti-CD20 monoclonal antibody therapy could be linked to chronic lymphocytic leukemia. However, we were not able to properly analyze the effect of anti-CD20 monoclonal antibody therapy in patients with chronic lymphocytic leukemia because of the limited number of such patients. Until more disease-specific data are available, these factors could be used to guide physicians in patient counseling with respect to a third vaccine dose. However, we believe that a third dose should be given in the context of prospective randomized clinical trials to overcome the lack of such evidence in these highly immunosuppressed patients. Finally, limitations of this study include the use of different serological tests in each center (results were not harmonized), the lack of neutralizing antibody testing, and the lack of SCoV2-R-A quantification in a significant number of cases. In contrast, the multicenter design, along with the large number of patients included, should be regarded as strengths.
Acknowledgments: The authors thank the Spanish Society of Hematology for support of the study. They sincerely appreciate the invaluable aid of microbiology services from all participating centers, in particular Santiago Garcia Muñoz (Microbiological Division, Hospital Clínico Universitario de Salamanca) and Tamar Talaván (Microbiological Division, Hospital Universitario Infanta Leonor, Madrid, Spain), for monitoring SCoV2-R-A in these highly immunosuppressed patients. The authors extend special thanks to the hematology units from all participating centers, as well as the patients, nurses, and study coordinators, for important contributions to this study.
REDCap (Research Electronic Data Capture) was developed by and is supported by the Vanderbilt Institute for Clinical and Translational Research.
Contribution: J.L.P., A.C., and A.S. conceived and designed the study; R.G.-S., M.G.-R., G.A.M.-M., I.R.-G., M.T., P.M.-B., S.M.-C., M.C., V.C., A.T., S.R.-P., and C.S. recruited patients for the study; and J.L.P., D.N., and R.M. analyzed data and generated the tables and figures.
Conflict-of-interest disclosure: The authors declare no competing financial interests.
Correspondence: José Luis Piñana, Division of Clinical Hematology, Hospital Clínico Universitario de Valencia, Avda Blasco Ibañez, 17, 46010 Valencia, Spain; e-mail: jlpinana@gmail.com.
References
Author notes
Requests for data sharing may be submitted to José Luis Piñana (jlpinana@gmail.com)
The full-text version of this article contains a data supplement.