The QuantiFERON Monitor<sup>®</sup> assay is predictive of infection post allogeneic hematopoietic cell transplantation

Douglas, Abby; Yu, Lingfei; Sundararajan, Vijaya; Szer, Jeff; Ritchie, David; Slavin, Monica A; Sasadeusz, Joe; Visvanathan, Kumar

doi:10.1111/tid.13260

Cited by 10 publications

(16 citation statements)

References 8 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…There is increasing interest in WB-based profiling of adaptive immune responses in infectious diseases and, to that end, a number of investigational and commercial assay systems have been developed [17,46]. WB assays for the detection of antigen-reactive T-cells have several important advantages over their PBMC-based counterparts as they require less blood volume and hands-on-time, facilitate improved standardization, and are often more cost-efficient [47][48][49].…”

Section: Discussionmentioning

confidence: 99%

“…To overcome these drawbacks, there is a growing interest in the development of whole blood (WB)-based protocols to determine T-cell responses to fungal antigens [15,16], following the clinical success of WB-based tests in tuberculosis and cytomegalovirus (CMV) diagnostics and research [17][18][19]. Although WB assays are more robust than PBMCbased protocols [16], concerns about impaired test performance remain when stimulation conditions are suboptimal, e.g., in the presence of immunosuppressive therapy or after long pre-analytic delays [16,[20][21][22][23].…”

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Development of a Simple and Robust Whole Blood Assay with Dual Co-Stimulation to Quantify the Release of T-Cellular Signature Cytokines in Response to Aspergillus fumigatus Antigens

Lauruschkat

Page

White

et al. 2021

JoF

View full text Add to dashboard Cite

Deeper understanding of mold-induced cytokine signatures could promote advances in the diagnosis and treatment of invasive mycoses and mold-associated hypersensitivity syndromes. Currently, most T-cellular immunoassays in medical mycology require the isolation of mononuclear cells and have limited robustness and practicability, hampering their broader applicability in clinical practice. Therefore, we developed a simple, cost-efficient whole blood (WB) assay with dual α-CD28 and α-CD49d co-stimulation to quantify cytokine secretion in response to Aspergillus fumigatus antigens. Dual co-stimulation strongly enhanced A. fumigatus-induced release of T-cellular signature cytokines detectable by enzyme-linked immunosorbent assay (ELISA) or a multiplex cytokine assay. Furthermore, T-cell-dependent activation and cytokine response of innate immune cells was captured by the assay. The protocol consistently showed little technical variation and high robustness to pre-analytic delays of up to 8 h. Stimulation with an A. fumigatus lysate elicited at least 7-fold greater median concentrations of key T-helper cell signature cytokines, including IL-17 and the type 2 T-helper cell cytokines IL-4 and IL-5 in WB samples from patients with Aspergillus-associated lung pathologies versus patients with non-mold-related lung diseases, suggesting high discriminatory power of the assay. These results position WB-ELISA with dual co-stimulation as a simple, accurate, and robust immunoassay for translational applications, encouraging further evaluation as a platform to monitor host immunity to opportunistic pathogens.

show abstract

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Development of a Simple and Robust Whole Blood Assay with Dual Co-Stimulation to Quantify the Release of T-Cellular Signature Cytokines in Response to Aspergillus fumigatus Antigens

Lauruschkat

Page

White

et al. 2021

JoF

View full text Add to dashboard Cite

show abstract

“…In fact the QFM levels seen in our cohort were more similar to bone marrow transplant recipients. 12 The ImmuKnow® assay (Cylex/Viracor-Eurofins, USA) is a widely studied immune biomarker that measures adenosine triphosphate (ATP) release from CD4+ T-lymphocytes after phytohemagglutinin-L (PHA) stimulation, which is thought to represent T-cell function. 4,21,22 Despite being FDA approved in 2002, there has not been widespread clinical uptake in this test mainly due to difficulties in defining cutoffs…”

Section: Discussionmentioning

confidence: 99%

“…11 More recently, QFM has been evaluated in bone marrow transplant recipients and low levels were associated with infections during the pre-engraftment period. 12 An improved ability to measure net state of immunosuppression would allow for individualization of immunosuppressive therapy before clinical events occur, potentially minimizing the risk of both under-immunosuppression leading to rejection and over-immunosuppression resulting in infection and drug toxicity. The aims of this study were to evaluate QFM both as a biomarker of immunosuppression and as a tool for the prediction of infection and rejection in a prospective observational cohort of lung transplant recipients (LTR).…”

Section: Back Groundmentioning

confidence: 99%

Evaluation of Quantiferon®‐Monitor as a biomarker of immunosuppression and predictor of infection in lung transplant recipients

Gardiner

Lee

Cristiano

et al. 2021

Transplant Infectious Dis

View full text Add to dashboard Cite

Background: Optimizing immunosuppression in lung transplant recipients (LTR) is crucially important in minimizing the risk of infection and rejection. Quantiferon®-Monitor (QFM) is a candidate immune function biomarker which has not yet been rigorously evaluated in the lung transplant setting. The aim of this prospective cohort study was to explore relationships between QFM results, immunosuppression, and infection/rejection in LTR. Methods: QFM, which measures interferon-γ after stimulation with innate and adaptive immune antigens, was tested before and at 2, 6, 12, 24 and 52 weeks post-transplant. Immunosuppression relationships were assessed with linear mixed effects models. Clinical outcomes were analyzed based on the preceding QFM result. Results: Eighty LTR were included. Median pre-transplant QFM levels were 171 IU/ mL (IQR 45-461), decreasing to 3 IU/mL (IQR 1-8) at 2 weeks post-transplant then progressively recovering toward baseline with time from transplant. Prednisolone was strongly inversely associated with QFM level (0.1 mg/kg dose increase correlating with 88 IU/mL QFM decrease, 95% CI 61-114, P < .001). Patients with QFM values <10 and <60 IU/mL were more likely to develop a serious opportunistic infection

show abstract

“…8,35 Recent studies reported that the ELISPOT assay for IFN-γ secretion of HCMV-specific CD8 + T cells performed well at predicting recurrent HCMV reactivation. 6,36 The HCMV serostatus of the patient and donor is one of the most important variables influencing HCMV-specific T cell immune reconstitution. 37,38 HCMV-seropositive recipients and donors (R + D + ) have a much faster reconstitution of HCMV-specific CD8 + T cells than HCMV-seropositive recipients transplanted from HCMVseronegative donors (R + D − ).…”

Section: Relationship Between Hcmv-igg Antibody and Ifn-γ Sfcs Countsmentioning

confidence: 99%

ELISPOT assay of interferon‐γ secretion for evaluating human cytomegalovirus reactivation risk in allo‐HSCT recipients

Liang

Xia

Zhang

et al. 2021

Journal of Medical Virology

View full text Add to dashboard Cite

Human cytomegalovirus (HCMV) is a common cause of significant morbidity and mortality in transplant recipients after allogeneic hematopoietic stem cell transplantation (allo-HSCT). We evaluated interferon-γ (IFN-γ) secretion by HCMV NLVspecific CD8 + T cells in HCMV-reactivated allo-HSCT recipients using an enzymelinked immunospot (ELISPOT) assay at 3 months post-transplantation. Blood samples from 47 recipients were tested for HCMV DNAemia, HCMV pp65 antigenemia, and anti-HCMV immunoglobulins (IgG/IgM) over 3 months post-transplantation. Of the 47 transplant recipients, 26 were HLA-A*02 positive and 21 were HLA-A*02 negative. The results were essentially consistent between the 47 transplant recipients and the HLA-A*02-positive recipients. HCMV DNAemia was not linearly correlated with IFN-γ spot-forming cells (SFCs) counts; IFN-γ SFCs counts did not differ significantly between the HCMV DNAemia-positive and -negative groups, whereas the HCMV-DNA virus loads were inversely correlated with the IFN-γ SFCs counts. HCMV pp65 antigenemia was not linearly correlated with IFN-γ SFCs counts; IFN-γ SFCs counts in the HCMV pp65 antigenemia-positive and -negative groups were similar. More IFN-γ SFCs counts were detected in transplant recipients with high anti-HCMV-IgG antibody titers than in those with low anti-HCMV-IgG titers pre-transplantation in the 47 recipients. Anti-HCMV-IgG antibody titers were positively linearly correlated with IFN-γ SFCs counts in HLA-A*02-positive recipients. The HCMV infection indicators used to monitor HCMV reactivation had different values in transplant recipients. The use of the IFN-γ SFCs counts measured by ELISPOT to evaluate the risk of HCMV reactivation needs further study.

show abstract

The QuantiFERON Monitor^® assay is predictive of infection post allogeneic hematopoietic cell transplantation

Cited by 10 publications

References 8 publications

Development of a Simple and Robust Whole Blood Assay with Dual Co-Stimulation to Quantify the Release of T-Cellular Signature Cytokines in Response to Aspergillus fumigatus Antigens

Development of a Simple and Robust Whole Blood Assay with Dual Co-Stimulation to Quantify the Release of T-Cellular Signature Cytokines in Response to Aspergillus fumigatus Antigens

Evaluation of Quantiferon®‐Monitor as a biomarker of immunosuppression and predictor of infection in lung transplant recipients

ELISPOT assay of interferon‐γ secretion for evaluating human cytomegalovirus reactivation risk in allo‐HSCT recipients

Contact Info

Product

Resources

About

The QuantiFERON Monitor® assay is predictive of infection post allogeneic hematopoietic cell transplantation

Cited by 10 publications

References 8 publications

Development of a Simple and Robust Whole Blood Assay with Dual Co-Stimulation to Quantify the Release of T-Cellular Signature Cytokines in Response to Aspergillus fumigatus Antigens

Development of a Simple and Robust Whole Blood Assay with Dual Co-Stimulation to Quantify the Release of T-Cellular Signature Cytokines in Response to Aspergillus fumigatus Antigens

Evaluation of Quantiferon®‐Monitor as a biomarker of immunosuppression and predictor of infection in lung transplant recipients

ELISPOT assay of interferon‐γ secretion for evaluating human cytomegalovirus reactivation risk in allo‐HSCT recipients

Contact Info

Product

Resources

About

The QuantiFERON Monitor^® assay is predictive of infection post allogeneic hematopoietic cell transplantation