Harmonization and qualification of an IFN-γ Enzyme-Linked ImmunoSpot assay (ELISPOT) to measure influenza-specific cell-mediated immunity within the FLUCOP consortium

Waerlop, Gwenn; Leroux‐Roels, Geert; Lambe, Teresa; Bellamy, Duncan; Medaglini, Donata; Pettini, Elena; Trieu, Mai-Chi; Davies, Richard A.; Bredholt, Geir; Montomoli, Emanuele; Gianchecchi, Elena; Clement, Frédéric

doi:10.3389/fimmu.2022.984642

Cited by 8 publications

(3 citation statements)

References 31 publications

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“…At present, the quantitative detection method of IFN-γ is conducted through immunological methods. ELISA [16] [17] [23] and Enzyme-Linked Immunospot Assay (ELISPOT) [24] [25] are the current clinically existing methods to detect IFN-γ. The reagent We use the prepared sensing method and detect a good linear relation between the fluorescence intensity and the level of IFN-γ within the range of 0.5 -100 ng/mL, and the LOD is 0.303 ng/mL.…”

Section: Discussionmentioning

confidence: 99%

Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-<i>γ</i>

Wen¹,

Song²,

Cui³

et al. 2023

JBM

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Purpose: Interferon-γ (INF-γ) is a cytokine that participates in the immune reaction of the body. Its level of secretion can reflect the immune response condition after the body is infected by pathogens, which is a significant indication of clinically-related diseases. Therefore, it is of great significance in application to develop a fluorescence biosensor to inspect INF-γ with rapidness, high sensitivity and high practicability. Method: The fluorescence sensor is made on the basis of the two-dimensional nano-material namely Carbon Nitride Nanosheet (CNNS) and the Aptamer probe to identify INF-γ (Apt@INF-γ). CNNS can quickly quench the Cy5 fluorescent dye modified on the Apt@INF-γ probe due to the Photoinduced Electron Transfer (PET), but when the INF-γ exists, Apt@INF-γ specifically identifies and combines it. The complex of Apt@INF-γ and INF-γ is away from CNNS, which can effectively block the fluorescent signal of Apt@INF-γ being quenched by CNNS. Result: The sensitive detection of IFN-γ protein can be achieved through the application of CNNS/Apt@INF-γ fluorescence sensing platform. In this method, the intensity of the fluorescent signal is positively correlated with the concentration of IFN-γ, of which the liner response range is 0.5 -100 ng/mL and the limit of detection is 0.303 ng/mL. In addition, this fluorescence sensing platform has the advantages of high specificity, simple operation and low costs. It can inspect the content of IFN-γ in clinical serum samples without interference. The actual recovery rate of serum samples is 97.11% -106.96%. Conclusion: Therefore, the CNNS/Apt@INF-γ sensing platform is expected to be implemented in the actual clinical detection, also conducive to developing a universal fluorescence biosensor to inspect other target materials.

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Section: Discussionmentioning

confidence: 99%

Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-<i>γ</i>

Wen¹,

Song²,

Cui³

et al. 2023

JBM

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“…The CD4 + polypositive (or polyfunctional) T-cell response detected here is generally important for an effective viral vaccine and often correlates with better protection against viral diseases ( 51 ). Therefore, with respect to correlates of protection, cell-mediated responses should be explored more thoroughly, as recently shown for flu vaccines ( 52 – 55 ). Cell-mediated responses elicited by norovirus vaccine candidates may contribute to vaccine-induced protection and should be investigated more thoroughly, as suggested by our data and other studies ( 20 , 56 – 58 ).…”

Section: Discussionmentioning

confidence: 99%

Immune responses in healthy adults elicited by a bivalent norovirus vaccine candidate composed of GI.4 and GII.4 VLPs without adjuvant

et al. 2023

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The development of an efficacious vaccine against norovirus is of paramount importance given its potential to reduce the global burden of norovirus-associated morbidity and mortality. Here, we report a detailed immunological analysis of a phase I, double-blind, placebo-controlled clinical trial performed on 60 healthy adults, ages 18 to 40. Total serum immunoglobulin and serum IgA against vaccine strains and cross-reactive serum IgG against non-vaccine strains were measured by enzyme immunoassays, whereas cell-mediated immune responses were quantified using intracellular cytokine staining by flow cytometry. A significant increase in humoral and cellular responses, e.g., IgA and CD4+ polypositive T cells, was triggered by the GI.4 Chiba 407 (1987) and GII.4 Aomori 2 (2006) VLP-based norovirus vaccine candidate rNV-2v, which is formulated without adjuvant. No booster effect was observed after the second administration in the pre-exposed adult study population. Furthermore, a cross-reactive immune response was elicited, as shown by IgG titers against GI.3 (2002), GII.2 OC08154 (2008), GII.4 (1999), GII.4 Sydney (2012), GII.4 Washington (2018), GII.6 Maryland (2018), and GII.17 Kawasaki 308 (2015). Due to viral infection via mucosal gut tissue and the high variety of potentially relevant norovirus strains, a focus should be on IgA and cross-protective humoral and cell-mediated responses in the development of a broadly protective, multi-valent norovirus vaccine.Clinical trial registrationhttps://clinicaltrials.gov, identifier NCT05508178. EudraCT number: 2019-003226-25.

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“…With the advancement of immunology-related basic research, the detection technologies for antigen-specific T lymphocytes are also rapidly developing and improving. ELISpot and ICS are classical techniques widely used to detect and enumerate activated antigen-specific T cells secreting cytokines such as IFN-g or TNF-a (63,64). Both assays combined with SARS-CoV-2 overlapping peptide pools or single epitope stimulation of peripheral blood mononuclear cells (PBMCs) or tissue samples are widely used in the detecting and identifying SARS-CoV-2 specific T cells, with the advantage of high sensitivity (17,22,28,65,66).…”

Section: Detection Methods Of Sars-cov-2 Specific T Cellmentioning

confidence: 99%

SARS-CoV-2 epitope-specific T cells: Immunity response feature, TCR repertoire characteristics and cross-reactivity

Yang

Wang²,

Sun³

et al. 2023

Front. Immunol.

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The devastating COVID-19 pandemic caused by SARS-CoV-2 and multiple variants or subvariants remains an ongoing global challenge. SARS-CoV-2-specific T cell responses play a critical role in early virus clearance, disease severity control, limiting the viral transmission and underpinning COVID-19 vaccine efficacy. Studies estimated broad and robust T cell responses in each individual recognized at least 30 to 40 SARS-CoV-2 antigen epitopes and associated with COVID-19 clinical outcome. Several key immunodominant viral proteome epitopes, including S protein- and non-S protein-derived epitopes, may primarily induce potent and long-lasting antiviral protective effects. In this review, we summarized the immune response features of immunodominant epitope-specific T cells targeting different SRAS-CoV-2 proteome structures after infection and vaccination, including abundance, magnitude, frequency, phenotypic features and response kinetics. Further, we analyzed the epitopes immunodominance hierarchy in combination with multiple epitope-specific T cell attributes and TCR repertoires characteristics, and discussed the significant implications of cross-reactive T cells toward HCoVs, SRAS-CoV-2 and variants of concern, especially Omicron. This review may be essential for mapping the landscape of T cell responses toward SARS-CoV-2 and optimizing the current vaccine strategy.

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Harmonization and qualification of an IFN-γ Enzyme-Linked ImmunoSpot assay (ELISPOT) to measure influenza-specific cell-mediated immunity within the FLUCOP consortium

Cited by 8 publications

References 31 publications

Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-<i>γ</i>

Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-<i>γ</i>

Immune responses in healthy adults elicited by a bivalent norovirus vaccine candidate composed of GI.4 and GII.4 VLPs without adjuvant

SARS-CoV-2 epitope-specific T cells: Immunity response feature, TCR repertoire characteristics and cross-reactivity

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Harmonization and qualification of an IFN-γ Enzyme-Linked ImmunoSpot assay (ELISPOT) to measure influenza-specific cell-mediated immunity within the FLUCOP consortium

Cited by 8 publications

References 31 publications

Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-&lt;i&gt;γ&lt;/i&gt;

Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-&lt;i&gt;γ&lt;/i&gt;

Immune responses in healthy adults elicited by a bivalent norovirus vaccine candidate composed of GI.4 and GII.4 VLPs without adjuvant

SARS-CoV-2 epitope-specific T cells: Immunity response feature, TCR repertoire characteristics and cross-reactivity

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Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-<i>γ</i>

Construction of Fluorescence Sensing Platform on the Basis of Carbon Nitride Nanosheet for the Detection of Interferon-<i>γ</i>