FRINK Linked Data Fragments server

Matches in SemOpenAlex for { <https://semopenalex.org/work/W2028441972> ?p ?o ?g. }

• W2028441972 endingPage "452" @default.
• W2028441972 startingPage "450" @default.
• W2028441972 abstract "This panel was optimized to assess CD4+ and CD8+ T cell responses to various tumor antigens from melanoma patients. The panel was tested on single-cell derived T cell isolates (SCD-T) and T cell lines derived from peripheral blood mononuclear cells (PBMC) from melanoma patients, T cell lines from the tumor environment of melanoma patients, and fresh and cryopreserved PBMC (healthy donors). Staining can be performed in 96-well plates for high-throughput. The T cell response to human melanoma is broad, encompassing both effector and regulatory T cell populations with diverse functional profiles (1). Tumor specific T cells with cytokine profiles that do not follow the standard Th1/Th2 dichotomy have been demonstrated (2, 3). These descriptions include tumor antigen-specific effector and regulatory T cells that co-produce Th1 and Th2 cytokines. Thus, immunological monitoring of T cells from melanoma patients needs to assess a wide spectrum of functions and often has access to only a limited number of cells. To provide a tool for this immunological monitoring, we developed a panel of Ab-conjugates for assessing cytokine profiles that cross “traditional” T cell subset boundaries. As such, this panel would be useful for those interested in human T cells with a mixed cytokine profile, such as induced regulatory T cells, IL-10+ CD8+ T cells, T cells involved in allergic responses, etc. Further, it should be useful for samples with limited cell numbers, such as tumor biopsies, fine-needle aspirations, or cerebral spinal fluid, as well as samples from which multiple separate samples for Th1 versus Th2 intracellular cytokine staining are not possible. This panel was developed following guidelines described previously (4). To maximize sensitivity, the brightest fluorochromes were reserved for IL-2, IL-4, IL-10, IFN-γ, and TNF-α. A dump channel was used to exclude dead cells, B cells, and monocytes/macrophages. Next, testing a collection of Ab-conjugates optimized the differentiation of T cell subsets. APC-Cy7 and Quantum dot (QD) 605 were selected for discrimination of CD4 and CD8, respectively, because of their stability in this panel (Fig. 1 and Table 1). Gating strategy and example staining. A: Cells in the singlet gate are selected, live CD3+ CD14− CD19− cells identified, followed by exclusion of dye aggregates (gray box) and after gating on small lymphocytes, CD4+ and CD8+ T cells are selected for further analysis. CD4+ and CD8+ T cells positive for individual cytokines are separately gated and subsequently, a Boolean gate encompassing all combinations (25) of cytokine+/− T cells is created. The median fluorescence intensity (MFI) of cytokine+ T cells is evaluated, providing a measure of the magnitude of the response. B and C: Determination of cytokine+ T cells following gating described in (A). B: Shown is a CD4+ T cell line derived from the tumor of a melanoma patient stimulated with an allogeneic melanoma tumor cell line. The frequency of T cells positive for IFN-γ, TNF-α, IL-2, or IL-10 following antigenic stimulation was significantly greater than unstimulated T cells. C: Shown is a CD4+ T cell line derived from the tumor of a melanoma patient stimulated with an autologous melanoma tumor cell line. The frequency of T cells positive for TNF-α, IL-10, or IL-4 following antigenic stimulation was significantly greater than unstimulated T cells. The T cell lines in B and C are from two different patients stimulated with the same melanoma cell line. Data in B and C are presented as low-resolution dot plots. Robust cytokine responses from mitogen-stimulated PBMC are presented in Supporting Information Figure S7. CD3 was labeled after fixing and permeabilizing the cells to ensure that activated T cells having down-regulated their TCR/CD3 complex were included in the analysis (4). To permit resolution of CD4 following activation of T cells with PMA and ionomycin (used as a mitogenic control), CD4 was also labeled post-fixation/permeabilization for all samples. Specificity of the cytokine staining is demonstrated by reduced staining following blocking steps prior to intracellular staining with the fluorochrome-conjugated anticytokine reagents: (i) the surface-stained, fixed, and permeabilized cells are blocked with purified anticytokine antibodies of the identical clones and (ii) the fluorochrome-conjugated reagents are blocked with recombinant human cytokine (Table 2). These blocking steps typically reduce cytokine+ staining to background levels, or to a level allowing unambiguous gate setting, and as such these fully stained and blocked samples are used to determine placement of cytokine+ gates. This provides an alternative to individual FMO controls for each cytokine, which may not be feasible due to limited cell numbers from patient samples. The level of autofluorescence of the T cell lines has not been a substantial confounder in these experiments and we have not noted marked differences between the autofluorescence of cultured as compared with uncultured T cells from healthy donors. The Health Sciences Institutional Review Board that serves both the William S. Middleton Memorial Veterans Hospital and the University of Wisconsin-Madison approved this study (Human Subjects Protocol # 1992-031). Written informed consent was obtained from the participants in this study. OMIP-001 was designed to detect cytokine-producing T cells, including IL-2, IFN-γ, and TNF-α (5). Our panel extends OMIP-001 with the addition of IL-4 and IL-10, thus broadening its potential application for the discrimination of T cells exhibiting traditional Th1 and Th2 responses, as well as those with unconventional cytokine profiles. Additional Supporting Information may be found in the online version of this article. Please note: The publisher is not responsible for the content or functionality of any supporting information supplied by the authors. Any queries (other than missing content) should be directed to the corresponding author for the article." @default.
• W2028441972 created "2016-06-24" @default.
• W2028441972 creator A5034081251 @default.
• W2028441972 creator A5062531155 @default.
• W2028441972 date "2012-03-19" @default.
• W2028441972 modified "2023-10-17" @default.
• W2028441972 title "OMIP‐008: Measurement of Th1 and Th2 cytokine polyfunctionality of human T cells" @default.
• W2028441972 cites W1995570137 @default.
• W2028441972 cites W2024794399 @default.
• W2028441972 cites W2033256177 @default.
• W2028441972 cites W2077106927 @default.
• W2028441972 cites W2144350507 @default.
• W2028441972 doi "https://doi.org/10.1002/cyto.a.22035" @default.
• W2028441972 hasPubMedCentralId "https://www.ncbi.nlm.nih.gov/pmc/articles/3418807" @default.
• W2028441972 hasPubMedId "https://pubmed.ncbi.nlm.nih.gov/22431369" @default.
• W2028441972 hasPublicationYear "2012" @default.
• W2028441972 type Work @default.
• W2028441972 sameAs 2028441972 @default.
• W2028441972 citedByCount "8" @default.
• W2028441972 countsByYear W20284419722012 @default.
• W2028441972 countsByYear W20284419722014 @default.
• W2028441972 countsByYear W20284419722019 @default.
• W2028441972 countsByYear W20284419722020 @default.
• W2028441972 countsByYear W20284419722023 @default.
• W2028441972 crossrefType "journal-article" @default.
• W2028441972 hasAuthorship W2028441972A5034081251 @default.
• W2028441972 hasAuthorship W2028441972A5062531155 @default.
• W2028441972 hasBestOaLocation W20284419721 @default.
• W2028441972 hasConcept C137061746 @default.
• W2028441972 hasConcept C147483822 @default.
• W2028441972 hasConcept C154317977 @default.
• W2028441972 hasConcept C167672396 @default.
• W2028441972 hasConcept C202751555 @default.
• W2028441972 hasConcept C203014093 @default.
• W2028441972 hasConcept C2776090121 @default.
• W2028441972 hasConcept C2777658100 @default.
• W2028441972 hasConcept C2777701055 @default.
• W2028441972 hasConcept C2778690821 @default.
• W2028441972 hasConcept C2779727006 @default.
• W2028441972 hasConcept C502942594 @default.
• W2028441972 hasConcept C55493867 @default.
• W2028441972 hasConcept C71924100 @default.
• W2028441972 hasConcept C86803240 @default.
• W2028441972 hasConcept C8891405 @default.
• W2028441972 hasConceptScore W2028441972C137061746 @default.
• W2028441972 hasConceptScore W2028441972C147483822 @default.
• W2028441972 hasConceptScore W2028441972C154317977 @default.
• W2028441972 hasConceptScore W2028441972C167672396 @default.
• W2028441972 hasConceptScore W2028441972C202751555 @default.
• W2028441972 hasConceptScore W2028441972C203014093 @default.
• W2028441972 hasConceptScore W2028441972C2776090121 @default.
• W2028441972 hasConceptScore W2028441972C2777658100 @default.
• W2028441972 hasConceptScore W2028441972C2777701055 @default.
• W2028441972 hasConceptScore W2028441972C2778690821 @default.
• W2028441972 hasConceptScore W2028441972C2779727006 @default.
• W2028441972 hasConceptScore W2028441972C502942594 @default.
• W2028441972 hasConceptScore W2028441972C55493867 @default.
• W2028441972 hasConceptScore W2028441972C71924100 @default.
• W2028441972 hasConceptScore W2028441972C86803240 @default.
• W2028441972 hasConceptScore W2028441972C8891405 @default.
• W2028441972 hasIssue "6" @default.
• W2028441972 hasLocation W20284419721 @default.
• W2028441972 hasLocation W20284419722 @default.
• W2028441972 hasLocation W20284419723 @default.
• W2028441972 hasLocation W20284419724 @default.
• W2028441972 hasOpenAccess W2028441972 @default.
• W2028441972 hasPrimaryLocation W20284419721 @default.
• W2028441972 hasRelatedWork W1479981577 @default.
• W2028441972 hasRelatedWork W1991879524 @default.
• W2028441972 hasRelatedWork W2073641733 @default.
• W2028441972 hasRelatedWork W2171435634 @default.
• W2028441972 hasRelatedWork W2318823989 @default.
• W2028441972 hasRelatedWork W2351297599 @default.
• W2028441972 hasRelatedWork W2366209661 @default.
• W2028441972 hasRelatedWork W2376209413 @default.
• W2028441972 hasRelatedWork W2387430262 @default.
• W2028441972 hasRelatedWork W2902056154 @default.
• W2028441972 hasVolume "81A" @default.
• W2028441972 isParatext "false" @default.
• W2028441972 isRetracted "false" @default.
• W2028441972 magId "2028441972" @default.
• W2028441972 workType "article" @default.