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Image Search Results
Journal: Immunology
Article Title: Anti‐CD52 antibody treatment in murine experimental autoimmune encephalomyelitis induces dynamic and differential modulation of innate immune cells in peripheral immune and central nervous systems
doi: 10.1111/imm.13437
Figure Lengend Snippet: Effect of anti‐CD52‐Ab treatment on the phenotype of periphery innate immune cells in EAE mice at first day post‐injection. Single‐cell suspensions were obtained from blood and spleen tissue of anti‐CD52‐Ab or vehicle‐treated EAE mice at first day after the final dose injection. Cells were stained for various surface markers and analysed by flow cytometry. (A) Flow cytometry gating strategy. (B) Blood and spleen CD11c + cells were analysed for expression of MHC‐II ( n = 9), CD40 ( n = 5), CD80 ( n = 5) and CD86 ( n = 9 blood; n = 5 spleen). (C) Blood and spleen CD11b + cells were analysed for expression of MHC‐II ( n = 8), CD40 ( n = 5), CD80 ( n = 5), CD86 ( n = 5), CD38 ( n = 5) and CD206 ( n = 9 blood; n = 7 spleen). Unpaired two‐tailed Student's t test. * p < 0·05, ** p < 0·01, *** p < 0·001
Article Snippet: To block non‐specific Fc receptors, cells were resuspended in anti‐mouse CD16/CD32 Fc block (eBioscience) for 10 min before incubation with the appropriate antibodies against: CD11b (#130‐113‐236), CD11c (#130‐102‐545), CD38 (#130‐109‐257),
Techniques: Injection, Staining, Flow Cytometry, Expressing, Two Tailed Test
Journal: Immunology
Article Title: Anti‐CD52 antibody treatment in murine experimental autoimmune encephalomyelitis induces dynamic and differential modulation of innate immune cells in peripheral immune and central nervous systems
doi: 10.1111/imm.13437
Figure Lengend Snippet: Effect of anti‐CD52‐Ab treatment on the phenotype and function of CNS innate immune cells in EAE mice at first day post‐injection. Single‐cell suspensions were obtained from CNS (brain and spinal cord) tissue of anti‐CD52‐Ab or vehicle‐treated EAE mice at first day after the final treatment dose. Cells were stained for various surface markers and analysed by flow cytometry. (A) Flow cytometry gating strategy. (B) CD11b + CD45 lo/neg resident microglia and (C) CNS CD11b + CD45 hi infiltrating macrophages and were analysed for expression of MHC‐II ( n = 10), CD40 ( n = 5), CD80 ( n = 5), CD86 ( n = 5 microglia; n = 9 macrophages) and CD206 ( n = 7 microglia; n = 5 macrophages). Unpaired two‐tailed Student's t test. CD11b + cells were isolated from CNS tissue of anti‐CD52‐Ab or vehicle‐treated mice at first day after the final treatment dose. (D) Respiratory burst activity of CD11b + ‐isolated cells. (E) Phagocytosis of FITC‐coated beads by CD11b + isolated cells. Unpaired two‐tailed Student's t test. (F) Cells were left unstimulated or were stimulated with LPS or Poly(I:C)(PIC) for 24 h and cytokine production determined by ELISA. Two‐way ANOVA with Sidak multiple comparisons test, * p < 0·05, ** p < 0·01, *** p < 0·001
Article Snippet: To block non‐specific Fc receptors, cells were resuspended in anti‐mouse CD16/CD32 Fc block (eBioscience) for 10 min before incubation with the appropriate antibodies against: CD11b (#130‐113‐236), CD11c (#130‐102‐545), CD38 (#130‐109‐257),
Techniques: Injection, Staining, Flow Cytometry, Expressing, Two Tailed Test, Isolation, Activity Assay, Enzyme-linked Immunosorbent Assay
Journal: Immunology
Article Title: Anti‐CD52 antibody treatment in murine experimental autoimmune encephalomyelitis induces dynamic and differential modulation of innate immune cells in peripheral immune and central nervous systems
doi: 10.1111/imm.13437
Figure Lengend Snippet: Effect of anti‐CD52‐Ab treatment on the phenotype of periphery and CNS innate immune cells in EAE mice at three weeks post‐injection. Single‐cell suspensions were obtained from blood, spleen and CNS (brain and spinal cord) tissue of anti‐CD52‐Ab or vehicle‐treated mice three weeks after the final treatment dose. Cells were stained for various surface markers and analysed by flow cytometry. (A) Blood and spleen CD11c + cells were analysed for expression of MHC‐II ( n = 9), CD40 ( n = 5), CD80 ( n = 5) and CD86 ( n = 9 blood; n = 5 spleen). (B) Blood and spleen CD11b + cells were analysed for expression of MHC‐II ( n = 8), CD40 ( n = 5), CD80 ( n = 5), CD86 ( n = 5), CD38 ( n = 5) and CD206 ( n = 9 blood; n = 7 spleen). (C) CNS CD11b + CD45 hi ‐infiltrating macrophages and CD11b + CD45 lo/neg resident microglia were analysed for expression of MHC‐II ( n = 10), CD40 ( n = 5), CD80 ( n = 5), CD86 ( n = 5 microglia; n = 9 macrophages) and CD206 ( n = 7 microglia; n = 5 macrophages). Unpaired two‐tailed Student's t test. * p < 0·05, ** p < 0·01, *** p < 0·001
Article Snippet: To block non‐specific Fc receptors, cells were resuspended in anti‐mouse CD16/CD32 Fc block (eBioscience) for 10 min before incubation with the appropriate antibodies against: CD11b (#130‐113‐236), CD11c (#130‐102‐545), CD38 (#130‐109‐257),
Techniques: Injection, Staining, Flow Cytometry, Expressing, Two Tailed Test
Journal: Immunology
Article Title: Anti‐CD52 antibody treatment in murine experimental autoimmune encephalomyelitis induces dynamic and differential modulation of innate immune cells in peripheral immune and central nervous systems
doi: 10.1111/imm.13437
Figure Lengend Snippet: Effect of anti‐CD52‐Ab treatment on the function of periphery and CNS innate immune cells in SCID mice at first day post‐injection. SCID mice were treated with either vehicle or 10 mg/kg murine anti‐CD52‐Ab‐Ab for five consecutive days. Single‐cell suspensions were then obtained from blood and spleen tissues first day after the final treatment dose. Cells were stained for various surface markers and analysed by flow cytometry. (A) Blood and spleen CD11c + cells were analysed for expression of MHC‐II, CD40, CD80 and CD86 (all n = 7). (B) Blood and spleen CD11b + cells were analysed for expression of MHC‐II, CD40, CD80, CD86, and CD206 (all n = 7). Unpaired two‐tailed Student's t test. * p < 0·05, ** p < 0·01, *** p < 0·001
Article Snippet: To block non‐specific Fc receptors, cells were resuspended in anti‐mouse CD16/CD32 Fc block (eBioscience) for 10 min before incubation with the appropriate antibodies against: CD11b (#130‐113‐236), CD11c (#130‐102‐545), CD38 (#130‐109‐257),
Techniques: Injection, Staining, Flow Cytometry, Expressing, Two Tailed Test
Journal: Translational Oncology
Article Title: Adipose tissue from oesophageal adenocarcinoma patients is differentially affected by chemotherapy and chemoradiotherapy regimens altering immune cell phenotype and cancer cell metabolism
doi: 10.1016/j.tranon.2025.102302
Figure Lengend Snippet: Chemoradiotherapy treated adipose secretome significantly increases immunoinhibitory markers TIM-3 on unpolarised Mɸ. A-L) Expression of unpolarised Mɸ phenotypic and immunoinhibitory markers including viability, CD68, CD11b, CD11c, HLA-DR, TIM-3, CD80, CD86, CD80+CD86+, CD163, CD206, and CD163+CD206+ following exposure to untreated, chemotherapy treated (FLOT) and chemoradiotherapy treated (CROSS) adipose conditioned media, (Friedman test with Dunn's correction). L) PCA analysis of Mɸs polarisation marker expression following culture with the treated adipose secretome through dimensionality reduction. All data expressed as mean ± SEM, n = 6, associated p-value displayed above comparison, only signifcant results shown.
Article Snippet: Antibodies used for Mɸ staining included CD11b-FITC, CD11c-Vio-Blue, CD80-PE, CD206-APC-Vio770, CD86-PerCp-Vio700, HLA-DR-Vio-Green, TIM-3-APC,
Techniques: Expressing, Marker, Comparison
Journal: Translational Oncology
Article Title: Adipose tissue from oesophageal adenocarcinoma patients is differentially affected by chemotherapy and chemoradiotherapy regimens altering immune cell phenotype and cancer cell metabolism
doi: 10.1016/j.tranon.2025.102302
Figure Lengend Snippet: Chemotherapy treated adipose secretome significantly increases M1 polarised Mɸ expression of phenotypic and immune-inhibitory ligands whilst the chemoradiotherapy treated adipose secretome increases M2 polarised Mɸ expression of CD206. A-I) Expression of LPS M1 primed Mɸ phenotypic and immunoinhibitory markers including viability, CD68, CD11b, CD11c, HLA-DR, TIM-3, CD80, CD86 as well as co-expression of CD80 and CD86 following exposure to untreated, chemotherapy treated (FLOT) and chemoradiotherapy treated (CROSS) adipose conditioned media, (Friedman test with Dunn's correction). J) PCA analysis of M1-primed Mɸ polarisation marker expression following culture with the treated adipose secretome through dimensionality reduction. K-S) Expression of IL-4 M2 primed Mɸ phenotypic and immunoinhibitory markers including viability, CD68, CD11b, CD11c, HLA-DR, TIM-3, CD163, CD206 as well as co-expression of CD163 and CD206 following exposure to chemotherapy treated (FLOT) and chemoradiotherapy treated (CROSS) adipose conditioned media, (Friedman test with Dunn's correction). T) PCA analysis of M2-primed Mɸ polarisation marker expression following culture with the treated adipose secretome through dimensionality reduction. All data expressed as mean ± SEM, n = 6, associated p-value displayed above comparison, only signifcant results shown.
Article Snippet: Antibodies used for Mɸ staining included CD11b-FITC, CD11c-Vio-Blue, CD80-PE, CD206-APC-Vio770, CD86-PerCp-Vio700, HLA-DR-Vio-Green, TIM-3-APC,
Techniques: Expressing, Marker, Comparison