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anti ifn γ  (Bioss)


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    Bioss anti ifn γ
    Anti Ifn γ, supplied by Bioss, used in various techniques. Bioz Stars score: 95/100, based on 91 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/anti ifn γ/product/Bioss
    Average 95 stars, based on 91 article reviews
    anti ifn γ - by Bioz Stars, 2026-03
    95/100 stars

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    anti ifnγ antibody  (Bioss)
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    Systemic deletion of ZNRF1 promotes EAE pathogenesis and neuroinflammation in mice. Age-matched female Znrf1 +/+ and Znrf1 −/− mice were immunized with 200 μg of MOG 35-55 peptide emulsified in Complete Freund’s Adjuvant (CFA), followed by intraperitoneal (i.p.) injection of 200 ng pertussis toxin (PTX) to induce EAE. a Clinical scores of EAE progression were monitored and recorded daily ( N = 40). b Body weights of immunized mice were measured and normalized to their respective weights at day 8 post-immunization ( N = 40). c At day 18 post-EAE induction, spinal cords from female Znrf1 +/+ and Znrf1 −/− mice were harvested to prepare single-cell suspensions. Cells were stained with antibodies against CD45, CD4, CD8, and CD11b, followed by flow cytometry analysis to quantify leucocytes (CD45 + ), T helper (Th) cells (CD45 + CD4 + ), cytotoxic T cells (CD45 + CD8 + ), and myeloid cells (CD45 + CD11b + ) ( N = 6). Representative flow plots and quantified cell numbers of infiltrating immune cells in the CNS are presented. d - f Spinal cord tissue sections from Znrf1 +/+ and Znrf1 −/− mice were collected and analyzed at day 18 post-EAE induction. d Tissue sections were stained with hematoxylin and eosin (H&E) to assess inflammatory cell infiltration and with luxol fast blue (LFB) to evaluate white matter demyelination. e and f Tissue sections were subjected to immunohistochemistry (IHC) using antibodies against CD3 (T cells) <t>and</t> <t>CD68</t> (macrophages) ( e ) or <t>IFNγ</t> (Th1 cells) and IL-17A (Th17 cells) ( f ). d - f Scale bars: 200 μm (whole spinal cord sections) and 100 μm (enlarged region #1 and #2). g Flow cytometric analysis of naïve CD4 + T cells (CD4 + CD44 − CD62L + ), central memory CD4 + T (T CM ) cells (CD4 + CD44 + CD62L + ), and effector memory CD4 + T (T EM ) cells (CD4 + CD44 + CD62L − ) in the spleens and draining lymph nodes (DLNs) of Znrf1 +/+ (N = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. h Flow cytometric analysis of naïve CD8 + T cells (CD8 + CD44 − CD62L + ), CD8 + T (T CM ) cells (CD8 + CD44 + CD62L + ), and effector memory CD8 + T (T EM ) cells (CD8 + CD44 + CD62L − ) in the spleens and DLNs of Znrf1 +/+ ( n = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. i -k Flow cytometric analysis of Th1 (CD4 + IFNγ + ) cells ( i ), Th17 (CD4 + IL-17A + ) cells ( j ), and cytotoxic T (CD8 + IFNγ + ) cells ( k ) in the spleens and DLNs of Znrf1 +/+ ( n = 3) and Znrf1 −/− mice ( N = 3) at day 18 post-EAE induction. ( a and b ) Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the Wilcoxon matched-pairs signed-rank test. d-f Representative spinal cord sections and quantification of infiltrating immune cells or demyelination in Znrf1 +/+ and Znrf1 −/− mice are shown. g - k Representative flow cytometry plots and quantified T cell populations in the spleens and DLNs. c - k Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the unpaired Student’s t -test
    Anti Ifnγ Antibody, supplied by Bioss, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    inf γ  (Bioss)
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    Systemic deletion of ZNRF1 promotes EAE pathogenesis and neuroinflammation in mice. Age-matched female Znrf1 +/+ and Znrf1 −/− mice were immunized with 200 μg of MOG 35-55 peptide emulsified in Complete Freund’s Adjuvant (CFA), followed by intraperitoneal (i.p.) injection of 200 ng pertussis toxin (PTX) to induce EAE. a Clinical scores of EAE progression were monitored and recorded daily ( N = 40). b Body weights of immunized mice were measured and normalized to their respective weights at day 8 post-immunization ( N = 40). c At day 18 post-EAE induction, spinal cords from female Znrf1 +/+ and Znrf1 −/− mice were harvested to prepare single-cell suspensions. Cells were stained with antibodies against CD45, CD4, CD8, and CD11b, followed by flow cytometry analysis to quantify leucocytes (CD45 + ), T helper (Th) cells (CD45 + CD4 + ), cytotoxic T cells (CD45 + CD8 + ), and myeloid cells (CD45 + CD11b + ) ( N = 6). Representative flow plots and quantified cell numbers of infiltrating immune cells in the CNS are presented. d - f Spinal cord tissue sections from Znrf1 +/+ and Znrf1 −/− mice were collected and analyzed at day 18 post-EAE induction. d Tissue sections were stained with hematoxylin and eosin (H&E) to assess inflammatory cell infiltration and with luxol fast blue (LFB) to evaluate white matter demyelination. e and f Tissue sections were subjected to immunohistochemistry (IHC) using antibodies against CD3 (T cells) <t>and</t> <t>CD68</t> (macrophages) ( e ) or <t>IFNγ</t> (Th1 cells) and IL-17A (Th17 cells) ( f ). d - f Scale bars: 200 μm (whole spinal cord sections) and 100 μm (enlarged region #1 and #2). g Flow cytometric analysis of naïve CD4 + T cells (CD4 + CD44 − CD62L + ), central memory CD4 + T (T CM ) cells (CD4 + CD44 + CD62L + ), and effector memory CD4 + T (T EM ) cells (CD4 + CD44 + CD62L − ) in the spleens and draining lymph nodes (DLNs) of Znrf1 +/+ (N = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. h Flow cytometric analysis of naïve CD8 + T cells (CD8 + CD44 − CD62L + ), CD8 + T (T CM ) cells (CD8 + CD44 + CD62L + ), and effector memory CD8 + T (T EM ) cells (CD8 + CD44 + CD62L − ) in the spleens and DLNs of Znrf1 +/+ ( n = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. i -k Flow cytometric analysis of Th1 (CD4 + IFNγ + ) cells ( i ), Th17 (CD4 + IL-17A + ) cells ( j ), and cytotoxic T (CD8 + IFNγ + ) cells ( k ) in the spleens and DLNs of Znrf1 +/+ ( n = 3) and Znrf1 −/− mice ( N = 3) at day 18 post-EAE induction. ( a and b ) Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the Wilcoxon matched-pairs signed-rank test. d-f Representative spinal cord sections and quantification of infiltrating immune cells or demyelination in Znrf1 +/+ and Znrf1 −/− mice are shown. g - k Representative flow cytometry plots and quantified T cell populations in the spleens and DLNs. c - k Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the unpaired Student’s t -test
    Inf γ, supplied by Bioss, used in various techniques. Bioz Stars score: 95/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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    Role of miR-4664-3p antagomir in a NSCLC xenograft mouse model. (A) Gross appearance of tumors in each group. (B) Measurement of tumor weight. (C) Tumor volume comparison between antagomir NC and miR-4664-3p antagomir groups. (D) Immunofluorescence staining of CD8 + T cells (red) and IFN-γ (green) in tumor tissues; nuclei were counterstained with DAPI (blue). (E, F) Quantification of CD8⁺ T cells and IFNγ⁺ CD8⁺ T cells. (G) Measurement of IFN-γ fluorescence intensity (IOD/Area). (H) qRT-PCR analysis of PRKCB mRNA expression in tumor tissues. * P < 0.05, ** P < 0.01, *** P < 0.001. ns, not significant.

    Journal: Frontiers in Oncology

    Article Title: MiR-4664-3p as a potential diagnostic, prognostic, and immunotherapeutic biomarker in NSCLC: modulation of tumor progression through CD8 + T cell regulation

    doi: 10.3389/fonc.2025.1642999

    Figure Lengend Snippet: Role of miR-4664-3p antagomir in a NSCLC xenograft mouse model. (A) Gross appearance of tumors in each group. (B) Measurement of tumor weight. (C) Tumor volume comparison between antagomir NC and miR-4664-3p antagomir groups. (D) Immunofluorescence staining of CD8 + T cells (red) and IFN-γ (green) in tumor tissues; nuclei were counterstained with DAPI (blue). (E, F) Quantification of CD8⁺ T cells and IFNγ⁺ CD8⁺ T cells. (G) Measurement of IFN-γ fluorescence intensity (IOD/Area). (H) qRT-PCR analysis of PRKCB mRNA expression in tumor tissues. * P < 0.05, ** P < 0.01, *** P < 0.001. ns, not significant.

    Article Snippet: Tumor tissues were processed for immunofluorescence with antibodies against CD8 (Abcam, ab217344) and IFN-γ (Bioss, bs-0480R), using TSA reagent (Pino-Bio) for signal amplification.

    Techniques: Comparison, Immunofluorescence, Staining, Fluorescence, Quantitative RT-PCR, Expressing

    Systemic deletion of ZNRF1 promotes EAE pathogenesis and neuroinflammation in mice. Age-matched female Znrf1 +/+ and Znrf1 −/− mice were immunized with 200 μg of MOG 35-55 peptide emulsified in Complete Freund’s Adjuvant (CFA), followed by intraperitoneal (i.p.) injection of 200 ng pertussis toxin (PTX) to induce EAE. a Clinical scores of EAE progression were monitored and recorded daily ( N = 40). b Body weights of immunized mice were measured and normalized to their respective weights at day 8 post-immunization ( N = 40). c At day 18 post-EAE induction, spinal cords from female Znrf1 +/+ and Znrf1 −/− mice were harvested to prepare single-cell suspensions. Cells were stained with antibodies against CD45, CD4, CD8, and CD11b, followed by flow cytometry analysis to quantify leucocytes (CD45 + ), T helper (Th) cells (CD45 + CD4 + ), cytotoxic T cells (CD45 + CD8 + ), and myeloid cells (CD45 + CD11b + ) ( N = 6). Representative flow plots and quantified cell numbers of infiltrating immune cells in the CNS are presented. d - f Spinal cord tissue sections from Znrf1 +/+ and Znrf1 −/− mice were collected and analyzed at day 18 post-EAE induction. d Tissue sections were stained with hematoxylin and eosin (H&E) to assess inflammatory cell infiltration and with luxol fast blue (LFB) to evaluate white matter demyelination. e and f Tissue sections were subjected to immunohistochemistry (IHC) using antibodies against CD3 (T cells) and CD68 (macrophages) ( e ) or IFNγ (Th1 cells) and IL-17A (Th17 cells) ( f ). d - f Scale bars: 200 μm (whole spinal cord sections) and 100 μm (enlarged region #1 and #2). g Flow cytometric analysis of naïve CD4 + T cells (CD4 + CD44 − CD62L + ), central memory CD4 + T (T CM ) cells (CD4 + CD44 + CD62L + ), and effector memory CD4 + T (T EM ) cells (CD4 + CD44 + CD62L − ) in the spleens and draining lymph nodes (DLNs) of Znrf1 +/+ (N = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. h Flow cytometric analysis of naïve CD8 + T cells (CD8 + CD44 − CD62L + ), CD8 + T (T CM ) cells (CD8 + CD44 + CD62L + ), and effector memory CD8 + T (T EM ) cells (CD8 + CD44 + CD62L − ) in the spleens and DLNs of Znrf1 +/+ ( n = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. i -k Flow cytometric analysis of Th1 (CD4 + IFNγ + ) cells ( i ), Th17 (CD4 + IL-17A + ) cells ( j ), and cytotoxic T (CD8 + IFNγ + ) cells ( k ) in the spleens and DLNs of Znrf1 +/+ ( n = 3) and Znrf1 −/− mice ( N = 3) at day 18 post-EAE induction. ( a and b ) Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the Wilcoxon matched-pairs signed-rank test. d-f Representative spinal cord sections and quantification of infiltrating immune cells or demyelination in Znrf1 +/+ and Znrf1 −/− mice are shown. g - k Representative flow cytometry plots and quantified T cell populations in the spleens and DLNs. c - k Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the unpaired Student’s t -test

    Journal: Journal of Neuroinflammation

    Article Title: Myeloid ZNRF1 suppresses autoimmune demyelination and neuroinflammation by regulating MHC-II-mediated T cell activation

    doi: 10.1186/s12974-025-03550-z

    Figure Lengend Snippet: Systemic deletion of ZNRF1 promotes EAE pathogenesis and neuroinflammation in mice. Age-matched female Znrf1 +/+ and Znrf1 −/− mice were immunized with 200 μg of MOG 35-55 peptide emulsified in Complete Freund’s Adjuvant (CFA), followed by intraperitoneal (i.p.) injection of 200 ng pertussis toxin (PTX) to induce EAE. a Clinical scores of EAE progression were monitored and recorded daily ( N = 40). b Body weights of immunized mice were measured and normalized to their respective weights at day 8 post-immunization ( N = 40). c At day 18 post-EAE induction, spinal cords from female Znrf1 +/+ and Znrf1 −/− mice were harvested to prepare single-cell suspensions. Cells were stained with antibodies against CD45, CD4, CD8, and CD11b, followed by flow cytometry analysis to quantify leucocytes (CD45 + ), T helper (Th) cells (CD45 + CD4 + ), cytotoxic T cells (CD45 + CD8 + ), and myeloid cells (CD45 + CD11b + ) ( N = 6). Representative flow plots and quantified cell numbers of infiltrating immune cells in the CNS are presented. d - f Spinal cord tissue sections from Znrf1 +/+ and Znrf1 −/− mice were collected and analyzed at day 18 post-EAE induction. d Tissue sections were stained with hematoxylin and eosin (H&E) to assess inflammatory cell infiltration and with luxol fast blue (LFB) to evaluate white matter demyelination. e and f Tissue sections were subjected to immunohistochemistry (IHC) using antibodies against CD3 (T cells) and CD68 (macrophages) ( e ) or IFNγ (Th1 cells) and IL-17A (Th17 cells) ( f ). d - f Scale bars: 200 μm (whole spinal cord sections) and 100 μm (enlarged region #1 and #2). g Flow cytometric analysis of naïve CD4 + T cells (CD4 + CD44 − CD62L + ), central memory CD4 + T (T CM ) cells (CD4 + CD44 + CD62L + ), and effector memory CD4 + T (T EM ) cells (CD4 + CD44 + CD62L − ) in the spleens and draining lymph nodes (DLNs) of Znrf1 +/+ (N = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. h Flow cytometric analysis of naïve CD8 + T cells (CD8 + CD44 − CD62L + ), CD8 + T (T CM ) cells (CD8 + CD44 + CD62L + ), and effector memory CD8 + T (T EM ) cells (CD8 + CD44 + CD62L − ) in the spleens and DLNs of Znrf1 +/+ ( n = 4) and Znrf1 −/− mice ( N = 4) at day 18 post-EAE induction. i -k Flow cytometric analysis of Th1 (CD4 + IFNγ + ) cells ( i ), Th17 (CD4 + IL-17A + ) cells ( j ), and cytotoxic T (CD8 + IFNγ + ) cells ( k ) in the spleens and DLNs of Znrf1 +/+ ( n = 3) and Znrf1 −/− mice ( N = 3) at day 18 post-EAE induction. ( a and b ) Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the Wilcoxon matched-pairs signed-rank test. d-f Representative spinal cord sections and quantification of infiltrating immune cells or demyelination in Znrf1 +/+ and Znrf1 −/− mice are shown. g - k Representative flow cytometry plots and quantified T cell populations in the spleens and DLNs. c - k Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the unpaired Student’s t -test

    Article Snippet: The slides were incubated with anti-CD3 antibody (#790–4341; clone, 2GV6; Ventana Medical Systems, Tucson, Arizona), anti-CD68 antibody (#ab125212; polyclonal; Abcam, Cambridge, UK), anti-IFNγ antibody (#BS-0480R; polyclonal, Bioss, Boston, USA), and anti-IL-17A antibody (#BS-1183R; polyclonal, Bioss, Boston, USA) at a 1:100 dilution for 120 min using the automated Ventana Benchmark XT system (Ventana Medical Systems).

    Techniques: Adjuvant, Injection, Staining, Flow Cytometry, Immunohistochemistry

    ZNRF1 deficiency in myeloid cells promotes EAE pathogenesis and neuroinflammation in mice. Age-matched female Znrf1 F/F and Znrf1 Δmye mice were immunized with 200 μg of MOG 35-55 peptide emulsified in CFA, followed by i.p. injection of 200 ng PTX to induce EAE. a Clinical scores of EAE progression were monitored and recorded daily (N = 42). b Body weights of immunized mice were measured and normalized to their respective weights at day 8 post-immunization. c At day 18 post-EAE induction, spinal cords from female Znrf1 F/F and Znrf1 Δmye mice were harvested to prepare single-cell suspensions. Cells were stained with antibodies against CD45, CD4, CD8, and CD11b, followed by flow cytometry analysis to quantify leucocytes (CD45 + ), Th cells (CD45 + CD4 + ), cytotoxic T cells (CD45 + CD8 + ), and myeloid cells (CD45 + CD11b + ) ( N = 6). d Flow cytometry analysis of Th1 (CD4 + IFNγ + ) and Th17 (CD4 + IL-17A + ) cells in the spinal cords of Znrf1 F/F ( N = 5) and Znrf1 Δmye mice ( N = 5) at day 18 post-EAE induction. e – g Spinal cord tissue sections from Znrf1 F/F and Znrf1 Δmye mice were collected and quantified at day 18 post-EAE induction. Tissue sections were subjected to H&E and LFB staining ( e ), and IHC staining using antibodies against CD3 (T cells) and CD68 (macrophages) ( f ) or IFNγ (Th1 cells) and IL-17A (Th1 cells) ( g ). Scale bars: 200 μm (whole spinal cord sections) and 100 μm (enlarged region #1 and #2). h - i Whole-mount imaging of the anterior ( h ) and posterior ( i ) spinal cord was performed in Znrf1 F/F and Znrf1 Δmye mice after EAE induction. At day 18 post-EAE induction, Znrf1 F/F and Znrf1 Δmye mice were perfused with wheat germ agglutinin (WGA) to label blood vessels (red). Spinal cords were collected and immunostained with antibodies against CD3 (green) to detect CD3 + T cells, lymphatic vessel endothelial hyaluronan receptor 1 (Lyve1) (magenta) for lymph vessels, and DAPI (white) for nuclei. Tissue clearing was performed as described in the METHODS section. Confocal images from whole-mount spinal cords and enlarged regions are shown. Scale bars: 2000 μm (whole-mount anterior spinal cord for Znrf1 F/F and Znrf1 Δmye mice and whole-mount posterior spinal cord for Znrf1 Δmye mice), 1000 μm (whole-mount posterior spinal cord for Znrf1 F/F mice), 200 μm (enlarged region #1), 100 μm (enlarged region #2 and #3). ( a , b ) Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the Wilcoxon matched-pairs signed-rank test. ( c and d ) Representative flow cytometry plots and quantified numbers of infiltrating immune cells in the CNS are shown. Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, determined by the unpaired Student’s t-test. ( e – g ) Representative spinal cord sections and quantification of infiltrating immune cells or demyelination in Znrf1 F/F and Znrf1 Δmye mice. Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, determined by the unpaired Student’s t-test

    Journal: Journal of Neuroinflammation

    Article Title: Myeloid ZNRF1 suppresses autoimmune demyelination and neuroinflammation by regulating MHC-II-mediated T cell activation

    doi: 10.1186/s12974-025-03550-z

    Figure Lengend Snippet: ZNRF1 deficiency in myeloid cells promotes EAE pathogenesis and neuroinflammation in mice. Age-matched female Znrf1 F/F and Znrf1 Δmye mice were immunized with 200 μg of MOG 35-55 peptide emulsified in CFA, followed by i.p. injection of 200 ng PTX to induce EAE. a Clinical scores of EAE progression were monitored and recorded daily (N = 42). b Body weights of immunized mice were measured and normalized to their respective weights at day 8 post-immunization. c At day 18 post-EAE induction, spinal cords from female Znrf1 F/F and Znrf1 Δmye mice were harvested to prepare single-cell suspensions. Cells were stained with antibodies against CD45, CD4, CD8, and CD11b, followed by flow cytometry analysis to quantify leucocytes (CD45 + ), Th cells (CD45 + CD4 + ), cytotoxic T cells (CD45 + CD8 + ), and myeloid cells (CD45 + CD11b + ) ( N = 6). d Flow cytometry analysis of Th1 (CD4 + IFNγ + ) and Th17 (CD4 + IL-17A + ) cells in the spinal cords of Znrf1 F/F ( N = 5) and Znrf1 Δmye mice ( N = 5) at day 18 post-EAE induction. e – g Spinal cord tissue sections from Znrf1 F/F and Znrf1 Δmye mice were collected and quantified at day 18 post-EAE induction. Tissue sections were subjected to H&E and LFB staining ( e ), and IHC staining using antibodies against CD3 (T cells) and CD68 (macrophages) ( f ) or IFNγ (Th1 cells) and IL-17A (Th1 cells) ( g ). Scale bars: 200 μm (whole spinal cord sections) and 100 μm (enlarged region #1 and #2). h - i Whole-mount imaging of the anterior ( h ) and posterior ( i ) spinal cord was performed in Znrf1 F/F and Znrf1 Δmye mice after EAE induction. At day 18 post-EAE induction, Znrf1 F/F and Znrf1 Δmye mice were perfused with wheat germ agglutinin (WGA) to label blood vessels (red). Spinal cords were collected and immunostained with antibodies against CD3 (green) to detect CD3 + T cells, lymphatic vessel endothelial hyaluronan receptor 1 (Lyve1) (magenta) for lymph vessels, and DAPI (white) for nuclei. Tissue clearing was performed as described in the METHODS section. Confocal images from whole-mount spinal cords and enlarged regions are shown. Scale bars: 2000 μm (whole-mount anterior spinal cord for Znrf1 F/F and Znrf1 Δmye mice and whole-mount posterior spinal cord for Znrf1 Δmye mice), 1000 μm (whole-mount posterior spinal cord for Znrf1 F/F mice), 200 μm (enlarged region #1), 100 μm (enlarged region #2 and #3). ( a , b ) Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, **** P < 0.0001, determined by the Wilcoxon matched-pairs signed-rank test. ( c and d ) Representative flow cytometry plots and quantified numbers of infiltrating immune cells in the CNS are shown. Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, *** P < 0.001, determined by the unpaired Student’s t-test. ( e – g ) Representative spinal cord sections and quantification of infiltrating immune cells or demyelination in Znrf1 F/F and Znrf1 Δmye mice. Data are presented as mean ± SD. ns, not significant. * P < 0.05, ** P < 0.01, determined by the unpaired Student’s t-test

    Article Snippet: The slides were incubated with anti-CD3 antibody (#790–4341; clone, 2GV6; Ventana Medical Systems, Tucson, Arizona), anti-CD68 antibody (#ab125212; polyclonal; Abcam, Cambridge, UK), anti-IFNγ antibody (#BS-0480R; polyclonal, Bioss, Boston, USA), and anti-IL-17A antibody (#BS-1183R; polyclonal, Bioss, Boston, USA) at a 1:100 dilution for 120 min using the automated Ventana Benchmark XT system (Ventana Medical Systems).

    Techniques: Injection, Staining, Flow Cytometry, Immunohistochemistry, Imaging