rabbit anti ifn γ (Bioss)

Bioss rabbit anti ifn γ

The accumulation of Gr-1 + CD11b + MDSC cells in the tumor microenvironment of the Apc Min/ + mice compared with the normal intestine tissues from the C57 mice; the Gr-1 + cells were decreased in the tumor microenvironment of the Apc Min/ + ;CD11b −/− mice ( a ). The number of the Ly6G + Ly6C low subset of MDSCs (gated on CD45 + cells) in the bone marrow of C57, CD11b −/− , Apc Min/ + and Apc Min/ + ;CD11b −/− mice ( b ) and in the peripheral blood, spleen and tumor tissues of the Apc Min/ + and Apc Min/ + ;CD11b −/− mice ( c ) was measured by FACS. The results of the IF staining and FACS represent of 11 independent mice (all mice were 16–weeks-old). The proteins expression of <t>IFN-γ</t> and CXCL9 in the tumor tissues from the Apc Min/ + and Apc Min/ + ;CD11b −/− mice was examined by immunoblotting ( d ). The protein bands intensities were quantitated and normalized to those of GAPDH. The statistical data are expressed as the means ± S.D. * P <0.05, ** P < 0.01 and *** P < 0.001. Scale bars: 50 μm ( a ).

Rabbit Anti Ifn 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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ifnγ (Bioss)

Bioss ifnγ

Lung metastasis in the LM8‐inoculated mice

Ifnγ, supplied by Bioss, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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bs-0481r (bioss)

bioss bs-0481r

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rabbit anti ifn g polyclonal antibody (Bioss)

Bioss rabbit anti ifn g polyclonal antibody

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anti ifn γ (Bioss)

Bioss anti ifn γ

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ifnγ alexafluor488 (Bioss)

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polyclonal rabbit serum specific for ifn (Genzyme)

Genzyme polyclonal rabbit serum specific for ifn

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ifn-γ polyclonal antibody (ImmunoWay Biotechnology Company)

ImmunoWay Biotechnology Company ifn-γ polyclonal antibody

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recombinant human ifn-α2b (Daiichi Pharmaceutical Co)

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polyclonal biotinylated anti-mouse ifn-γ antibody (PeproTech)

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biotinylated anti-ifn-γ polyclonal detector antibody (Becton Dickinson)

Becton Dickinson biotinylated anti-ifn-γ polyclonal detector antibody

T-cell repertoire diversity and SIV-specific immune response in malaria- and SIV-infected monkeys. A Diversity index differences with respect to the 8th week of SIV infection (corresponding to malaria introduction in the S + P group). Repertoire diversity was restored in the S + P group but not in the P + S group. A significant difference between the S + P and P + S groups was observed for the Shannon diversity index. P -values computed using ANOVA. B Ratio of SIV-specific clonotype frequency with respect to the control point (8th week of SIV infection, corresponding to malaria introduction in the S + P group). The S + P group, but not the P + S group, was characterized by a persistently higher SIV-specific clonotype frequency. P -values were calculated using ANOVA. C New SIV-specific clonotype production. Fractions of existing (detected at previous sampling point) and new SIV-specific clonotypes shown for each monkey in the P + S, S and S + P groups. A significant increase in new SIV-specific clonotype production was observed in the S + P group during the whole period of Plasmodium infection (at 11–17 weeks and 50 weeks post SIV infection). D Frequency of <t>IFN-g-producing</t> SIV Gag-specific PBMCs. Number of <t>IFN-γ-producing</t> PBMCs against pooled SIV Gag peptides analyzed by ELISPOT. The sample sizes were 6, 4 and 5 on day 49 and 4, 3, and 5 on day 161 of the S, P + S and S + P groups, respectively. SFC: spot-forming cells

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polyclonal antibody to ifn-gamma (PeproTech)

PeproTech polyclonal antibody to ifn-gamma

Conjugation of BP to cytokines relative to <t> IFN-γ </t>

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Image Search Results

Journal: Scientific Reports

Article Title: CD11b deficiency suppresses intestinal tumor growth by reducing myeloid cell recruitment

doi: 10.1038/srep15948

Figure Lengend Snippet: The accumulation of Gr-1 + CD11b + MDSC cells in the tumor microenvironment of the Apc Min/ + mice compared with the normal intestine tissues from the C57 mice; the Gr-1 + cells were decreased in the tumor microenvironment of the Apc Min/ + ;CD11b −/− mice ( a ). The number of the Ly6G + Ly6C low subset of MDSCs (gated on CD45 + cells) in the bone marrow of C57, CD11b −/− , Apc Min/ + and Apc Min/ + ;CD11b −/− mice ( b ) and in the peripheral blood, spleen and tumor tissues of the Apc Min/ + and Apc Min/ + ;CD11b −/− mice ( c ) was measured by FACS. The results of the IF staining and FACS represent of 11 independent mice (all mice were 16–weeks-old). The proteins expression of IFN-γ and CXCL9 in the tumor tissues from the Apc Min/ + and Apc Min/ + ;CD11b −/− mice was examined by immunoblotting ( d ). The protein bands intensities were quantitated and normalized to those of GAPDH. The statistical data are expressed as the means ± S.D. * P <0.05, ** P < 0.01 and *** P < 0.001. Scale bars: 50 μm ( a ).

Article Snippet: The primary antibodies were used for immunohistochemical (IHC), immunofluorescence (IF) analysis and Western blotting (WB) assays: and mouse anti-BrdU antibody (RPN202, diluted at 1:150 for IHC) was obtained from GE Healthcare (Little Chalfond, UK); rabbit anti-CyclinD1 (BM0771, diluted at 1:100 for IHC and 1:400 for WB), rabbit anti-CD34 (BA0532, diluted at 1:100 for IHC), rabbit anti-CD45 (BA3371, diluted at 1:100 for IHC) and rabbit anti-p65 (BA0610, diluted at 1:100 for IHC) were obtained from Boster (Wuhan, China); mouse anti-TNF-α (ab10863, diluted at 1:5000 for WB) was obtained from Abcam (Cambridge, UK); rabbit anti-IFN-γ (bs-0480R), rabbit anti-CXCL-9 (bs-2551R) (both diluted at 1:500 for WB), rabbit anti-CD11b (bs-1014R) and rabbit anti-Gr-1 (bs-2576R, diluted at 1:100 for IF) were obtained from Bioss (Beijing, China); mouse anti-Cytokeratin 8 (CK8, ZM-0310, diluted at 1:100 for IF) was purchased from ZSGB-BIO (Beijing, China); mouse anti-CD11b (Santa Cruz, USA, diluted at 1:100 for IF); mouse anti-E-cadherin (#610181, diluted at 1:100 for IHC and 1:5000 for WB) and mouse anti-β-catenin (#610154, diluted at 1:100 for IHC, and 1:2000 for WB) were purchased from BD Transduction Laboratories (Franklin Lakes, NJ); rabbit anti-GAPDH (#2118s, diluted at 1:2000 for WB) was purchased from CST (USA); rabbit anti-pp65 (Ser276, sc-101749, diluted at 1:500 for IHC) was obtained from Santa Cruz Biotechnology Inc. (USA).

Techniques: Staining, Expressing, Western Blot

Journal: FASEB bioAdvances

Article Title: Manipulation of the tumor microenvironment by cytokine gene transfection enhances dendritic cell‐based immunotherapy

doi: 10.1096/fba.2019-00052

Figure Lengend Snippet: Lung metastasis in the LM8‐inoculated mice

Article Snippet: Cells infiltrating tumor tissues were evaluated by immunohistochemistry using following primary Abs: for IFNγ, Bioss Cat# bs‐0480R‐PE‐Cy7, RRID:AB_11092092; for CD40L, Biorbyt Cat# orb10326, RRID:AB_10746923; for CD8, clone 53‐6.7, Thermo Fisher Scientific Cat# 14‐0081‐81, RRID:AB_467086; for Foxp3, clone FJK‐16s, Thermo Fisher Scientific Cat# 14‐5773‐80, RRID:AB_467575; for Iba1, Wako Pure Chemical Industries Inc, Cat# 019‐19741, RRID:AB_839504; for granzyme B, Spring Bioscience Cat# E2580, RRID:AB_1661202.

Techniques:

Effect of IFNγ and CD40L (Comb) gene‐transfection on DC‐based therapy. (A) Survival of mice with the indicated treatments. (B) The relative tumor volume (with the volume on day 0 set at 1) of each mouse in the control groups. Black solid lines indicate the relative tumor volumes of the [Untreated] group; black dotted lines indicate those of the [Cont (IT)] group; gray solid lines indicate those of the [Cont (IV)] group. (C) The relative tumor volume of each mouse in the intratumoral (IT) gene‐administrated group. Black solid lines indicate relative tumor volumes of the [Comb (IT) +DC] group. Black dotted lines indicate those of the [Comb (IT)] group. Gray solid lines indicate those of the [Cont (IT) + DC] group. (D) The relative tumor volume of each mouse in the intravenous (IV) gene‐administrated group. Black solid lines indicate relative tumor volumes of the [Comb (IV) +DC] group. Black dotted lines indicate those of the [Comb (IV)] group. Gray solid lines indicate those of the [Cont (IV) + DC] group. Experiments were performed independently three times using a total of six mice in each group. All mice were humanely euthanized according to the criteria in Section . * P < .05, vs the [Cont (IT)] group. ** P < .05 vs the [Untreated] group, and P < .01, vs the [Cont (IV)] group. *** P < .05 vs the [Untreated] group, and P < .005, vs the [Cont (IT) +DC] group or the [Cont (IV) +DC] group, respectively

Journal: FASEB bioAdvances

Article Title: Manipulation of the tumor microenvironment by cytokine gene transfection enhances dendritic cell‐based immunotherapy

doi: 10.1096/fba.2019-00052

Figure Lengend Snippet: Effect of IFNγ and CD40L (Comb) gene‐transfection on DC‐based therapy. (A) Survival of mice with the indicated treatments. (B) The relative tumor volume (with the volume on day 0 set at 1) of each mouse in the control groups. Black solid lines indicate the relative tumor volumes of the [Untreated] group; black dotted lines indicate those of the [Cont (IT)] group; gray solid lines indicate those of the [Cont (IV)] group. (C) The relative tumor volume of each mouse in the intratumoral (IT) gene‐administrated group. Black solid lines indicate relative tumor volumes of the [Comb (IT) +DC] group. Black dotted lines indicate those of the [Comb (IT)] group. Gray solid lines indicate those of the [Cont (IT) + DC] group. (D) The relative tumor volume of each mouse in the intravenous (IV) gene‐administrated group. Black solid lines indicate relative tumor volumes of the [Comb (IV) +DC] group. Black dotted lines indicate those of the [Comb (IV)] group. Gray solid lines indicate those of the [Cont (IV) + DC] group. Experiments were performed independently three times using a total of six mice in each group. All mice were humanely euthanized according to the criteria in Section . * P < .05, vs the [Cont (IT)] group. ** P < .05 vs the [Untreated] group, and P < .01, vs the [Cont (IV)] group. *** P < .05 vs the [Untreated] group, and P < .005, vs the [Cont (IT) +DC] group or the [Cont (IV) +DC] group, respectively

Techniques: Transfection

Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on the infiltration of CD8 + cells into LM8 tumors. Tumor tissue was collected from mice with the indicated treatments at 7 d after the second treatment. Immunohistochemistry was performed to detect CD8 + cells present in the tumor tissue. (A) Typical photos of tumors collected from the indicated treatment groups are shown. Expression of CD8 is shown as brown color products. (B) Counts of CD8 + cells in 1000 cells in tumors are shown. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Journal: FASEB bioAdvances

Article Title: Manipulation of the tumor microenvironment by cytokine gene transfection enhances dendritic cell‐based immunotherapy

doi: 10.1096/fba.2019-00052

Figure Lengend Snippet: Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on the infiltration of CD8 + cells into LM8 tumors. Tumor tissue was collected from mice with the indicated treatments at 7 d after the second treatment. Immunohistochemistry was performed to detect CD8 + cells present in the tumor tissue. (A) Typical photos of tumors collected from the indicated treatment groups are shown. Expression of CD8 is shown as brown color products. (B) Counts of CD8 + cells in 1000 cells in tumors are shown. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Techniques: Transfection, Immunohistochemistry, Expressing

Effect of the IFNγ and CD40L (Comb) gene‐transfection therapy on tumor‐infiltrating cells. Tumor tissue was collected from mice with the indicated treatments at 7 d after the second treatment. The Iba 1 + activated macrophage and granzyme B + killer cells in the tumor tissue were detected by immunohistochemistry. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Journal: FASEB bioAdvances

Article Title: Manipulation of the tumor microenvironment by cytokine gene transfection enhances dendritic cell‐based immunotherapy

doi: 10.1096/fba.2019-00052

Figure Lengend Snippet: Effect of the IFNγ and CD40L (Comb) gene‐transfection therapy on tumor‐infiltrating cells. Tumor tissue was collected from mice with the indicated treatments at 7 d after the second treatment. The Iba 1 + activated macrophage and granzyme B + killer cells in the tumor tissue were detected by immunohistochemistry. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Techniques: Transfection, Immunohistochemistry

Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on tumor‐infiltrating cells. Tumor tissue was collected from mice with the indicated treatments at 7 d after the second treatment. Mature DCs (MHC II high CD83 + cells), MDSCs (CD11b + , Gr1 + cells), NK (NK1.1 + ) cells and PD‐L1 + cells in the tumor tissues were detected in FCM. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Journal: FASEB bioAdvances

Article Title: Manipulation of the tumor microenvironment by cytokine gene transfection enhances dendritic cell‐based immunotherapy

doi: 10.1096/fba.2019-00052

Figure Lengend Snippet: Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on tumor‐infiltrating cells. Tumor tissue was collected from mice with the indicated treatments at 7 d after the second treatment. Mature DCs (MHC II high CD83 + cells), MDSCs (CD11b + , Gr1 + cells), NK (NK1.1 + ) cells and PD‐L1 + cells in the tumor tissues were detected in FCM. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Techniques: Transfection

Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on systemic immune responses. Spleen cells were collected from the LM8 tumor‐bearing mice with the indicated treatments at 7 d after the second treatment. Cytotoxic activity of the cells against LM8 (A), BW5147 (B), and YAC‐1 (C) was evaluated in vitro. The experiments were repeated twice. Each experiment was performed using three mice in each treatment group. A typical result is shown. All mice were humanely euthanized according to the criteria in Section . Results are expressed as mean ± SE. * P < .05, ** P < .01 vs the [Untreated] group, † P < .05 vs the [Comb (IT) + DC] and [Comb (IV)] group at the E/T ratio

Journal: FASEB bioAdvances

Article Title: Manipulation of the tumor microenvironment by cytokine gene transfection enhances dendritic cell‐based immunotherapy

doi: 10.1096/fba.2019-00052

Figure Lengend Snippet: Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on systemic immune responses. Spleen cells were collected from the LM8 tumor‐bearing mice with the indicated treatments at 7 d after the second treatment. Cytotoxic activity of the cells against LM8 (A), BW5147 (B), and YAC‐1 (C) was evaluated in vitro. The experiments were repeated twice. Each experiment was performed using three mice in each treatment group. A typical result is shown. All mice were humanely euthanized according to the criteria in Section . Results are expressed as mean ± SE. * P < .05, ** P < .01 vs the [Untreated] group, † P < .05 vs the [Comb (IT) + DC] and [Comb (IV)] group at the E/T ratio

Techniques: Transfection, Activity Assay, In Vitro

Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on spleen cells. Spleen was collected from mice with the indicated treatments at 7 days after the second treatment. Mature DCs (MHC II high CD83 + cells), MDSCs (CD11b + , Gr1 + cells), NK (NK1.1 + ) cells and PDL‐1 + cells in the tumor tissues were detected in FCM. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Journal: FASEB bioAdvances

Article Title: Manipulation of the tumor microenvironment by cytokine gene transfection enhances dendritic cell‐based immunotherapy

doi: 10.1096/fba.2019-00052

Figure Lengend Snippet: Effect of IFNγ and CD40L (Comb) gene‐transfection therapy on spleen cells. Spleen was collected from mice with the indicated treatments at 7 days after the second treatment. Mature DCs (MHC II high CD83 + cells), MDSCs (CD11b + , Gr1 + cells), NK (NK1.1 + ) cells and PDL‐1 + cells in the tumor tissues were detected in FCM. Results are expressed as mean ± SE. The experiment was performed using three mice in each treatment group. All mice were humanely euthanized according to the criteria in Section . * P < .05, ** P < .01 by the Tukey‐Kramer test

Techniques: Transfection

Journal: International Journal of Molecular Sciences

Article Title: Alginate Oligosaccharides Repair Liver Injury by Improving Anti-Inflammatory Capacity in a Busulfan-Induced Mouse Model

doi: 10.3390/ijms24043097

Figure Lengend Snippet: Antibodies used for WB and IHF.

Article Snippet: IFN-γ , bs-0481R , www.bioss.com.cn.

Techniques:

Journal: Cell Communication and Signaling : CCS

Article Title: Subsequent malaria enhances virus-specific T cell immunity in SIV-infected Chinese rhesus macaques

doi: 10.1186/s12964-022-00910-7

Figure Lengend Snippet: T-cell repertoire diversity and SIV-specific immune response in malaria- and SIV-infected monkeys. A Diversity index differences with respect to the 8th week of SIV infection (corresponding to malaria introduction in the S + P group). Repertoire diversity was restored in the S + P group but not in the P + S group. A significant difference between the S + P and P + S groups was observed for the Shannon diversity index. P -values computed using ANOVA. B Ratio of SIV-specific clonotype frequency with respect to the control point (8th week of SIV infection, corresponding to malaria introduction in the S + P group). The S + P group, but not the P + S group, was characterized by a persistently higher SIV-specific clonotype frequency. P -values were calculated using ANOVA. C New SIV-specific clonotype production. Fractions of existing (detected at previous sampling point) and new SIV-specific clonotypes shown for each monkey in the P + S, S and S + P groups. A significant increase in new SIV-specific clonotype production was observed in the S + P group during the whole period of Plasmodium infection (at 11–17 weeks and 50 weeks post SIV infection). D Frequency of IFN-g-producing SIV Gag-specific PBMCs. Number of IFN-γ-producing PBMCs against pooled SIV Gag peptides analyzed by ELISPOT. The sample sizes were 6, 4 and 5 on day 49 and 4, 3, and 5 on day 161 of the S, P + S and S + P groups, respectively. SFC: spot-forming cells

Article Snippet: The plates were washed with PBST (PBS containing 0.05% Tween-20), and a biotinylated anti-IFN-γ polyclonal detector antibody (BD Biosciences) was added.

Techniques: Infection, Sampling, Enzyme-linked Immunospot

Conjugation of BP to cytokines relative to IFN-γ

Journal:

Article Title: Benzylpenicillin differentially conjugates to IFN-?, TNF-?, IL-1?, IL-4 and IL-13 but selectively reduces IFN-? activity

doi: 10.1046/j.1365-2249.2003.02069.x

Figure Lengend Snippet: Conjugation of BP to cytokines relative to IFN-γ

Article Snippet: For analysis of BP effects on cytokine multimer formation, blots were incubated with polyclonal antibody to IFN-γ, TNF-α or IL-2 (Peprotech), at 0·2 or 0·4 μg/ml and visualized in the same way.

Techniques: Conjugation Assay

BP has no effect on cytokine oligomerization. IFN-γ, IL-2 and TNF-α, each at 10 µg/ml in PBS, were incubated with or without 5 mg/ml BP overnight at 37°C. Samples were analysed by SDS-PAGE and Western blotted with the appropriate polyclonal anti-cytokine antibody.

Journal:

Article Title: Benzylpenicillin differentially conjugates to IFN-?, TNF-?, IL-1?, IL-4 and IL-13 but selectively reduces IFN-? activity

doi: 10.1046/j.1365-2249.2003.02069.x

Figure Lengend Snippet: BP has no effect on cytokine oligomerization. IFN-γ, IL-2 and TNF-α, each at 10 µg/ml in PBS, were incubated with or without 5 mg/ml BP overnight at 37°C. Samples were analysed by SDS-PAGE and Western blotted with the appropriate polyclonal anti-cytokine antibody.

Techniques: Incubation, SDS Page, Western Blot

Effect of BP on the ability of(a)IL-1β,(b)TNF-α or(c)IFN-γ to induce CD54 expression on A549 cells. Each cytokine (100 ng/ml) was incubated in RT2 with (○) or without (•) BP (2 mg/ml) for 4 days at 37°C, then each preparation was assayed at 0·02, 0·2, 2 or 10 ng/ml. Confluent layers of A549 cells in 96-well plates were incubated overnight with cytokine preparations. After fixing, CD54 expression was measured by ELISA. ▴ Cytokine incubated 4 days alone, 2 mg/ml BP added immediately before assay. Results represent mean ± SEM of 3 (IL-1β and TNF-α) or 4 (IFN-γ) experiments, each performed in triplictate. *P < 0·05, by paired Student's t-test, for comparison of untreated to BP-treated IFN-γ.

Journal:

Article Title: Benzylpenicillin differentially conjugates to IFN-?, TNF-?, IL-1?, IL-4 and IL-13 but selectively reduces IFN-? activity

doi: 10.1046/j.1365-2249.2003.02069.x

Figure Lengend Snippet: Effect of BP on the ability of(a)IL-1β,(b)TNF-α or(c)IFN-γ to induce CD54 expression on A549 cells. Each cytokine (100 ng/ml) was incubated in RT2 with (○) or without (•) BP (2 mg/ml) for 4 days at 37°C, then each preparation was assayed at 0·02, 0·2, 2 or 10 ng/ml. Confluent layers of A549 cells in 96-well plates were incubated overnight with cytokine preparations. After fixing, CD54 expression was measured by ELISA. ▴ Cytokine incubated 4 days alone, 2 mg/ml BP added immediately before assay. Results represent mean ± SEM of 3 (IL-1β and TNF-α) or 4 (IFN-γ) experiments, each performed in triplictate. *P < 0·05, by paired Student's t-test, for comparison of untreated to BP-treated IFN-γ.

Techniques: Expressing, Incubation, Enzyme-linked Immunosorbent Assay, Comparison

Effect of temperature on BP conjugation to IFN-γ. IFN-γ, at 10 µg/ml in PBS, was incubated with or without 5 mg/ml BP overnight at 4 or 37°C. Samples were analysed by SDS-PAGE and Western blotted with rabbit polyclonal anti-BP antibody.

Journal:

Article Title: Benzylpenicillin differentially conjugates to IFN-?, TNF-?, IL-1?, IL-4 and IL-13 but selectively reduces IFN-? activity

doi: 10.1046/j.1365-2249.2003.02069.x

Figure Lengend Snippet: Effect of temperature on BP conjugation to IFN-γ. IFN-γ, at 10 µg/ml in PBS, was incubated with or without 5 mg/ml BP overnight at 4 or 37°C. Samples were analysed by SDS-PAGE and Western blotted with rabbit polyclonal anti-BP antibody.

Techniques: Conjugation Assay, Incubation, SDS Page, Western Blot

Effect of temperature and serum on BP reduction of IFN-γ activity. IFN-γ was incubated, at 100 ng/ml, at different temperatures in RT2, or in varying concentrations of FCS for 4 days with or without 2 mg/ml BP. Confluent layers of A549 cells in 96-well plates were incubated overnight with each cytokine preparation at a final concentration of 2 ng/ml. After fixing, CD54 expression was measured by ELISA. Results represent mean ± SEM of 4 experiments, each performed in triplictate.*P < 0·01 by paired Student's t-test, for comparison of untreated to BP-treated IFN-γ.□ medium alone, IFN-γ, ▪ IFN-γ+ BP.

Journal:

Article Title: Benzylpenicillin differentially conjugates to IFN-?, TNF-?, IL-1?, IL-4 and IL-13 but selectively reduces IFN-? activity

doi: 10.1046/j.1365-2249.2003.02069.x

Figure Lengend Snippet: Effect of temperature and serum on BP reduction of IFN-γ activity. IFN-γ was incubated, at 100 ng/ml, at different temperatures in RT2, or in varying concentrations of FCS for 4 days with or without 2 mg/ml BP. Confluent layers of A549 cells in 96-well plates were incubated overnight with each cytokine preparation at a final concentration of 2 ng/ml. After fixing, CD54 expression was measured by ELISA. Results represent mean ± SEM of 4 experiments, each performed in triplictate.*P < 0·01 by paired Student's t-test, for comparison of untreated to BP-treated IFN-γ.□ medium alone, IFN-γ, ▪ IFN-γ+ BP.

Techniques: Activity Assay, Incubation, Concentration Assay, Expressing, Enzyme-linked Immunosorbent Assay, Comparison

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