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mouse abcf1 sirna  (Santa Cruz Biotechnology)


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    Santa Cruz Biotechnology mouse abcf1 sirna
    <t>ABCF1</t> promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.
    Mouse Abcf1 Sirna, supplied by Santa Cruz Biotechnology, used in various techniques. Bioz Stars score: 92/100, based on 4 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/mouse abcf1 sirna/product/Santa Cruz Biotechnology
    Average 92 stars, based on 4 article reviews
    mouse abcf1 sirna - by Bioz Stars, 2026-02
    92/100 stars

    Images

    1) Product Images from "An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses"

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    Journal: bioRxiv

    doi: 10.1101/2023.12.31.573785

    ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.
    Figure Legend Snippet: ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.

    Techniques Used: Activity Assay, Staining

    ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected out of three ABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the PE-αCD8 antibody and then stained with fluorescein by heat shock. Data is representative of two separate experiments.
    Figure Legend Snippet: ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected out of three ABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the PE-αCD8 antibody and then stained with fluorescein by heat shock. Data is representative of two separate experiments.

    Techniques Used: Activity Assay, Staining

    ABCF1 +/- mice produce fewer IFN γ positive CD8+ T lymphocytes after infection with VSV. ABCF1+/- splenocytes showed fewer IFNγ positive CD8+ T lymphocytes. Figure shown represents the results of one experiment, which was later repeated three times with similar results.
    Figure Legend Snippet: ABCF1 +/- mice produce fewer IFN γ positive CD8+ T lymphocytes after infection with VSV. ABCF1+/- splenocytes showed fewer IFNγ positive CD8+ T lymphocytes. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Techniques Used: Infection

    ABCF1+/- CTLs were as efficient as ABCF1 +/+ at killing of chromium. loaded VSV specific target lymphocytes. CTL activity was measured by the release of 51 Cr into the supernatant. Figure shown represents the results of one experiment, which was later repeated three times with similar results.
    Figure Legend Snippet: ABCF1+/- CTLs were as efficient as ABCF1 +/+ at killing of chromium. loaded VSV specific target lymphocytes. CTL activity was measured by the release of 51 Cr into the supernatant. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Techniques Used: Activity Assay

    ABCF1 is essential for the production of ISG (Interferon-Stimulated Gene) specific cytokines expression of INF- α and β after Poly(I:C) stimulation. A bar graph illustrating the fold change in the levels of INF-α and β cytokines detected in the cell culture supernatants. These findings provide insights into the impact of Abcf1 -specific siRNA treatment, both with and without Poly(I:C), on the secretion of cytokines and chemokines as well as the activation of key signaling pathways and transcription factors within BMDMs. Expression levels of the protein was assessed by western blotting analysis.
    Figure Legend Snippet: ABCF1 is essential for the production of ISG (Interferon-Stimulated Gene) specific cytokines expression of INF- α and β after Poly(I:C) stimulation. A bar graph illustrating the fold change in the levels of INF-α and β cytokines detected in the cell culture supernatants. These findings provide insights into the impact of Abcf1 -specific siRNA treatment, both with and without Poly(I:C), on the secretion of cytokines and chemokines as well as the activation of key signaling pathways and transcription factors within BMDMs. Expression levels of the protein was assessed by western blotting analysis.

    Techniques Used: Expressing, Cell Culture, Activation Assay, Protein-Protein interactions, Western Blot

    ABCF1 plays a role in regulating the phosphorylation levels of NF- κ B p65 and IRF3. A) Cytoplasmic and nuclear fractions obtained from BMDMs under different conditions were subjected to western blot analysis to assess the levels of transcription factors associated with Poly(I:C) stimulation confirming our hypothesis; Western Blot band sizes are as follows: anti- p65 (65 kD); anti p-p65 (65 kD); anti IRF3 (47 kD); anti p-IRF3 (36 kD); anti ABCF1 (110 kD); anti GAPDH (36 kD); anti histone H3 (15 kD); Dimerized-IRF3 (73 kD); IRF3 (36 kD) B) Whole-cell lysates were separated using native PAGE gel electrophoresis, and the analysis focused on examining the dimerization of IRF3, a transcription factor. Expression levels of the protein was assessed by western blotting analysis. Fold change calculations, as specified in the materials and methods section, were employed to quantify changes in the data. The bar graphs displayed in the figures represent the mean values along with standard deviations. The data presented here is representative of three separate experiments.
    Figure Legend Snippet: ABCF1 plays a role in regulating the phosphorylation levels of NF- κ B p65 and IRF3. A) Cytoplasmic and nuclear fractions obtained from BMDMs under different conditions were subjected to western blot analysis to assess the levels of transcription factors associated with Poly(I:C) stimulation confirming our hypothesis; Western Blot band sizes are as follows: anti- p65 (65 kD); anti p-p65 (65 kD); anti IRF3 (47 kD); anti p-IRF3 (36 kD); anti ABCF1 (110 kD); anti GAPDH (36 kD); anti histone H3 (15 kD); Dimerized-IRF3 (73 kD); IRF3 (36 kD) B) Whole-cell lysates were separated using native PAGE gel electrophoresis, and the analysis focused on examining the dimerization of IRF3, a transcription factor. Expression levels of the protein was assessed by western blotting analysis. Fold change calculations, as specified in the materials and methods section, were employed to quantify changes in the data. The bar graphs displayed in the figures represent the mean values along with standard deviations. The data presented here is representative of three separate experiments.

    Techniques Used: Phospho-proteomics, Western Blot, Clear Native PAGE, Nucleic Acid Electrophoresis, Expressing

    ABCF1 Parallels OAS1a Expression and Controls 2-5A Activity A) The immunoprecipitates were immunoblotted with anti-ABCF1 and anti-OAS1a antibodies. B) ABCF1 was over-expressed (Over Exp.) in BMDMs, an equal amount of whole cell lysates was immunoprecipitated with anti-ABCF1 antibody and the immunoprecipitates were detected with anti-ABCF1 and anti-OAS1a antibodies using western blots. C) Protein levels of OAS1a, ABCE1 and RNase L were analyzed from whole cell lysates from Abcf1 siRNA-treated BMDMs in presence or absence of Poly(I:C). Expression levels of the protein was assessed by western blotting analysis. D) Increased pyrophosphate production (a readout of 2-5A activity) was measured in scrambled and Abcf1 siRNA treated BMDMs in presence and absence of recombinant OAS1. E) Total RNA was extracted from Abcf1 siRNA treated BMDMs in presence or absence of Poly(I:C) and was run on a Agilent 2100 Bioanalyzer. 28S and 18S RNA have been shown and RIN score was calculated. Bars indicate the mean ±standard deviation. The data is representative of 3 separate experiments. The expression of ABCF1 follows a pattern that parallels the expression of OAS1a, and it also exerts control over the activity of 2-5A. This suggests a regulatory relationship where ABCF1’s expression correlates with OAS1a expression and influences the activity of 2-5A.
    Figure Legend Snippet: ABCF1 Parallels OAS1a Expression and Controls 2-5A Activity A) The immunoprecipitates were immunoblotted with anti-ABCF1 and anti-OAS1a antibodies. B) ABCF1 was over-expressed (Over Exp.) in BMDMs, an equal amount of whole cell lysates was immunoprecipitated with anti-ABCF1 antibody and the immunoprecipitates were detected with anti-ABCF1 and anti-OAS1a antibodies using western blots. C) Protein levels of OAS1a, ABCE1 and RNase L were analyzed from whole cell lysates from Abcf1 siRNA-treated BMDMs in presence or absence of Poly(I:C). Expression levels of the protein was assessed by western blotting analysis. D) Increased pyrophosphate production (a readout of 2-5A activity) was measured in scrambled and Abcf1 siRNA treated BMDMs in presence and absence of recombinant OAS1. E) Total RNA was extracted from Abcf1 siRNA treated BMDMs in presence or absence of Poly(I:C) and was run on a Agilent 2100 Bioanalyzer. 28S and 18S RNA have been shown and RIN score was calculated. Bars indicate the mean ±standard deviation. The data is representative of 3 separate experiments. The expression of ABCF1 follows a pattern that parallels the expression of OAS1a, and it also exerts control over the activity of 2-5A. This suggests a regulatory relationship where ABCF1’s expression correlates with OAS1a expression and influences the activity of 2-5A.

    Techniques Used: Expressing, Activity Assay, Immunoprecipitation, Western Blot, Recombinant, Standard Deviation, Control



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    <t>ABCF1</t> promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.
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    ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.

    Article Snippet: Specifically, knockdown of the ABCF1 gene was accomplished using Mouse Abcf1 siRNA obtained from Santa Cruz Biotechnology (catalog number sc-140760), consistently resulting in a reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Activity Assay, Staining

    ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected out of three ABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the PE-αCD8 antibody and then stained with fluorescein by heat shock. Data is representative of two separate experiments.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected out of three ABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the PE-αCD8 antibody and then stained with fluorescein by heat shock. Data is representative of two separate experiments.

    Article Snippet: Specifically, knockdown of the ABCF1 gene was accomplished using Mouse Abcf1 siRNA obtained from Santa Cruz Biotechnology (catalog number sc-140760), consistently resulting in a reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Activity Assay, Staining

    ABCF1 +/- mice produce fewer IFN γ positive CD8+ T lymphocytes after infection with VSV. ABCF1+/- splenocytes showed fewer IFNγ positive CD8+ T lymphocytes. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 +/- mice produce fewer IFN γ positive CD8+ T lymphocytes after infection with VSV. ABCF1+/- splenocytes showed fewer IFNγ positive CD8+ T lymphocytes. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Article Snippet: Specifically, knockdown of the ABCF1 gene was accomplished using Mouse Abcf1 siRNA obtained from Santa Cruz Biotechnology (catalog number sc-140760), consistently resulting in a reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Infection

    ABCF1+/- CTLs were as efficient as ABCF1 +/+ at killing of chromium. loaded VSV specific target lymphocytes. CTL activity was measured by the release of 51 Cr into the supernatant. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1+/- CTLs were as efficient as ABCF1 +/+ at killing of chromium. loaded VSV specific target lymphocytes. CTL activity was measured by the release of 51 Cr into the supernatant. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Article Snippet: Specifically, knockdown of the ABCF1 gene was accomplished using Mouse Abcf1 siRNA obtained from Santa Cruz Biotechnology (catalog number sc-140760), consistently resulting in a reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Activity Assay

    ABCF1 is essential for the production of ISG (Interferon-Stimulated Gene) specific cytokines expression of INF- α and β after Poly(I:C) stimulation. A bar graph illustrating the fold change in the levels of INF-α and β cytokines detected in the cell culture supernatants. These findings provide insights into the impact of Abcf1 -specific siRNA treatment, both with and without Poly(I:C), on the secretion of cytokines and chemokines as well as the activation of key signaling pathways and transcription factors within BMDMs. Expression levels of the protein was assessed by western blotting analysis.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 is essential for the production of ISG (Interferon-Stimulated Gene) specific cytokines expression of INF- α and β after Poly(I:C) stimulation. A bar graph illustrating the fold change in the levels of INF-α and β cytokines detected in the cell culture supernatants. These findings provide insights into the impact of Abcf1 -specific siRNA treatment, both with and without Poly(I:C), on the secretion of cytokines and chemokines as well as the activation of key signaling pathways and transcription factors within BMDMs. Expression levels of the protein was assessed by western blotting analysis.

    Article Snippet: Specifically, knockdown of the ABCF1 gene was accomplished using Mouse Abcf1 siRNA obtained from Santa Cruz Biotechnology (catalog number sc-140760), consistently resulting in a reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Expressing, Cell Culture, Activation Assay, Protein-Protein interactions, Western Blot

    ABCF1 plays a role in regulating the phosphorylation levels of NF- κ B p65 and IRF3. A) Cytoplasmic and nuclear fractions obtained from BMDMs under different conditions were subjected to western blot analysis to assess the levels of transcription factors associated with Poly(I:C) stimulation confirming our hypothesis; Western Blot band sizes are as follows: anti- p65 (65 kD); anti p-p65 (65 kD); anti IRF3 (47 kD); anti p-IRF3 (36 kD); anti ABCF1 (110 kD); anti GAPDH (36 kD); anti histone H3 (15 kD); Dimerized-IRF3 (73 kD); IRF3 (36 kD) B) Whole-cell lysates were separated using native PAGE gel electrophoresis, and the analysis focused on examining the dimerization of IRF3, a transcription factor. Expression levels of the protein was assessed by western blotting analysis. Fold change calculations, as specified in the materials and methods section, were employed to quantify changes in the data. The bar graphs displayed in the figures represent the mean values along with standard deviations. The data presented here is representative of three separate experiments.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 plays a role in regulating the phosphorylation levels of NF- κ B p65 and IRF3. A) Cytoplasmic and nuclear fractions obtained from BMDMs under different conditions were subjected to western blot analysis to assess the levels of transcription factors associated with Poly(I:C) stimulation confirming our hypothesis; Western Blot band sizes are as follows: anti- p65 (65 kD); anti p-p65 (65 kD); anti IRF3 (47 kD); anti p-IRF3 (36 kD); anti ABCF1 (110 kD); anti GAPDH (36 kD); anti histone H3 (15 kD); Dimerized-IRF3 (73 kD); IRF3 (36 kD) B) Whole-cell lysates were separated using native PAGE gel electrophoresis, and the analysis focused on examining the dimerization of IRF3, a transcription factor. Expression levels of the protein was assessed by western blotting analysis. Fold change calculations, as specified in the materials and methods section, were employed to quantify changes in the data. The bar graphs displayed in the figures represent the mean values along with standard deviations. The data presented here is representative of three separate experiments.

    Article Snippet: Specifically, knockdown of the ABCF1 gene was accomplished using Mouse Abcf1 siRNA obtained from Santa Cruz Biotechnology (catalog number sc-140760), consistently resulting in a reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Phospho-proteomics, Western Blot, Clear Native PAGE, Nucleic Acid Electrophoresis, Expressing

    ABCF1 Parallels OAS1a Expression and Controls 2-5A Activity A) The immunoprecipitates were immunoblotted with anti-ABCF1 and anti-OAS1a antibodies. B) ABCF1 was over-expressed (Over Exp.) in BMDMs, an equal amount of whole cell lysates was immunoprecipitated with anti-ABCF1 antibody and the immunoprecipitates were detected with anti-ABCF1 and anti-OAS1a antibodies using western blots. C) Protein levels of OAS1a, ABCE1 and RNase L were analyzed from whole cell lysates from Abcf1 siRNA-treated BMDMs in presence or absence of Poly(I:C). Expression levels of the protein was assessed by western blotting analysis. D) Increased pyrophosphate production (a readout of 2-5A activity) was measured in scrambled and Abcf1 siRNA treated BMDMs in presence and absence of recombinant OAS1. E) Total RNA was extracted from Abcf1 siRNA treated BMDMs in presence or absence of Poly(I:C) and was run on a Agilent 2100 Bioanalyzer. 28S and 18S RNA have been shown and RIN score was calculated. Bars indicate the mean ±standard deviation. The data is representative of 3 separate experiments. The expression of ABCF1 follows a pattern that parallels the expression of OAS1a, and it also exerts control over the activity of 2-5A. This suggests a regulatory relationship where ABCF1’s expression correlates with OAS1a expression and influences the activity of 2-5A.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 Parallels OAS1a Expression and Controls 2-5A Activity A) The immunoprecipitates were immunoblotted with anti-ABCF1 and anti-OAS1a antibodies. B) ABCF1 was over-expressed (Over Exp.) in BMDMs, an equal amount of whole cell lysates was immunoprecipitated with anti-ABCF1 antibody and the immunoprecipitates were detected with anti-ABCF1 and anti-OAS1a antibodies using western blots. C) Protein levels of OAS1a, ABCE1 and RNase L were analyzed from whole cell lysates from Abcf1 siRNA-treated BMDMs in presence or absence of Poly(I:C). Expression levels of the protein was assessed by western blotting analysis. D) Increased pyrophosphate production (a readout of 2-5A activity) was measured in scrambled and Abcf1 siRNA treated BMDMs in presence and absence of recombinant OAS1. E) Total RNA was extracted from Abcf1 siRNA treated BMDMs in presence or absence of Poly(I:C) and was run on a Agilent 2100 Bioanalyzer. 28S and 18S RNA have been shown and RIN score was calculated. Bars indicate the mean ±standard deviation. The data is representative of 3 separate experiments. The expression of ABCF1 follows a pattern that parallels the expression of OAS1a, and it also exerts control over the activity of 2-5A. This suggests a regulatory relationship where ABCF1’s expression correlates with OAS1a expression and influences the activity of 2-5A.

    Article Snippet: Specifically, knockdown of the ABCF1 gene was accomplished using Mouse Abcf1 siRNA obtained from Santa Cruz Biotechnology (catalog number sc-140760), consistently resulting in a reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Expressing, Activity Assay, Immunoprecipitation, Western Blot, Recombinant, Standard Deviation, Control

    ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected from threeABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the αnti-CD8 antibody and αnti-CD4 antibody. We depict the staining of two ABCF1+/- and one wild-type littermate controls. Data is representative of two separate experiments.

    Article Snippet: Specifically, knockdown of the Abcf1 gene utilized Mouse Abcf1 siRNA from Santa Cruz Biotechnology (catalog number sc-140760), resulting in a consistent reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Activity Assay, Staining

    ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected out of three ABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the PE-αCD8 antibody and then stained with fluorescein by heat shock. Data is representative of two separate experiments.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 promoter activity in CD8+ T cells from the thymus and the spleen. Spleens and thymi were dissected out of three ABCF1+/- (top panels) and three of their wild-type littermate controls (bottom panels). Cells were labelled with the PE-αCD8 antibody and then stained with fluorescein by heat shock. Data is representative of two separate experiments.

    Article Snippet: Specifically, knockdown of the Abcf1 gene utilized Mouse Abcf1 siRNA from Santa Cruz Biotechnology (catalog number sc-140760), resulting in a consistent reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Activity Assay, Staining

    ABCF1 +/- mice produce fewer IFN γ positive CD8+ T lymphocytes after infection with VSV. ABCF1+/- splenocytes showed fewer IFNγ positive CD8+ T lymphocytes. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 +/- mice produce fewer IFN γ positive CD8+ T lymphocytes after infection with VSV. ABCF1+/- splenocytes showed fewer IFNγ positive CD8+ T lymphocytes. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Article Snippet: Specifically, knockdown of the Abcf1 gene utilized Mouse Abcf1 siRNA from Santa Cruz Biotechnology (catalog number sc-140760), resulting in a consistent reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Infection

    ABCF1+/- CTLs were as efficient as ABCF1 +/+ at killing of chromium. loaded VSV specific target lymphocytes. CTL activity was measured by the release of 51 Cr into the supernatant. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1+/- CTLs were as efficient as ABCF1 +/+ at killing of chromium. loaded VSV specific target lymphocytes. CTL activity was measured by the release of 51 Cr into the supernatant. Figure shown represents the results of one experiment, which was later repeated three times with similar results.

    Article Snippet: Specifically, knockdown of the Abcf1 gene utilized Mouse Abcf1 siRNA from Santa Cruz Biotechnology (catalog number sc-140760), resulting in a consistent reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Activity Assay

    ABCF1 is essential for the production of ISG (Interferon-Stimulated Gene) specific cytokines expression of INF- α and β after Poly(I:C) stimulation. A bar graph illustrating the fold change in the levels of INF-α and β cytokines detected in the cell culture supernatants. These findings provide insights into the impact of Abcf1 -specific siRNA treatment, both with and without Poly(I:C), on the secretion of cytokines and chemokines as well as the activation of key signaling pathways and transcription factors within BMDMs. Expression levels of the protein was assessed by western blotting analysis.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 is essential for the production of ISG (Interferon-Stimulated Gene) specific cytokines expression of INF- α and β after Poly(I:C) stimulation. A bar graph illustrating the fold change in the levels of INF-α and β cytokines detected in the cell culture supernatants. These findings provide insights into the impact of Abcf1 -specific siRNA treatment, both with and without Poly(I:C), on the secretion of cytokines and chemokines as well as the activation of key signaling pathways and transcription factors within BMDMs. Expression levels of the protein was assessed by western blotting analysis.

    Article Snippet: Specifically, knockdown of the Abcf1 gene utilized Mouse Abcf1 siRNA from Santa Cruz Biotechnology (catalog number sc-140760), resulting in a consistent reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Expressing, Cell Culture, Activation Assay, Protein-Protein interactions, Western Blot

    ABCF1 plays a role in regulating the phosphorylation levels of NF- κ B p65 and IRF3. A) Cytoplasmic and nuclear fractions obtained from BMDMs under different conditions were subjected to western blot analysis to assess the levels of transcription factors associated with Poly(I:C) stimulation confirming our hypothesis; Western Blot band sizes are as follows: anti- p65 (65 kD); anti p-p65 (65 kD); anti IRF3 (47 kD); anti p-IRF3 (36 kD); anti ABCF1 (110 kD); anti GAPDH (36 kD); anti histone H3 (15 kD); Dimerized-IRF3 (73 kD); IRF3 (36 kD) B) Whole-cell lysates were separated using native PAGE gel electrophoresis, and the analysis focused on examining the dimerization of IRF3, a transcription factor. Expression levels of the protein was assessed by western blotting analysis. Fold change calculations, as specified in the materials and methods section, were employed to quantify changes in the data. The bar graphs displayed in the figures represent the mean values along with standard deviations. The data presented here is representative of three separate experiments.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 plays a role in regulating the phosphorylation levels of NF- κ B p65 and IRF3. A) Cytoplasmic and nuclear fractions obtained from BMDMs under different conditions were subjected to western blot analysis to assess the levels of transcription factors associated with Poly(I:C) stimulation confirming our hypothesis; Western Blot band sizes are as follows: anti- p65 (65 kD); anti p-p65 (65 kD); anti IRF3 (47 kD); anti p-IRF3 (36 kD); anti ABCF1 (110 kD); anti GAPDH (36 kD); anti histone H3 (15 kD); Dimerized-IRF3 (73 kD); IRF3 (36 kD) B) Whole-cell lysates were separated using native PAGE gel electrophoresis, and the analysis focused on examining the dimerization of IRF3, a transcription factor. Expression levels of the protein was assessed by western blotting analysis. Fold change calculations, as specified in the materials and methods section, were employed to quantify changes in the data. The bar graphs displayed in the figures represent the mean values along with standard deviations. The data presented here is representative of three separate experiments.

    Article Snippet: Specifically, knockdown of the Abcf1 gene utilized Mouse Abcf1 siRNA from Santa Cruz Biotechnology (catalog number sc-140760), resulting in a consistent reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Phospho-proteomics, Western Blot, Clear Native PAGE, Nucleic Acid Electrophoresis, Expressing

    ABCF1 Parallels OAS1a Expression and Controls 2-5A Activity A) The immunoprecipitates were immunoblotted with anti-ABCF1 and anti-OAS1a antibodies. B) ABCF1 was over-expressed (Over Exp.) in BMDMs, an equal amount of whole cell lysates was immunoprecipitated with anti-ABCF1 antibody and the immunoprecipitates were detected with anti-ABCF1 and anti-OAS1a antibodies using western blots. C) Protein levels of OAS1a, ABCE1 and RNase L were analyzed from whole cell lysates from Abcf1 siRNA-treated BMDMs in presence or absence of Poly(I:C). Expression levels of the protein was assessed by western blotting analysis. D) Increased pyrophosphate production (a readout of 2-5A activity) was measured in scrambled and Abcf1 siRNA treated BMDMs in presence and absence of recombinant OAS1. E) Total RNA was extracted from Abcf1 siRNA treated BMDMs in presence or absence of Poly(I:C) and was run on a Agilent 2100 Bioanalyzer. 28S and 18S RNA have been shown and RIN score was calculated. Bars indicate the mean ±standard deviation. The data is representative of 3 separate experiments. The expression of ABCF1 follows a pattern that parallels the expression of OAS1a, and it also exerts control over the activity of 2-5A. This suggests a regulatory relationship where ABCF1’s expression correlates with OAS1a expression and influences the activity of 2-5A.

    Journal: bioRxiv

    Article Title: An ATP-Binding Cassette Transporter Gene Links Innate and Adaptive Immune Responses

    doi: 10.1101/2023.12.31.573785

    Figure Lengend Snippet: ABCF1 Parallels OAS1a Expression and Controls 2-5A Activity A) The immunoprecipitates were immunoblotted with anti-ABCF1 and anti-OAS1a antibodies. B) ABCF1 was over-expressed (Over Exp.) in BMDMs, an equal amount of whole cell lysates was immunoprecipitated with anti-ABCF1 antibody and the immunoprecipitates were detected with anti-ABCF1 and anti-OAS1a antibodies using western blots. C) Protein levels of OAS1a, ABCE1 and RNase L were analyzed from whole cell lysates from Abcf1 siRNA-treated BMDMs in presence or absence of Poly(I:C). Expression levels of the protein was assessed by western blotting analysis. D) Increased pyrophosphate production (a readout of 2-5A activity) was measured in scrambled and Abcf1 siRNA treated BMDMs in presence and absence of recombinant OAS1. E) Total RNA was extracted from Abcf1 siRNA treated BMDMs in presence or absence of Poly(I:C) and was run on a Agilent 2100 Bioanalyzer. 28S and 18S RNA have been shown and RIN score was calculated. Bars indicate the mean ±standard deviation. The data is representative of 3 separate experiments. The expression of ABCF1 follows a pattern that parallels the expression of OAS1a, and it also exerts control over the activity of 2-5A. This suggests a regulatory relationship where ABCF1’s expression correlates with OAS1a expression and influences the activity of 2-5A.

    Article Snippet: Specifically, knockdown of the Abcf1 gene utilized Mouse Abcf1 siRNA from Santa Cruz Biotechnology (catalog number sc-140760), resulting in a consistent reduction of 79-81% compared to control samples treated with scrambled siRNA.

    Techniques: Expressing, Activity Assay, Immunoprecipitation, Western Blot, Recombinant, Standard Deviation, Control