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Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
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Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
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Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
Class B Cpg, supplied by InvivoGen, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
Alhydrogel Adjuvant 2%, supplied by InvivoGen, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Sangon Biotech cpg odn 1826
Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
Cpg Odn 1826, supplied by Sangon Biotech, used in various techniques. Bioz Stars score: 86/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
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Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
Cpg Oligodeoxynucleotide, supplied by InvivoGen, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg <t>of</t> <t>CpG-B</t> in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.
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Image Search Results


Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg of CpG-B in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.

Journal: iScience

Article Title: VPS33B regulates MHC class II antigen presentation in dendritic cells to drive CD4 T cell immunity

doi: 10.1016/j.isci.2026.116052

Figure Lengend Snippet: Impaired CD4 and CD8 T cell priming is not due to inherent T cell-intrinsic defects in mice lacking VPS33B in DCs and other myeloid cells (A) Schematic of experimental set-up for adoptive T cell transfer and protein immunization. CD45.1 + OT-I and OT-II T cells were isolated and transferred into VPS33B WT and VPS33B ΔCSF1R mice. 24 h later, mice were immunized with 50 μg of OVA and 5 μg of LPS or 10 μg of CpG-B in IFA (100 μL/mouse; hock injection). 7 days later, IgLNs were collected and subject to flow cytometry. (B) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-II and OT-I cells from immunized LNs to the right. (C) Representative flow plots gating for transferred OT-I (live, CD90.2 + , Vα2 + , CD8 + , CD45.1 + ) or transferred OT-II (live, CD90.2 + , Vα2 + , CD8 − , CD45.1 + ) T cells. Pre-gated on live, CD90.2 + , Vα2 + cells. Quantification of % CD45.1 + , Vα2 + OT-I and OT-II cells from immunized LNs to the right. Error bars shown as mean ± SEM. n = 4–5 biological replicates for one independent experiment. Statistical analysis was performed by unpaired t test. ∗ p < . 05 , ∗∗ p < 0 . 01 , ∗∗∗p < 0 . 0001 , n.s. = not significant.

Article Snippet: CpG-B , Invivogen , Cat#Tlrl-1668.

Techniques: Isolation, Injection, Flow Cytometry