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cd38  (Proteintech)


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    Structured Review

    Proteintech cd38
    (A) Volcano plot of significant upregulated and downregulated genes in GF tissue, using p < 0.05 and a threshold of 1.2-fold change in expression as a cutoff for analysis. <t>CD38</t> (p < 0.001, FC = 1.55), RSAD2 (p < 0.001, FC = 0.08), GABRR1 (p < 0.001, FC = 0.08), FN1 (p < 0.001, FC = 0.54), IFI6 (p < 0.001, FC = 0.37), IRAK1BP1 (p < 0.001, FC = 1.74), RGS1 (p < 0.001, FC = 3.22) are labeled in bold. (B) Graphical reconstruction of immune activation Ingenuity Pathway Analysis result, showing differentially expressed genes in our tissue related to this pathway. Panel made with BioRender. (C) Representative immunohistochemical images of the PFCII-III in control and GF animals. CD38 + (red), DAPI + (blue), and Iba1 + (white) staining (left, scale bar 200µm), a middle inset of the leftmost image (middle, scale bar 50µm), and a single channel (CD38) of this inset (right, scale bar 50µm) for each group n=3/animals per group. Data supported by Extended Data Table 6-1.
    Cd38, supplied by Proteintech, used in various techniques. Bioz Stars score: 94/100, based on 34 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/cd38/product/Proteintech
    Average 94 stars, based on 34 article reviews
    cd38 - by Bioz Stars, 2026-05
    94/100 stars

    Images

    1) Product Images from "Germ-free piglets display variable neuroinflammatory-like perturbations in prefrontal cortical microglia"

    Article Title: Germ-free piglets display variable neuroinflammatory-like perturbations in prefrontal cortical microglia

    Journal: bioRxiv

    doi: 10.64898/2026.03.22.713463

    (A) Volcano plot of significant upregulated and downregulated genes in GF tissue, using p < 0.05 and a threshold of 1.2-fold change in expression as a cutoff for analysis. CD38 (p < 0.001, FC = 1.55), RSAD2 (p < 0.001, FC = 0.08), GABRR1 (p < 0.001, FC = 0.08), FN1 (p < 0.001, FC = 0.54), IFI6 (p < 0.001, FC = 0.37), IRAK1BP1 (p < 0.001, FC = 1.74), RGS1 (p < 0.001, FC = 3.22) are labeled in bold. (B) Graphical reconstruction of immune activation Ingenuity Pathway Analysis result, showing differentially expressed genes in our tissue related to this pathway. Panel made with BioRender. (C) Representative immunohistochemical images of the PFCII-III in control and GF animals. CD38 + (red), DAPI + (blue), and Iba1 + (white) staining (left, scale bar 200µm), a middle inset of the leftmost image (middle, scale bar 50µm), and a single channel (CD38) of this inset (right, scale bar 50µm) for each group n=3/animals per group. Data supported by Extended Data Table 6-1.
    Figure Legend Snippet: (A) Volcano plot of significant upregulated and downregulated genes in GF tissue, using p < 0.05 and a threshold of 1.2-fold change in expression as a cutoff for analysis. CD38 (p < 0.001, FC = 1.55), RSAD2 (p < 0.001, FC = 0.08), GABRR1 (p < 0.001, FC = 0.08), FN1 (p < 0.001, FC = 0.54), IFI6 (p < 0.001, FC = 0.37), IRAK1BP1 (p < 0.001, FC = 1.74), RGS1 (p < 0.001, FC = 3.22) are labeled in bold. (B) Graphical reconstruction of immune activation Ingenuity Pathway Analysis result, showing differentially expressed genes in our tissue related to this pathway. Panel made with BioRender. (C) Representative immunohistochemical images of the PFCII-III in control and GF animals. CD38 + (red), DAPI + (blue), and Iba1 + (white) staining (left, scale bar 200µm), a middle inset of the leftmost image (middle, scale bar 50µm), and a single channel (CD38) of this inset (right, scale bar 50µm) for each group n=3/animals per group. Data supported by Extended Data Table 6-1.

    Techniques Used: Expressing, Labeling, Activation Assay, Immunohistochemical staining, Control, Staining



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    (A) Volcano plot of significant upregulated and downregulated genes in GF tissue, using p < 0.05 and a threshold of 1.2-fold change in expression as a cutoff for analysis. <t>CD38</t> (p < 0.001, FC = 1.55), RSAD2 (p < 0.001, FC = 0.08), GABRR1 (p < 0.001, FC = 0.08), FN1 (p < 0.001, FC = 0.54), IFI6 (p < 0.001, FC = 0.37), IRAK1BP1 (p < 0.001, FC = 1.74), RGS1 (p < 0.001, FC = 3.22) are labeled in bold. (B) Graphical reconstruction of immune activation Ingenuity Pathway Analysis result, showing differentially expressed genes in our tissue related to this pathway. Panel made with BioRender. (C) Representative immunohistochemical images of the PFCII-III in control and GF animals. CD38 + (red), DAPI + (blue), and Iba1 + (white) staining (left, scale bar 200µm), a middle inset of the leftmost image (middle, scale bar 50µm), and a single channel (CD38) of this inset (right, scale bar 50µm) for each group n=3/animals per group. Data supported by Extended Data Table 6-1.
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    MV-Blina infected cells secrete target-binding secBlina, which initiates ALL cell kill more <t>efficiently</t> <t>than</t> <t>CD19/CD3-bsTE</t> (A) Vero cells secrete secBlina. secBlina was harvested from the supernatant of infected Vero cells, followed by purification and concentration. Eluate (2 μg protein) was detected via His-tag by Western Blot in comparison to the commercial CD19/CD3-bsTE (1.8 μg). (B) Purified and concentrated secBlina binds specifically to target cells. Binding to target cells was confirmed by flow cytometry using CD3 − CD19 + REH, CD3 + CD19 - Jurkat, and CD3 − CD19 - K562 cell lines incubated with secBlina. Binding of secBlina to target cells was detected by flow cytometry via a His-tag antibody. (C) secBlina strongly binds to REH target cells. The REH cell line was first incubated with 1 μg secBlina. Increasing concentrations of CD19/CD3-bsTE were then added to displace cell-bound secBlina. Cell-bound secBlina was detected via an HA tag antibody by flow cytometry. (D) T cells in human PBMCs are activated by secBlina. Pooled PBMCs were stimulated with an (E) T cells are activated by secBlina during co-culture of PBMCs with REH cells. Pooled PBMCs were co-cultured with REH cells in a 1:1-ratio for 24 h while being treated with secBlina or the CD19/CD3-bsTE. Activated CD2 + CD69 + T cells were detected by flow cytometry. (F) MV-Blina infected leukemia cells produce and secrete secBlina. REH and Jurkat cells are shown 72 h post MV infection or Opti-MEM control. secBlina was detected by His-tag IF staining. Scale bars 50 μm. (G) secBlina effectively induces REH target cell kill compared to CD19/CD3-bsTE, whereas K562 control cells are unaffected. Target (T) cells REH (left panels) and negative control cells K562 (right panels) were incubated with secBlina (green) or CD19/CD3-bsTE (blue) for 24 h at indicated concentrations in the presence of PBMCs (effector; E) at different E:T ratios. Specific cell kill was determined by flow cytometry. Results in A, B, C, and F are shown as representatives of three independent experiments. Data are shown as mean ± SD of n = 3 (D, E) or n = 5 (G) independent experiments. Statistical analysis was performed using two-way ANOVA with Dunnett’s correction. ns, not significant; ∗, p < 0.05; ∗∗, p < 0.01; ∗∗∗, p < 0.001; and ∗∗∗∗, p < 0.0001.
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    Image Search Results


    (A) Volcano plot of significant upregulated and downregulated genes in GF tissue, using p < 0.05 and a threshold of 1.2-fold change in expression as a cutoff for analysis. CD38 (p < 0.001, FC = 1.55), RSAD2 (p < 0.001, FC = 0.08), GABRR1 (p < 0.001, FC = 0.08), FN1 (p < 0.001, FC = 0.54), IFI6 (p < 0.001, FC = 0.37), IRAK1BP1 (p < 0.001, FC = 1.74), RGS1 (p < 0.001, FC = 3.22) are labeled in bold. (B) Graphical reconstruction of immune activation Ingenuity Pathway Analysis result, showing differentially expressed genes in our tissue related to this pathway. Panel made with BioRender. (C) Representative immunohistochemical images of the PFCII-III in control and GF animals. CD38 + (red), DAPI + (blue), and Iba1 + (white) staining (left, scale bar 200µm), a middle inset of the leftmost image (middle, scale bar 50µm), and a single channel (CD38) of this inset (right, scale bar 50µm) for each group n=3/animals per group. Data supported by Extended Data Table 6-1.

    Journal: bioRxiv

    Article Title: Germ-free piglets display variable neuroinflammatory-like perturbations in prefrontal cortical microglia

    doi: 10.64898/2026.03.22.713463

    Figure Lengend Snippet: (A) Volcano plot of significant upregulated and downregulated genes in GF tissue, using p < 0.05 and a threshold of 1.2-fold change in expression as a cutoff for analysis. CD38 (p < 0.001, FC = 1.55), RSAD2 (p < 0.001, FC = 0.08), GABRR1 (p < 0.001, FC = 0.08), FN1 (p < 0.001, FC = 0.54), IFI6 (p < 0.001, FC = 0.37), IRAK1BP1 (p < 0.001, FC = 1.74), RGS1 (p < 0.001, FC = 3.22) are labeled in bold. (B) Graphical reconstruction of immune activation Ingenuity Pathway Analysis result, showing differentially expressed genes in our tissue related to this pathway. Panel made with BioRender. (C) Representative immunohistochemical images of the PFCII-III in control and GF animals. CD38 + (red), DAPI + (blue), and Iba1 + (white) staining (left, scale bar 200µm), a middle inset of the leftmost image (middle, scale bar 50µm), and a single channel (CD38) of this inset (right, scale bar 50µm) for each group n=3/animals per group. Data supported by Extended Data Table 6-1.

    Article Snippet: Sections were blocked with 5% donkey serum, 1% BSA in PBST for 1 hour, and then stained with Iba1 (Wako, catalog #NC9288364), Ki67 (Abcam, catalog #ab16667), and CD38 (Proteintech, catalog #60006-1-Ig) overnight at 4°C.

    Techniques: Expressing, Labeling, Activation Assay, Immunohistochemical staining, Control, Staining

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    Journal: Molecular Therapy Oncology

    Article Title: A measles virus encoding a CD19/CD3 bispecific T cell engager shows enhanced preclinical anti-BCP-ALL efficacy without significant toxicity

    doi: 10.1016/j.omton.2026.201127

    Figure Lengend Snippet: MV-Blina infected cells secrete target-binding secBlina, which initiates ALL cell kill more efficiently than CD19/CD3-bsTE (A) Vero cells secrete secBlina. secBlina was harvested from the supernatant of infected Vero cells, followed by purification and concentration. Eluate (2 μg protein) was detected via His-tag by Western Blot in comparison to the commercial CD19/CD3-bsTE (1.8 μg). (B) Purified and concentrated secBlina binds specifically to target cells. Binding to target cells was confirmed by flow cytometry using CD3 − CD19 + REH, CD3 + CD19 - Jurkat, and CD3 − CD19 - K562 cell lines incubated with secBlina. Binding of secBlina to target cells was detected by flow cytometry via a His-tag antibody. (C) secBlina strongly binds to REH target cells. The REH cell line was first incubated with 1 μg secBlina. Increasing concentrations of CD19/CD3-bsTE were then added to displace cell-bound secBlina. Cell-bound secBlina was detected via an HA tag antibody by flow cytometry. (D) T cells in human PBMCs are activated by secBlina. Pooled PBMCs were stimulated with an (E) T cells are activated by secBlina during co-culture of PBMCs with REH cells. Pooled PBMCs were co-cultured with REH cells in a 1:1-ratio for 24 h while being treated with secBlina or the CD19/CD3-bsTE. Activated CD2 + CD69 + T cells were detected by flow cytometry. (F) MV-Blina infected leukemia cells produce and secrete secBlina. REH and Jurkat cells are shown 72 h post MV infection or Opti-MEM control. secBlina was detected by His-tag IF staining. Scale bars 50 μm. (G) secBlina effectively induces REH target cell kill compared to CD19/CD3-bsTE, whereas K562 control cells are unaffected. Target (T) cells REH (left panels) and negative control cells K562 (right panels) were incubated with secBlina (green) or CD19/CD3-bsTE (blue) for 24 h at indicated concentrations in the presence of PBMCs (effector; E) at different E:T ratios. Specific cell kill was determined by flow cytometry. Results in A, B, C, and F are shown as representatives of three independent experiments. Data are shown as mean ± SD of n = 3 (D, E) or n = 5 (G) independent experiments. Statistical analysis was performed using two-way ANOVA with Dunnett’s correction. ns, not significant; ∗, p < 0.05; ∗∗, p < 0.01; ∗∗∗, p < 0.001; and ∗∗∗∗, p < 0.0001.

    Article Snippet: For the displacement assay, 1 × 10 6 REH cells were incubated with 1 μg secBlina for 30 min, followed by increasing concentrations of a research-grade analog of the CD19/CD3-bsTE blinatumomab (BPS Bioscience) for an additional 30 min, all at 4°C. secBlina bound to target cells was detected using rabbit anti-HA antibody (clone EPR22819-101, 1:600, ab256483, Abcam) for 30 min at 4°C, followed by a goat-anti-rabbit IgG (H&L) AF488 (1:2000, ab150077, Abcam).

    Techniques: Infection, Binding Assay, Purification, Concentration Assay, Western Blot, Comparison, Flow Cytometry, Incubation, Co-Culture Assay, Cell Culture, Control, Staining, Negative Control