Intracellular ifn γ 4s b3

Manufactured by BD

The Intracellular IFN-γ (4S.B3) is a laboratory equipment product. It is used to detect and measure the presence of interferon-gamma (IFN-γ) within cells. This product provides a tool for researchers to analyze cellular immune responses.

Automatically generated - may contain errors

Lab products found in correlation

48 well plate, by BD (2 mentions) Mabs cd3 ucht1, by BD (2 mentions) Soluble cd28 cd28.2, by BD (2 mentions) T cell isolation kit, by STEMCELL (2 mentions) Leukocyte activation cocktail, by BD (2 mentions) Ccr7 3d12, by BD (1 mentions)

Close spelling variants of this product

IFN-γ (4S.B3) Intracellular IFN-γ IFN-γ

2 protocols using intracellular ifn γ 4s b3

Allogeneic T Cell Activation by Dendritic and Natural Killer Cells

Check if the same lab product or an alternative is used in the 5 most similar protocols

Syngeneic immature DC and NK cells or nicDC and nicNK cells (1×10⁵ DC: 2×10⁵ NK/well) exposed to Alum or TLR agonists for 8 hrs were subsequently co-cultured in 48-well plates (Falcon, Franklin Lakes, NJ) at a 1:10 ratio with CFSE labeled allogeneic naïve T cells isolated from PBMC using T cell isolation kit (StemCell Technologies, Vancouver, Canada). On day 5, the proliferating cells were transferred into new plates and rested in IL-2-containing medium (5 ng/ml) up to 10 days. The cells were subsequently collected and stained with CD4 (L200), CD8 (SK1), and CCR7 (3D12) (primary co-cultures). The remaining T cells were transferred to plates pre-coated with 10 μg/ml mAbs CD3 (UCHT1) and 2 μg/ml soluble CD28 (CD28.2) (BD Biosciences, San Diego, CA) for 72 hrs. The T cells were then stimulated for 4–6 hrs with leukocyte activation cocktail (BD Biosciences) containing Brefeldin A before staining with CD4 (L200), CD8 (SK1), CCR7 (3D12), and intracellular IFN-γ (4S.B3) (BD Biosciences, San Diego, CA) (secondary co-cultures). The frequency and amount of IFN-γ were further analyzed using Flow Cytometry and ELISA.

Nouri-Shirazi M., Tamjidi S., Nourishirazi E, & Guinet E. (2018). Combination of TLR8 and TLR4 agonists reduces the degrading effects of nicotine on DC-NK mediated effector T cell generation. International immunopharmacology, 61, 54-63.

+ Open protocol

+ Expand

Allogeneic T Cell Activation by DCs and NK Cells

Check if the same lab product or an alternative is used in the 5 most similar protocols

Syngeneic immature DCs and NK cells (1×10⁵ DC: 2×10⁵ NK/well) exposed to Alum or TLR agonists for 8hrs were subsequently co-cultured in 48-well plates (Falcon, Franklin Lakes, NJ) at a 1:10 ratio with CFSE labeled allogeneic naïve T cells isolated from PBMCs using T cell isolation kit (StemCell Technologies, Vancouver, Canada). The purity of the enriched T cells was >95% based upon prevalence of CD3+CD56- phenotypes. On day 5, the proliferating cells were transferred into new plates and rested in IL-2-containing medium (5ng/ml) up to 10 days. The cells were subsequently collected and stained with CD4 (L200), CD8 (SK1), and CCR7 (3D12) (primary co-cultures). The remaining T cells were transferred to plates pre-coated with 10μg/ml mAbs CD3 (UCHT1) and 2μg/ml soluble CD28 (CD28.2) (BD Biosciences, San Diego, CA) for 72hrs. The T cells were then stimulated for 4–6hrs with leukocyte activation cocktail (BD Biosciences) containing Brefeldin A before staining with CD4 (L200), CD8 (SK1), CCR7 (3D12), and intracellular IFN-γ (4S.B3) (BD Biosciences, San Diego, CA) (secondary co-cultures). The frequency and amount of IFN-γ were further analyzed using Flow Cytometry and ELISA.

Nouri-Shirazi M., Tamjidi S., Nourishirazi E, & Guinet E. (2017). TLR8 combined withTLR3 or TLR4 agonists enhances DC-NK driven effector Tc1 cells. Immunology letters, 193, 58-66.

+ Open protocol

+ Expand

About PubCompare

Our mission is to provide scientists with the largest repository of trustworthy protocols and intelligent analytical tools, thereby offering them extensive information to design robust protocols aimed at minimizing the risk of failures.

We believe that the most crucial aspect is to grant scientists access to a wide range of reliable sources and new useful tools that surpass human capabilities.

However, we trust in allowing scientists to determine how to construct their own protocols based on this information, as they are the experts in their field.

Ready to get started?

Revolutionizing how scientists
search and build protocols!