CD4+CD25+ Regulatory T Cell Isolation Kit, mouse

The CD4
+
CD25
+
Regulatory T Cell Isolation Kit, mouse was developed for the isolation of CD4
+
CD25
+
regulatory T cells (Treg) from single-cell suspensions of mouse spleen and lymph nodes. The isolation is performed in a fast two-step procedure.

Data and images for
CD4
+
CD25
+
Regulatory T Cell Isolation Kit
, mouse

Figures

Figure 1

CD4
+
CD25
+
regulatory T cells were isolated from mouse spleen cell suspension by using the CD4
+
CD25
+
Regulatory T Cell Isolation Kit, an LD and two MS Columns, a MidiMACS™ Separator and a MiniMACS™ Separator. The cells were fluorescently stained with CD25-PE and CD4‑FITC (A) or Anti-FoxP3-APC (B) and analyzed by flow cytometry using the MACSQuant
®
Analyzer. Cell debris and dead cells were excluded from analysis based on scatter signals and propidium iodide fluorescence.
A:
B:
Before separation
View details

Figure 1

CD4
+
CD25
+
regulatory T cells were isolated from mouse spleen cell suspension by using the CD4
+
CD25
+
Regulatory T Cell Isolation Kit, an LD and two MS Columns, a MidiMACS™ Separator and a MiniMACS™ Separator. The cells were fluorescently stained with CD25-PE and CD4‑FITC (A) or Anti-FoxP3-APC (B) and analyzed by flow cytometry using the MACSQuant
®
Analyzer. Cell debris and dead cells were excluded from analysis based on scatter signals and propidium iodide fluorescence.
View details

Figure 1

CD4
+
CD25
+
regulatory T cells were isolated from mouse spleen cell suspension by using the CD4
+
CD25
+
Regulatory T Cell Isolation Kit, an LD and two MS Columns, a MidiMACS™ Separator and a MiniMACS™ Separator. The cells were fluorescently stained with CD25-PE and CD4‑FITC (A) or Anti-FoxP3-APC (B) and analyzed by flow cytometry using the MACSQuant
®
Analyzer. Cell debris and dead cells were excluded from analysis based on scatter signals and propidium iodide fluorescence.
CD4+CD25- T cells
View details

Figure 1

CD4
+
CD25
+
regulatory T cells were isolated from mouse spleen cell suspension by using the CD4
+
CD25
+
Regulatory T Cell Isolation Kit, an LD and two MS Columns, a MidiMACS™ Separator and a MiniMACS™ Separator. The cells were fluorescently stained with CD25-PE and CD4‑FITC (A) or Anti-FoxP3-APC (B) and analyzed by flow cytometry using the MACSQuant
®
Analyzer. Cell debris and dead cells were excluded from analysis based on scatter signals and propidium iodide fluorescence.
View details

Figure 1

CD4
+
CD25
+
regulatory T cells were isolated from mouse spleen cell suspension by using the CD4
+
CD25
+
Regulatory T Cell Isolation Kit, an LD and two MS Columns, a MidiMACS™ Separator and a MiniMACS™ Separator. The cells were fluorescently stained with CD25-PE and CD4‑FITC (A) or Anti-FoxP3-APC (B) and analyzed by flow cytometry using the MACSQuant
®
Analyzer. Cell debris and dead cells were excluded from analysis based on scatter signals and propidium iodide fluorescence.
Isolated CD4+CD25+ regulatory T cells
View details

Figure 1

CD4
+
CD25
+
regulatory T cells were isolated from mouse spleen cell suspension by using the CD4
+
CD25
+
Regulatory T Cell Isolation Kit, an LD and two MS Columns, a MidiMACS™ Separator and a MiniMACS™ Separator. The cells were fluorescently stained with CD25-PE and CD4‑FITC (A) or Anti-FoxP3-APC (B) and analyzed by flow cytometry using the MACSQuant
®
Analyzer. Cell debris and dead cells were excluded from analysis based on scatter signals and propidium iodide fluorescence.
View details

Figure 1

CD4
+
CD25
+
regulatory T cells were isolated from mouse spleen cell suspension by using the CD4
+
CD25
+
Regulatory T Cell Isolation Kit, an LD and two MS Columns, a MidiMACS™ Separator and a MiniMACS™ Separator. The cells were fluorescently stained with CD25-PE and CD4‑FITC (A) or Anti-FoxP3-APC (B) and analyzed by flow cytometry using the MACSQuant
®
Analyzer. Cell debris and dead cells were excluded from analysis based on scatter signals and propidium iodide fluorescence.

Figure 2

View details
Working scheme of the CD4
+
CD25
+
Regulatory T Cell Isolation Kit.

Figure 2

Working scheme of the CD4
+
CD25
+
Regulatory T Cell Isolation Kit.

Specifications for
CD4
+
CD25
+
Regulatory T Cell Isolation Kit
, mouse

Overview

The CD4
+
CD25
+
Regulatory T Cell Isolation Kit, mouse was developed for the isolation of CD4
+
CD25
+
regulatory T cells (Treg) from single-cell suspensions of mouse spleen and lymph nodes. The isolation is performed in a fast two-step procedure.

Detailed product information

Background information

CD4
+
CD25
+
immunoregulatory T cells have been shown to actively suppress immune responses against autologous and foreign antigens
in vivo
and
in vitro
. CD25, the IL-2Rα chain, is also expressed on activated CD4
+
T cells, CD8
+
T cells, dendritic cells, and B cells.

Detailed separation procedure

The isolation is performed in a two-step procedure. First, non-CD4
+
are indirectly magnetically labeled with a cocktail of biotin-conjugated antibodies against CD8, CD11b, CD45R, CD49b, Ter-119 and Anti-Biotin MicroBeads. The labeled cells are subsequently depleted over a MACS
®
Column. In the second step, the flow-through fraction of pre-enriched CD4
+
T cells is labeled with CD25 MicroBeads for subsequent positive selection of CD4
+
CD25
+
regulatory T cells (Tregs). Use our optimized protocol to save 30 minutes of handling time.

Downstream applications

Regulatory T cells isolated from mouse lymph nodes with the CD4
+
CD25
+
Regulatory T Cell Isolation Kit were used in coculture experiments with dendritic cells to study priming of dendritic cells for tolerance induction
in vitro
and after adoptive transfer of primed dendritic cells
in vivo
.
1
Furthermore, they were isolated and used in various models for adoptive transfer experiments
2
, e.g. in an experimental autoimmune thyroiditis mouse model
3
, and a melanoma mouse model where they prevented tumor immunity
4
. In addition,
in vitro
suppression assays were performed with isolated regulatory T cells.
5,6

Columns

For the first magnetic separation (depletion): LD or autoMACS
®
Columns. For the second magnetic separation (positive selection): MS or autoMACS Columns.

Resources for
CD4
+
CD25
+
Regulatory T Cell Isolation Kit
, mouse

Documents and Protocols

Brochures/posters

Regulatory T cell research

Reviews for
CD4
+
CD25
+
Regulatory T Cell Isolation Kit
, mouse

CD4+CD25+ Reg T cell isolation kit, mouse

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CD4+CD25+ Regulatory T Cell Isolation Kit, mouse (130-091-041)

The general aim of my research was to test the ability of Regulatory T cells from drug treated mice to suppress the proliferation of effector T cells. I used this product in order to isolate the CD4+CD25+ regulatory T cell population from spleens and lymph nodes of control and drug-treated mice. I chose this kit because of the time and ease of use.

Treg Isolation

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CD4+CD25+ Regulatory T Cell Isolation Kit, mouse (130-091-041)

This Kit is very useful for isolating CD4+CD25+ Tregs from LN and Spleen, in order to culture Tregs, using them for RT PCR or for adoptive cell transfer experiments. I especially use it for performing in vivo Treg suppression assays, in which you transfer Tregs together with naive CD4+ T cells into immunodeficient RAG-/- mice. In this assay, the Tregs should prevent the colitogenic activity of the transferred naive CD4+ T cells.

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References for
CD4
+
CD25
+
Regulatory T Cell Isolation Kit
, mouse

Publications

  1. Fallarino, F. et al. (2003) Modulation of tryptophan catabolism by regulatory T cells. Nat Immunol 4: 1206-1212
  2. Schwarz, A. et al. (2004) Ultraviolet radiation-induced regulatory T cells not only inhibit the induction but can suppress the effector phase of contact hypersensitivity. J Immunol 172: 1036-1043
  3. Gangi, E. et al. (2005)
    IL-10-producing CD4
    +
    CD25
    +
    regulatory T cells play a critical role in granulocyte-macrophage colony-stimulating factor-induced suppression of experimental autoimmune thyroiditis.
    J Immunol 174: 7006-7013
  4. Turk, MJ. et al. (2004) Concomitant tumor immunity to a poorly immunogenic melanoma is prevented by regulatory T cells. J. Exp. Med. 200: 771-782
  5. Kashiwada, M. et al. (2006)
    Downstream of tyrosine kinases-1 and Src homology 2-containing inositol 5′-phosphatase are required for regulation of CD4
    +
    CD25
    +
    T cell development.
    J Immunol 176: 3958-3965
  6. Choileain, N. N. et al. (2006) Enhanced regulatory T cell activity is an element of the host response to injury. J Immunol 176: 225-236

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