YILIMART - Anti-Ly49C/I-APC, mouse, REAL296, 100 t

Clone REAL296 is an antibody fragment derived from the full Ly-49C/I antibody molecule. It displays no binding to Fc receptors. The recombinantly engineered antibody fragments are multimerized to form the REAlease Complex to bind markers with high avidity.

Clone REAL296 recognizes the mouse lymphocyte antigen 49c (Ly-49C), a type II transmembrane protein which is also known as killer cell lectin-like receptor 3 (Klra3). Clone REAL296 reacts with Ly-49C of BALB, B6, NZB, C57BL, and Ly-49I of B6 mice strains. Ly-49 family members are both activating and inhibitory receptors and are mainly receptors for MHC class I molecules. Ly-49C is a cell surface molecule expressed on a subpopulation of murine natural killer (NK) cells and NK1.1 T cells that are involved in the specific rejection of H-2d or H-2f (hemopoietic histocompatibility determinant 2) bone marrow cell grafts. It transduces a negative signal to NK cells upon recognition of class I antigens. The particular allele of Ly-49C, i.e., C57BL versus BALB, determines to a large extent which class I antigen (H-2Kb for B6, Kb and H-2d for BALB/c or BALB.B) sends negative signals to Ly-49C

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NK cells. Clone REAL296 blocks the binding of Ly-49C to MHC class I antigens of the b, d, k, and s haplotypes. The epitope recognized by REAL296 may be masked on NK cells due to interactions with MHC class I molecules.

The REAlease Kits consist of the respective fluorochrome-conjugated REAlease Complexes and the REAlease Support Kit for removal of the REAlease Complexes and optional relabeling with different fluorochrome-conjugated REAlease Complexes.

Alternative names

Klra3, Klra9

Technical specifications

Antigen: Ly-49C/I
Clone: REAL296
Isotype control: REAL Control
Alternative names of antigen: Klra3, Klra9
Distribution of antigen: NK cells
Product format: Reagents are supplied in buffer containing stabilizer and 0.05% sodium azide.
Storage: Store protected from light at 2–8 °C. Do not freeze.
Available conjugates: APC, PE

Figure 1

Splenocytes from C56BL/6 mice were stained with REAlease Anti-Ly-49C/I-APC (B) or with the corresponding REAL Control (A). REAlease Anti-Ly-49C/I-APC was released using the REAlease Release Reagent (C). To show epitope accessibility after REAlease Complex release, the cells were washed with the REAlease Stop Reagent and restained with REAlease Anti-Ly-49C/I-APC (D). Cells were labeled with CD49b antibodies in addition and analyzed by flow cytometry using the MACSQuant

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Analyzer. Cell debris and dead cells were excluded from the analysis based on scatter signals and propidium iodide (PI) fluorescence.

A:	B:

C:	D:

Figure 2

Splenocytes from C56BL/6 mice were stained with REAlease Anti-Ly-49C/I Complexes or with the corresponding REAL Control (left images) as well as with CD49b antibodies and analyzed by flow cytometry using the MACSQuant

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Analyzer. Cell debris and dead cells were excluded from the analysis based on scatter signals and propidium iodide (PI) fluorescence.

Selected references
1. Stoneman, E. R. et al. (1995) Cloning and characterization of 5E6(Ly-49C), a receptor molecule expressed on a subset of murine natural killer cells. J. Exp. Med. 182(2): 305-313
2. Brennan, J. et al. (1996) Heterogeneity among Ly-49C natural killer (NK) cells: characterization of highly related receptors with differing functions and expression patterns. J. Exp. Med. 184(6): 2085-2090
3. Yu, Y. Y. et al. (1996) The role of Ly49A and 5E6(Ly49C) molecules in hybrid resistance mediated by murine natural killer cells against normal T cell blasts. Immunity 4(1): 67-76

Anti-Ly49C/I-APC, mouse, REAL296, 100 t

For research use only

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Alternative names

Technical specifications

Figure 1

Figure 2

Selected references

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