Other Products

Human IFN-γ Matched Antibody Pair for ELISpot

Catalogue #: SL10024A

$405.00

In stock

Human IFN-γ Matched Antibody Pair for ELISpot5 × 96 wells


Pre-titered capture antibody and biotinylated detection antibody matched pair for the development of enzyme-linked immunospot (ELISpot) assays for the quantitation of single cells releasing human interferon-γ (IFN-γ)


This product is not available for online ordering.  Please enquire via email. 

Description

Details

INTENDED USE

Pre-titered capture antibody and biotinylated detection antibody matched pair for the development of enzyme-linked immunospot (ELISpot) assays for the quantitation of single cells releasing human IFN-γ.  

A recommended assay protocol is provided. The dilutions of capture antibody and detection antibody is determined according to this protocol. The researcher can optimize the dilutions if it is necessary. 

For laboratory research use only. Not for use in diagnostic procedures.

INTRODUCTION 

Interferon gamma (IFN-γ) is a multifunctional protein first observed to have antiviral activity in cultures of Sindbis virus-infected human leukocytes stimulated by PHA. (1)) The biochemistry and biological activities of the interferons have been extensively reviewed. Produced by both CD4+ and CD8+ T lymphocytes and natural killer (NK) cells, INF-γ is now known to be both an inhibitor of viral replication and a regulator of numerous immunological functions. IFN-γ influences the class of antibody produced by B cells up-regulates classes I and II MHC complex antigens and increases the efficiency of macrophage-mediated killing of intracellular parasites. (2, 3) Most of the activities attributed to IFN-γ are believed to be mediated by IFN-γ-induced proteins. The appearance of such proteins is a consequence of IFN-γ binding to a specific receptor that is distinct from the receptor for IFN-a and β. (4) Human IFN-γ is reported to be active only on human and non-human primate cells. (5) The biochemistry and biological activities of the interferons have been extensively reviewed.  (2-9) 

Human IFN-γ is a 143 amino acid residue glycoprotein with MW of 20 or 25 kDa that demonstrates little sequence homology to IFN-α and b. (10-13) Naturally occurring IFN-γ is found as either of two molecular-weight-species, differing in degree of glycosylation. The 25 kDa species is glycosylated at both potential N-linked glycosylation sites on the molecule (Asn 25 and 97), while the 20 kDa species is glycosylated only at Asn97. (17, 18) In neither case glycosylation is required for biological activity. (13, 16) Two allelic variants of IFN-g have been described differing by the presence of an Arg or Gln at position 137. (10, 16) 

Although the cDNA encoding for IFN-γ predicts a protein of 146 amino acid residues, the form secreted by mammalian cells shows a truncation of three amino acid residues from the N-terminus and the conversion of the fourth residue from glutamic acid to pyroglutamate. (11) The secreted form of IFN-γ has no potential for the formation of disulfide bonds. (13) Human IFN-γ apparently exists as a head-to-tail dimmer in solution with the C-terminus of one monomer aligned with the N-terminus of the other monomer. (18, 19)  

IFN-γ possesses a variety of functions. Produced by CD8+, NK and TH2 T helper cells, IFN-γ has documented antiviral, antiprotozoal and immunomodulatory activities, (20-24) although IFN-a and IFN-β seem to have more potential antiviral activities than IFN-γ. (24) The antiprotozoal activity of IFN-γ against Toxoplasma and Chlamydia is believed to result from indoleamine 2, 3-dioxygenase activity, an enzyme induced by IFN-γ. (25) The immunomodulatory effects of IFN-γ are extensive and diverse.   In monocyte/ macrophages, IFN-γ increases expression of class 1 MHC antigens; increases the production of IL-1, platelet-activating factor, H2O2, and pterin; protects monocytes against LAK cell-mediated lysis; down-regulates IL-8 mRNA expression that is up-regulating TGF-β receptor expression and up-regulating expression of the IL-2Rγ subunit. (23, 25, 26-29) It has also been demonstrated to be chemotactic for monocytes but not neutrophils. (30) IFN-γ selectively enhances both Ig G2a secretion by LPS-stimulated B cell activation. (31, 32) IFN-γ has also been reported to induce its own expression. IFN-γ production accompanying local inflammation results in the induction of IFN-g mRNA synthesis at distant sites. This effect could be due to circulating IFN-γ or the production of IFN-γ by migrating cells (33). IFN-γ has also been shown to up-regulate ICAM-1 but not E-selectin or VCAM-1 expression on endothelial cells (34). Finally, IFN-γ has recently been implicated in the development of a cholinergic phenotype in embryonic septal neurons. In cultures of rat septal nuclei, IFN-γ induced the development of cholinergic neurons.                       

This ELISpot kit is developed to detect and visualize of single cells secreting human IFN-γ.

Additional

Additional Information

Product Specificity Human IFN-γ Matched Antibody Pair for ELISpot
Application Refer to Insert
Size 5 × 96 wells
Contact Us