Human Phospho-Src (Y419) DuoSet IC ELISA

Standard Curve

The Human Phospho-Src (Y419) DuoSet® IC ELISA specifically recognizes human Src phosphorylated at Y419 as determined by peptide competition.

A lysate prepared from MDA-MB-468 human breast cancer cells treated with 50 mM sodium pervanadate for 20 minutes was analyzed with this ELISA. The Human Phospho-Src (Y419) Detection Antibody was either untreated (no peptide) or preincubated with a phospho-peptide containing the phospho-Src Y419 phosphorylation site, a phospho-peptide containing the Ret Y905 phosphorylation site, a phospho-peptide containing the Tie-2 Y1100 phosphorylation site, or a phospho-peptide containing the PP2A Y307 phosphorylation site. Peptides were used at 40 ng/mL. Only the phospho-peptide containing the Src Y419 phosphorylation site blocked the signal, indicating that the ELISA is specific for human Src phosphorylation.

Amounts of human phosphorylated Src, as quantified by the Human Phospho-Src (Y419) DuoSet® IC ELISA, are consistent with the relative amounts of phosphorylated Src determined by qualitative Western Blot analysis.

Quantification of phosphorylated Scr (Y419) in pervabadate-treated human MDA-MB-468 cells. Lysates prepared from MDA-MB-468 human breast cancer cells treated with 50 mM sodium pervanadate for the indicated times were quantified with this DuoSet® IC ELISA. The same lysates were also immunoblotted (inset) with either Human Phospho-Src (Y419) Polyclonal Antibody (Catalog # AF2685) or Human/Mouse/Rat Src Polyclonal Antibody (Catalog # AF3389). The DuoSet® IC ELISA results are consistent with the relative amounts of phosphorylated Src family members detected by Western Blot. The immunoblot with anti-Src antibody indicated that total levels of human Src remained constant during incubation with sodium pervanadate.