| Code | CSB-RA013481A396phHU |
| Size | US$210 |
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| Application | Recommended Dilution |
|---|---|
| WB | 1:500-1:5000 |
Tau protein, encoded by the MAPT gene, serves as a critical regulator of microtubule stability in neurons and has become one of the most intensively studied targets in neurodegenerative disease research. Phosphorylation at serine 396 represents a particularly significant post-translational modification, as hyperphosphorylation at this site is closely associated with the formation of neurofibrillary tangles characteristic of Alzheimer's disease and related tauopathies. Detecting this specific phosphorylation event enables researchers to investigate tau pathology mechanisms, evaluate therapeutic interventions, and characterize disease progression at the molecular level.
This recombinant monoclonal antibody, generated against a synthetic phosphopeptide corresponding to human Phospho-MAPT at serine 396, offers the reproducibility and consistency that phospho-specific detection demands. Because recombinant production ensures a sequence-defined antibody with minimal lot-to-lot variation, researchers can confidently compare results across extended studies and between laboratories. The rabbit IgG format provides excellent signal-to-noise characteristics for sensitive phosphoprotein detection.
Validation in Western blot applications demonstrates reliable performance in HeLa whole cell lysate, detecting the expected 80 kDa band that corresponds to the predicted molecular weight of tau protein. The recommended working dilution range of 1:500 to 1:5000 provides flexibility for optimization across different experimental conditions and sample types. Additional validation for ELISA applications extends the utility of this antibody for quantitative phospho-tau measurements.
For neuroscience researchers investigating tau biology, neurodegeneration mechanisms, or screening potential therapeutic compounds targeting tau phosphorylation, this antibody delivers the specificity and consistency essential for meaningful phosphoprotein analysis in human samples.
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