| Code | CSB-RA013714MA1HU |
| Size | US$210 |
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| Application | Recommended Dilution |
|---|---|
| IF | 1:20-1:200 |
| FC | 1:20-1:200 |
MET, also known as hepatocyte growth factor receptor (HGFR), serves as a critical receptor tyrosine kinase that orchestrates cellular responses to its ligand HGF/scatter factor. This signaling axis drives fundamental biological processes including cell proliferation, motility, and morphogenesis, while its dysregulation through amplification, mutation, or overexpression has been implicated across numerous cancer types. Understanding MET biology remains essential for researchers investigating oncogenic signaling, metastatic progression, and therapeutic resistance mechanisms.
This recombinant monoclonal antibody, clone 33A12, offers the reproducibility and consistency that demanding research applications require. Generated through recombinant expression technology, every lot derives from the same defined sequence, eliminating the batch-to-batch variability that can compromise longitudinal studies or multi-site collaborations. The mouse IgG2a isotype antibody has been affinity-purified to ensure high specificity for human MET protein.
Validation studies demonstrate reliable performance across multiple detection platforms. Immunofluorescence analysis of SH-SY5Y neuroblastoma cells reveals clear cellular staining patterns when counterstained with DAPI, with effective results achieved at dilutions ranging from 1:20 to 1:200. Flow cytometry applications have been validated using HeLa cells, where surface staining produces distinct positive population shifts compared to isotype controls, confirming the antibody's utility for detecting membrane-localized MET. The antibody is additionally suitable for ELISA-based detection methods.
For researchers exploring receptor tyrosine kinase signaling, cancer biology, or epigenetic regulation pathways, this antibody provides a dependable tool for characterizing MET expression and localization. The validated performance in both fixed-cell immunofluorescence and live-cell flow cytometry offers flexibility for diverse experimental workflows examining this therapeutically relevant target.
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