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Nombre del producto
Anti-N1-Phosphohistidine (1-pHis) Antibody, clone SC50-3, clone SC50-3, from rabbit
biological source
rabbit
antibody form
purified antibody
antibody product type
primary antibodies
clone
SC50-3, monoclonal
species reactivity
human, E. coli
species reactivity (predicted by homology)
all
technique(s)
dot blot: suitable
western blot: suitable
isotype
IgG
shipped in
wet ice
target post-translational modification
phosphorylation (N1-pHis)
Quality Level
1 of 4
Este artículo | ZRB1352 | ZRB1351 | MABS1352 |
|---|---|---|---|
| clone SC50-3, monoclonal | clone SC56-2, monoclonal, recombinant monoclonal | clone SC39-6, monoclonal, recombinant monoclonal | clone SC56-2, monoclonal |
| biological source rabbit | biological source rabbit (recombinant) | biological source rabbit (recombinant) | biological source rabbit |
| antibody form purified antibody | antibody form purified antibody | antibody form purified antibody | antibody form purified antibody |
| species reactivity human, E. coli | species reactivity human | species reactivity human | species reactivity human, E. coli |
| isotype IgG | isotype IgG | isotype IgG | isotype IgG |
| shipped in wet ice | shipped in ambient | shipped in ambient | shipped in wet ice |
Analysis Note
Western Blotting Analysis: 0.24 µg/mL of this antibody detected recombinant human NME1 (NM23-H1) with N1-phosphohistidine (1-pHis) in a 5 µg aliquot of autophosphorylation reaction.
Application
Western Blotting Analysis: Clone SC50-3 hybridoma culture supernatant was employed for Western blotting analysis of heat-sensitive histidine N1-phosphorylation (1-pHis) of exogenously expressed NM23-H1/NME1 fusion proteins in lysates from transformed E. coli and HEK293 transfectants (Fuhs, S.R., et al. (2015). Cell. 162(1):198-210).
Note: DO NOT HEAT SAMPLES prior to phosphohistidine detection. Histidine phosphorylation is heat and acid labile. To generate negative control for specificity test, an aliquot of sample can be heated at 95ºC for 10-15 minutes to reverse histidine phosphorylation. Alternatively, an aliquot of sample can be incubated under acidified pH at 37ºC for 15 minutes to reduce histidine phosphorylation. Acidify each 100 µL sample with 25 µL of 1 M HCl before the incubation, then neutralize with 25 µL of 1 M NaOH prior to phosphohistidine detection.
Biochem/physiol Actions
General description
Immunogen
Other Notes
Physical form
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Clase de almacenamiento
12 - Non Combustible Liquids
wgk
WGK 1
flash_point_f
Not applicable
flash_point_c
Not applicable
Certificados de análisis (COA)
Busque Certificados de análisis (COA) introduciendo el número de lote del producto. Los números de lote se encuentran en la etiqueta del producto después de las palabras «Lot» o «Batch»
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A major focus of breast cancer research is to understand the mechanisms responsible for disease progression and drug resistance. Toward that end, it has been found that approximately two thirds of all human breast carcinomas overexpress the Estrogen Receptor α (ERα) protein and it remains the primary pharmacological target for endocrine therapy1,2. The normal cellular function of ERα is as a transcription factor that mediates a wide variety of physiological processes, many of which are dependent upon phosphorylation of the receptor at specific amino acid residues3,4. Indeed, ERα is known to be phosphorylated at a multitude of different sites, yet how these all correlate to disease remains unclear5. Here, we interrogated multiple sites of ERα for phosphorylation status by screening an extensive panel of different breast cancer patient samples and other non-breast cancer tissue microarray (TMA) slide samples to determine their relevance to disease.
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