DCP-Bio1 is dimedone based and contains a biotin tag making it compatible with several techniques and forms of analysis.
Features:
-Contains cleavable biotin tag
-Stable, reproducible binding to cysteine sulfenic acid (-SOH) at pH 6.0 - 8.0
-Great for In vitro and In vivo applications
-Compatible with WB, ELISA, and Affinity Isolation
Redox-sensitive cysteine residues in proteins may serve as important components of oxidative signaling or sensors of oxidative stress. Cysteine sulfenic acid modification is an emerging area of interest for those studying biological signal transduction within the cell.
Cysteine sulfenic acid formation in proteins results from the oxidative modification of susceptible cysteine residues by mild oxidizing agents such as hydrogen peroxide, alkyl hydroperoxides, and peroxynitrite. These sulfenic acid modified proteins can be identified by their ability to form adducts with dimedone, but this reagent provides no spectral or affinity tag to such adduct to allow for later analysis. DCP-Bio1 can be used to effectively detect the formation of cysteine sulfenic acid in the redox regulation of proteins, and with the presence of a biotin label, DCP-Bio1 is compatible with several techniques and forms of analysis post-labeling.
Product Type: | Small Molecule |
Name: | DCP-Bio1; 3-(2,4-dioxocyclohexyl)propyl 5-((3aR,6S,6aS)-hexahydro-2-oxo-1H-thieno[3,4-d]imidazol-6-yl)pentanoate |
Chemical Formula: | C19H28N2O5S |
Source: | synthetic |
Molecular Weight: | 396.5 g/mol |
Format: | solid |
Purity: | >98% pure, see Poole, et al., 2007 |
Solubility: | At least 500 mM in DMSO, at least 5 mg/ml in acetonitrile |
Stability: | stable > 6 months at -20 degC |
Spectral Information: | No visible absorbance; NMR data, etc. in Poole et al., 2007 |
Storage: | room temperature for short term, -20 degC for long term.Stock solution in DMSO can be added to cell lysis buffer, preferrably keeping final [DMSO] < 2% for labeling proteins. Can be dissolved in acetonitrile to prepare aliquots and redry. |
产品说明书:DCP-Bio1
From the laboratories of Leslie B. Poole, PhD and S. Bruce King, PhD, Wake Forest School of Medicine.
Poole, L.B., Klomsiri, C., Knaggs, S.A., Furdui, C.M., Nelson, K.J., Thomas, M.J., Fetrow, J.S., Daniel, L.W. & King, S.B. Fluorescent and affinity-based tools to detect cysteine sulfenic acid formation in proteins. Bioconjug Chem 18, 2004-17 (2007). PMC2526167
Klomsiri, C., Nelson, K.J., Bechtold, E., Soito, L., Johnson, L.C., Lowther, W.T., Ryu, S.E., King, S.B., Furdui, C.M. & Poole, L.B. Use of dimedone-based chemical probes for sulfenic acid detection: evaluation of conditions affecting probe incorporation into redox-sensitive proteins. Methods Enzymol 473, 77-94 (2010)
Nelson, K.J., Klomsiri, C., Codreanu, S.G., Soito, L., Liebler, D.C., Rogers, L.C., Daniel, L.W. & Poole, L.B. Use of dimedone-based chemical probes for sulfenic acid detection; methods to visualize and identify labeled proteins. Methods Enzymol 473, 95-115 (2010).
DCP-Bio1 Application References
Oshikawa, J., Urao, N., Kim, H.W., Kaplan, N., Razvi, M., McKinney, R., Poole, L.B., Fukai, T. & Ushio-Fukai, M. Extracellular SOD-derived H2O2 promotes VEGF signaling in caveolae/lipid rafts and post-ischemic angiogenesis in mice. PLoS One 5, e10189 (2010). PMC2858087
Kaplan, N., Urao, N., Furuta, E., Kim, S.J., Razvi, M., Nakamura, Y., McKinney, R.D., Poole, L.B., Fukai, T. & Ushio-Fukai, M. Localized cysteine sulfenic acid formation by vascular endothelial growth factor:role in endothelial cell migration and angiogenesis. Free Radic Res 45, 1124-35 (2011).
Wani, R., Qian, J., Yin, L., Bechtold, E., King, S.B., Poole, L.B., Paek, E., Tsang, A.W. & Furdui, C.M. Isoform-specific regulation of Akt by PDGF-induced reactive oxygen species. Proc Natl Acad Sci U S A 108, 10550-5 (2011).
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