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Join us! · InformexUSA 2012 · New Orleans, Louisiana · February 14-17, 2012 · Booth 2514

S-Nitrosylated Protein Detection Kit

Cayman Chemical Item Number 10006518

SNO Detection

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Description

Nitric oxide (NO) is produced by three distinct isoforms of nitric oxide synthase and functions as a key signaling molecule in physiology and pathophysiology.1,2 NO transduces its effects by reacting either directly with heme and non-heme centers of proteins or indirectly via further oxidation to various reactive nitrogen species (RNS).3,4Nitrosylation refers to the binding of an NO group to a transition metal, as typified in the activation of soluble guanylate cyclase, or to a thiol (SH) group of protein cysteine residues resulting in the formation of an S-NO moiety. This latter reaction, termed S-nitrosylation, is mediated by reactive nitrogen species of higher oxidation states of NO, such as NO2 and N2O3.5,6 S-Nitrosylation is a reversible, and seemingly specific, post-translational modification that regulates the activity of a large number of targets, including metabolic, structural, cytoskeletal, and signaling proteins.7 Cayman’s S-Nitrosylated Protein Detection Assay employs a modification of the Jaffrey et al. 'Biotin-switch' method to allow for the direct visualization of S-nitrosylated proteins in whole cells or tissues, as well as by western blot analysis.8,9 Using this method, free SH groups are first blocked and any S-NO bonds present in the sample are then cleaved. Biotinylation of the newly formed SH groups provides the basis for visualization using streptavidin-based colorimetric or fluorescence detection.

1 Alderton, W.K., Cooper, C.E., and Knowles, R.G. Nitric oxide synthases: Structure, function, and inhibition. Biochem J 357 593-615 (2001).

2 Bredt, D.S. Endogenous nitric oxide synthesis: Biological functions and pathophysiology. Free Radic Res 31 577-596 (1999).

3 Beckman, J.S., and Koppenol, W.H. Nitric oxide, superoxide, and peroxynitrite: The good, the bad, and the ugly. Am J Physiol 271 C1424-C1437 (1996).

4 Kelm, M. Nitric oxide metabolism and breakdown. Biochim Biophys Acta 1411 273-289 (1999).

5 Mannick, J.B., and Schonhoff, C.M. Nitrosylation: The next phosphorylation? Arch Biochem Biophys 408 1-6 (2002).

6 Martínez-Ruiz, A., and Lamas, S. S-nitrosylation: A potential new paradigm in signal transduction. Cardiovasc Res 62 43-52 (2004).

7 Stamler, J.S., Lamas, S., and Fang, F.C. Nitrosylation: The prototypic redox-based signaling mechanism. Cell 106 675-683 (2001).

8 Ckless, K., Reynaert, N.L., Taatjes, D.J., et al. In situ detection and visualization of S-nitrosylated proteins following chemical derivatization: Identification of Ran GTPase as a target for S-nitrosylation. Nitric Oxide 11 216-227 (2004).

9 Jaffrey, S.R., Erdjument-Bromage, H., Ferris, C.D., et al. Protein S-nitrosylation: A physiological signal for neuronal nitric oxide. Nat Cell Biol 3(2) 193-197 (2001 Feb 2).

Synonyms
  • SNO Detection
Stability 1 year
Storage -20°C
Shipping Wet ice in continental US; may vary elsewhere

Background Reading

Alderton, W.K., Cooper, C.E., and Knowles, R.G. Nitric oxide synthases: Structure, function, and inhibition. Biochem J 357 593-615 (2001).

Martínez-Ruiz, A., and Lamas, S. S-nitrosylation: A potential new paradigm in signal transduction. Cardiovasc Res 62 43-52 (2004).

Bredt, D.S. Endogenous nitric oxide synthesis: Biological functions and pathophysiology. Free Radic Res 31 577-596 (1999).

Stamler, J.S., Lamas, S., and Fang, F.C. Nitrosylation: The prototypic redox-based signaling mechanism. Cell 106 675-683 (2001).

Mannick, J.B., and Schonhoff, C.M. Nitrosylation: The next phosphorylation? Arch Biochem Biophys 408 1-6 (2002).

Jaffrey, S.R., Erdjument-Bromage, H., Ferris, C.D., et al. Protein S-nitrosylation: A physiological signal for neuronal nitric oxide. Nat Cell Biol 3(2) 193-197 (2001 Feb 2).

Beckman, J.S., and Koppenol, W.H. Nitric oxide, superoxide, and peroxynitrite: The good, the bad, and the ugly. Am J Physiol 271 C1424-C1437 (1996).

Kelm, M. Nitric oxide metabolism and breakdown. Biochim Biophys Acta 1411 273-289 (1999).

Ckless, K., Reynaert, N.L., Taatjes, D.J., et al. In situ detection and visualization of S-nitrosylated proteins following chemical derivatization: Identification of Ran GTPase as a target for S-nitrosylation. Nitric Oxide 11 216-227 (2004).

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10006518-1EA
S-Nitrosylation Wash Buffer (10X) 1 ea
S-Nitrosylation Buffer A 1 ea
S-Nitrosylation Buffer B (5X) 1 ea
S-Nitrosylation Reducing Reagent 3 × 1 ea
S-Nitrosylation Labeling Reagent 3 × 1 ea
S-Nitrosylation Detection Reagent I (HRP) 1 ea
S-Nitrosylation Detection Reagent II (Fluorescein) 1 ea
S-Nitrosylation Blocking Reagent 3 × 1 ea
Size Price Quantity Subtotal
1 ea $265.00 $0.00
Bulk Contact
Cart Total $0.00

This product is also available to buy in bulk quantities.

Please contact our Sales Department for a quote or to purchase.

Pricing updated 2012-02-12. Prices are subject to change without notice.

To ask for assistance with one of our products please contact a Technical Support Scientist.

Warning This product is not for human or veterinary use.

You may be eligible to receive a free sample S-Nitrosylated Protein Detection Kit under the Cayman Challenge program.

Let Cayman analyze your samples for you. See EIA Service for details and availability.

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Batch-specific Information

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FAQs

In the S-Nitrosylated Protein Detection Kit is there any point early in the procedure where the protocol can be stopped overnight?

It is possible to stop the procedure at either of the two acetone protein precipitations (step 7 or step 13 under the Sample Preparation section). At either point you can leave the precipitates at -20°C overnight.

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If no dark room is available, how important is the performance of steps 1-12 under indirect light in the S-Nitrosylated Protein Detection Kit protocol?

If you can turn off some of the overhead lights in the lab and avoid using a lamp directly on the bench, that will help.

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In the S-Nitrosylated Protein Detection Kit there is not a protocol for use of a whole tissue homogenate. There is a protocol for isolated tissue cell pellet, but nothing starting from whole tissues. Is there a way to use this kit?

For a soft tissue where cells can be isolated one may: isolate, wash and pellet the cells, pick up at step 3 to lyse cells and block free thiols. For solid tissue samples, homogenize at 0.1 g/ml buffer in 20 mM Tris pH 8.0, or P-SNO Cell Lysis Buffer (Buffer A). Centrifuge here to eliminate major debris (1000xg, 10 minutes). Repeat the homogenization with the ice-cold supernatant and sonicate if needed (to ensure complete lysis, check for remaining intact cells by microscopy). Quantify the protein concentration and dilute to 2 mg/ml if needed. Treat the sample going forward as a cell lysate by adding the reconstituted blocking reagent (1 mL stock solution) to the current sample volume in 1:9 proportion.

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For the S-Nitrosylated Protein Detection Assay Kit is it is okay to have β-mercaptoethanol in the Laemmli buffer?

Yes, it is okay to have β-mercaptoethanol in the Laemmli buffer in the S-Nitrosylated Protein Detection Assay Kit. The Biotin will not dissociate from the protein.

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What sample types can be used with the S-Nitrosylation Protein Detection Kit?

The protocol in the S-Nitrosylated Protein Detection Kit (cat. 10006518) refers to use of a cell pellet which can be obtained from cultured cells, or blood cells. Alternatively, the assay can be used with purified protein. If using a purified protein, begin by resuspending the protein sample and incubating at 2mg/mL in Buffer A containing Blocking Reagent; this will keep the blocking reagent in excess. At this point, free thiols on the protein are blocked and you can continue with the acetone precipitations in step 6. For gel analysis, load only 1-5 µg of protein per lane to avoid overloading the protein.

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