Image of a kit SensoLyte MFP Protein Phosphatase Assay Kit Fluorimetric
Assay-kits

SensoLyte® MFP Protein Phosphatase Assay Kit Fluorimetric - 1 kit

354.00
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  • Cat.Number : AS-71104
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Protein phosphatases have received great attention as drug-screening targets. MFP is a proprietary fluorogenic substrate for most phosphatases, i.e., alkaline phosphatases, acid phosphatases, protein tyrosine phosphatases, and serine/threonine phosphatases. The phosphatase-induced hydrolysis of MFP yields an intense fluorescent product that has excitation wavelength around 470 nm, and maximum emission around 510 nm. This characteristic makes the substrate adaptable to all the fluorescence instruments. SensoLyte® MFP Protein Phosphatase Assay Kit uses MFP to quantify protein phosphatase activities. The kit can be used for characterizing kinetics of enzyme reaction and high throughput screening of protein phosphatase inhibitors. The kit contains: - MFP phosphatase substrate - Protein phosphatase inhibitor - Assay buffer - A 'mix and read' assay protocol that is compatible with HTS liquid handling instruments.

Specifications

Packaging
Kits components
  • Component A: MFP (1 vial), Ex/Em= 470 nm/510 nm upon phosphate group removal 1 mL Component B: Assay buffer: 60 mL Component C: 10X Lysis buffer: 50 mL : Component D: Triton X-100: 500 µL Component E: Stop solution: 30 mL Component F: 1 M DTT: 100 µl
Properties
Absorbance (nm)
  • 470
Emission (nm)
  • 510
Storage & stability
Storage Conditions
  • Store all kit components at -20°C. Components B, C, D, E can be stored at room temperature for convenience.
Activity
Application
Biomarker Target
Detection Method
Detection Limit
  • 5 ng/ml
Research Area
Sub-category Research Area
Usage
  • Research use
Codes
Code Nacres
  • NA.32

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Citations

SIK1 is part of a cell sodium-sensing network that regulates active sodium transport through a calcium-dependent process

Proc Natl Acad Sci U S A . 2007 Oct 15 ; 104(43) 16922 | DOI : 10.1073/pnas.0706838104

  • M. Sjöström
  • et al

Phospho-regulation of HsCdc14A by polo-like kinase 1 is essential for mitotic progression

JBC . 2020 Mar 19 ; 282 27414 | DOI : 10.1074/jbc.M703555200

  • K. Yuan
  • et al