K-Ras4B Mutant Protein: G12V (human recombinant with 6xHis-tag)

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Study of G12V K-Ras4B exchange activity with different GEFs
Identification of G12V K-Ras4B exchange factors (GEFs)
Positive control for GEF studies
Biochemical characterization of G12V K-Ras4B protein interactions
Western blot standard

The biological activity of G12V K-Ras4B can be determined from the ability of the SOS1 exchange domain (SOS1-ExD) to catalyze the exchange of GDP for GTP onto mutant K-Ras4B. A standard biological assay for monitoring the biological activity of G12V KRas4B is an exchange assay utilizing the 2X Exchange Buffer from the RhoGEF exchange assay kit (Cat.# BK100) and the human SOS1 GEF domain (Cat.# CS-SOS1).

1. Dilute SOS1-ExD protein (Cat.# CS-SOS1) to 1 ?M (0.06 mg/ml) with Dilution Buffer.
2. Dilute G12V K-Ras4B to 50 ?M (1.1 mg/ml) with Dilution Buffer.
3. Dissolve lyophilized 2X Exchange Buffer in 5 ml Milli-Q water and keep at room temperature.
4. Set up the plate reader for kinetic fluorescence measurements (Excitation wavelength at 360 nm and emission wavelength at 440 nm) with readings every 30 seconds for 30 minutes.
5. Add the following components together and mix well by gentle pipetting:
Association/Exchange reaction mix / 96 well black plate
2x Exchange Buffer / 50 ?l
dH₂O / 26 ?l
50 ?M G12V K-Ras4B / 4 ?l
6. Pipette 20 ?l of 1 ?M SOS1-ExD protein or Dilution Buffer into their respective wells and immediately pipette up and down twice and begin reading the fluorescence.
7. Once the readings are complete and the plate reader file has been saved, the exchange rate can be calculated by reducing the data to Vmax with the software that accompanies the plate reader.

Legend: GDP-Bodipy-FL-loaded N-Ras protein was added to duplicate wells of a 96-well half area plate containing diluted Exchange Buffer and mixed well. To initiate the dissociation exchange reaction, 1 mM GTP plus Ras-GRF GEF protein (rows A to G), or 1 mM GTP only in Dilution Buffer (row H), was added to the wells, mixed, and fluorescence measurements were obtained using a Tecan SpectraFluor Plus Spectrophotometer. Ras-GRF was diluted 2 fold from row A through row G starting at 4 ?M. Note the rapid drop in fluorescence in rows A, B and C which is indicative of fast exchange, and the nearly flat line of row H which indicates no exchange is occurring in the absence of Ras-GRF.