A 20 μg sample of full length bovine cardiac myosin protein (lane A) and the corresponding S1 myosin (lane B) were separated by electrophoresis using a 4-20% SDS-PAGE gel and stained with Coomassie Blue.The arrow indicates the myosin heavy chain (approx. 200 kDa), arrow heads indicate the RLC(approx. 20 kDa) and two ELC isoforms (approx. 25 and 21 kDa).Protein quantitation was performed using the Precision Red™ Protein Assay Reagent (Cat.# ADV02). Mark12 molecular weight markers are from Invitrogen.

Biological Activity Assay

The biological activity of bovine cardiac myosin S1 fragment can be determined from its rate of F-actin activated ATP hydrolysis.The assay is constructed by first polymerizing actin to form Factin,then the cardiac Tropomyosin/Troponin complex (TT complex) is mixed with the actin filaments in a stoichiometric amount. This creates coated filaments which are analogous to the thin filaments of muscle fibers. Myosin is added in substoichiometric amounts and the reaction initiated with ATP and calcium. Stringentquality control ensures that in the absence of calcium the TT complex completely inhibits myosin ATPase. On addition of 10 uMcalcium myosin ATPase will be restored. Calcium binds to Troponin C which dissociates from F-actin allowing myosin to bind.

Reagents

1. Cardiac TT complex (1 x 1 mg, # TT05)

2. Cardiac Myosin S1 (0.25 mg), # MYS03)

3. Cardiac Actin (1 mg, Cat. # AD99-A)

4. ATPase Assay Biochem Kit (Cat. # BK051)

5. 100 mM ATP in 50 mM Tris-HCl pH 7.5 (100ul)

6. 1 M Dithiothreitol in water (100 ul).

7. PM12 Reaction buffer (12 mM Pipes-KOH, pH 7.0, 2 mM MgCl₂).8. 500 mM EGTA-Na pH 8.0.

Equipment

1. Spectrophotometer capable of measuring absorbance at 360 nm (+/- 5 nm bandwidth). We recommend a Spectra-Max M2 (Molecular Devices), filter based machines are not suitable.

2. Half area 96 well microtiter plate (Corning Cat.# 3696 or 3697)

3. Multi-channel pipette

Method

The following major steps are recognized:

Step 1. Assemble required reagents and compounds. (30min).

Step 2. Prepare F-actin polymer stock. (1h).

Step 3. Prepare Thin Filament stock (1.5h)

Step 4. Prepare Motor Mix and plate reader. (15min).

Step 5. Pipette Motor Mix into wells and start reaction/plate reader. (10min).

F-actin polymer stock

1. Resuspend AD99 with 2.5ml of Buffer to 0.4mg/ml (measure protein concentration for better reproducibility), in buffer 5mM Pipes-KOH pH 7.0, 500uM ATP, 500uM DTT.

2. Place at RT for 10min to solubilize the actin.

3. Then add 2.0 mM MgCl2 and 2.0 mM EGTA and incubate at RT for 20 min to polymerize. (shelf life 1h at RT).

Thin Filament stock

1. Resuspend 1 x 1mg TT05 on ice with ice cold water to 5 mg/ml. (200ul per vial for 1mg vial).

2. Mix the following to make 1.2 ml of actin/TT05 (TF):

1000 μl of F-actin stock

200 μl of TT05

3. Incubate at RT for 20min.

4. Centrifuge at 100K xg 4°C for 1h.