Calculate enzyme activity, specific activity, and turnover number. Convert between enzyme units, katal, and specific activity measurements.
Enzyme activity is a measure of the quantity of active enzyme present, defined by the rate at which the enzyme converts substrate to product under specified conditions. The international unit (U) of enzyme activity is the amount that catalyzes the conversion of 1 micromole of substrate per minute. The SI unit, the katal (kat), represents 1 mole of substrate converted per second.
Specific activity — enzyme activity per milligram of total protein — is the key metric for tracking enzyme purification. As contaminant proteins are removed during purification, specific activity increases. A successful purification typically increases specific activity 100-10,000 fold. Total activity should remain constant or decrease only slightly through purification steps; a large drop indicates enzyme denaturation or loss.
The turnover number (kcat) represents the maximum number of substrate molecules converted to product per enzyme active site per unit time. Combined with the Michaelis constant (Km), it defines the catalytic efficiency (kcat/Km), which is the most comprehensive measure of enzyme performance. This calculator handles all common enzyme activity calculations and unit conversions used in biochemistry research and industrial enzymology.
Streamline enzyme activity calculations for research, quality control, and industrial applications. Essential for tracking purification progress, comparing enzyme preparations, and converting between activity units used by different suppliers. This enzyme activity calculator helps you compare outcomes quickly and reduce avoidable mistakes when making day-to-day care decisions. Use the estimate as a planning baseline and confirm final decisions with a qualified professional when risk is high.
Enzyme Activity (U) = Δ[product] (μmol) / time (min). Specific Activity = Activity (U) / total protein (mg). Turnover Number: kcat = Vmax / [E]total = (activity × MW) / (protein mass × 10⁶). 1 katal = 6 × 10⁷ U. Purification Fold = specific activity (step) / specific activity (crude).
Result: Activity = 0.5 U/mL, Specific Activity = 0.25 U/mg
If 5 μmol of product forms in 10 minutes in 1 mL, the activity is 5/10 = 0.5 U/mL. With 2 mg/mL protein, specific activity = 0.5/2 = 0.25 U/mg. For a 45 kDa enzyme, kcat = (0.5 × 45000)/(2 × 10⁶) = 0.011 s⁻¹ per active site.
Enzyme activity is measured by monitoring the rate of substrate consumption or product formation. Spectrophotometric assays (measuring absorbance change) are the most common because they allow continuous, real-time monitoring. Coupled assays link the enzyme reaction to a secondary reaction that produces a detectable product (e.g., NAD⁺/NADH at 340 nm). Fluorometric assays offer higher sensitivity for low-activity samples. Radiometric assays using isotope-labeled substrates provide the highest sensitivity but require special handling and waste disposal.
A purification table tracks total protein, total activity, specific activity, purification fold, and percent yield at each step. The starting material (crude extract) defines the baseline. Ammonium sulfate precipitation, ion exchange chromatography, size exclusion, and affinity chromatography are common purification steps. Each step should increase specific activity while maintaining high percent yield. If specific activity doesn't increase at a step, that step isn't effectively separating your enzyme from contaminants.
In industrial applications, enzyme activity is often expressed in proprietary units specific to the application — for example, SKB (starch-digesting) units for amylases, FIP units for lipases, or Anson units for proteases. The relationship between these units and standard U depends on the specific assay conditions. Industrial enzymes are typically sold based on activity per volume or mass of preparation, with specific activity being less relevant since purity is not the goal — functional performance at minimum cost is what matters.
One unit (U) of enzyme activity is the amount that catalyzes the conversion of 1 micromole of substrate per minute under defined conditions (typically 25°C or 30°C, optimal pH). This keeps planning practical and lowers the chance of preventable errors.
The katal (kat) is the SI unit of catalytic activity: 1 kat = 1 mol/s. Since enzymes work on microscale, nanokatals (nkat) or microkatals (μkat) are more practical. 1 U = 16.67 nkat.
Specific activity (U/mg protein) indicates enzyme purity. Higher values mean a greater fraction of the protein is your enzyme of interest. A pure enzyme has maximum specific activity.
It depends on the starting material. From crude cell lysate, 100-1000 fold purification is typical. From serum, 10,000+ fold may be needed. Each chromatography step usually gives 5-20 fold purification.
Some active enzyme is inevitably lost at each step (incomplete binding/elution, denaturation, proteolysis). A yield of 20-50% per step is typical. Optimizing each step minimizes losses.
Catalytic efficiency (kcat/Km) measures how efficiently an enzyme converts substrate at low concentrations. The theoretical maximum is the diffusion limit (~10⁸-10⁹ M⁻¹s⁻¹). Enzymes approaching this limit are called "catalytically perfect."