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Investigate the effect of heat denaturation on the rate of enzyme activity Simplified Revision Notes

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Investigate the effect of heat denaturation on the rate of enzyme activity

Materials needed:

  • Hydrogen Peroxide (substrate)
  • Celery (contains enzyme catalase)
  • pH buffer 9/10 (keeps pH constant)
  • Thermostatically controlled water bath (varying temperatures: 30°C, 100°C)
  • Washing up liquid (measure the rate of activity by volume of foam produced and breaks down the cell wall)
  • Graduated cylinders
  • Plastic droppers

Method:

  1. Place 10 cm³ of celery, 1 drop of washing-up liquid, and 10 cm³ of pH buffer together in a graduated cylinder.
  2. In another graduated cylinder, add 5 cm³ of hydrogen peroxide.
  3. Place both graduated cylinders in a thermostatically controlled water bath set at 30°C for 2 minutes to allow all reagents to reach the exact temperature.
  4. After 2 minutes, add the hydrogen peroxide to the graduated cylinder containing the other reagents.
  5. Record the volume of foam produced after 1 to 2 minutes (the foam volume measures enzyme activity by indicating the amount of oxygen produced).
  6. Repeat the experiment at 100°C.
  7. Compare and comment on the volume of foam produced at each temperature.

Results:

Temperature30°C100°C
Volume of foam
cm³ / 2 minutes
40 cm³0 cm³

A large volume of foam was produced at 30°C, as this is the optimum temperature for the enzyme catalase, resulting in the greatest enzyme activity. At 100°C, no foam was produced because the heat caused the enzyme to become denatured, meaning it lost its 3D, folded, globular shape and no longer functions.

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