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Friday, March 1, 2019

Effect of Changes in Substrate Concentration on the Reaction Rate

Effect of changes in substratum submerging on the chemical response roam of an enzyme IB biology Internal Assessment 3/23/12 Research Question Effect of changes in substrate assiduity come in on the reaction rate of an enzyme Introduction In this essay, the substrate is atomic number 1 hydrogen hydrogen peroxide. The purpose of this investigation is to find out the affinity between the substrate preoccupancy and the rate of reaction. Substrates are molecules that are acted upon by enzymes. For instance, amylase, an enzyme found in saliva, helps break down complex starch molecules (substrates) into little sugar molecules (products).In other biochemical reactions, substrates require assistance of specific enzymes to pass water new products. When the sum of money of enzyme stays constant, the substrate concentration go away govern the rate of reaction. However, when the number of substrate molecules exceeds the available number of enzyme, the rate of reaction will no lo nger increase, but stay constant. If in that location is a constant amount of enzyme, as the concentration of a substrate increased, the rate of reaction will increase as well. This is because of molecular collisions.If you have much reactant molecules, there are more to collide. Aim The effect of hydrogen peroxide on the enzyme activity of catalase Hypothesis When the amount of enzyme stays constant, the substrate concentration will determine the rate of reaction CONTROLLED VARIABLES Units Possible effect(s) on results summation of enzyme 2. 8g an extra drop of enzyme can fudge the rate of reaction size and type of shew pipages 30ml The size and type of establish pipeworks were constant, because they can alter the pressure Units RangeINDEPENDENT VARIABLE Hydrogen Peroxide (Substrate) immersion ml 5,10,15,20,25,30 DEPENDENDENT VARIABLE Rate of Reaction Seconds 80 secs VARIABLES METHOD FOR absolute VARIABLES CONTROLLED VARIABLES Method for control 1. Amount of enzym e all(prenominal) liver-colored used were at a constant weight of 2. 8g 2. Size of leaven tube All test tubes were 30ml METHOD FOR COLLECTING DATA 1. Prepare a tube rack and place 6 30ml tubes in them. 2. Weigh liver at a constant 2. 8g. 3. Place the 6 pieces of liver into the test tubes. 4.Obtain 3% hydrogen peroxide and a graduated cylinder. 5. Pour 5ml into test tube 1, 10ml into test tube 2, 15ml into test tube, 20ml into test tube 4, 25 ml into test tube 5, 30ml into test tube 6 (but not at once one after the another) . 6. Once hydrogen is in the test tube start the stop watch to see how long it will take to react. 7. Repeat the action in no. 5 & 6, hexad times for each(prenominal) tube. 8. Observe what happens to the liver while reacting to the hydrogen peroxide. 9. devolve up the station and pour liver into a waste beaker. 0. purify each of the test tubes out and vagabond the materials away. The materials used in this experiment are I. 50-ml graduated cylinder II. Fr esh liver III. 6 test tubes (30 ml) IV. 3% Hydrogen peroxide V. Disposable Pipettes VI. Stopwatch VII. Digital plateful VIII. 50ml beaker IX. Test tube rack X. Plastic knife XI. Scissors soft DATA. The reaction started as soon as Catalase touched the surface of hydrogen peroxide. More concentrated hydrogen peroxide produced more oxygen bubbles and the reaction rate was faster.As more substrate was added the reaction was faster. Once the 5ml of hydrogen peroxide was put into the test tube with the liver, the reaction rate was slow. As the amount of hydrogen peroxide increased the reaction became faster. When putting the 15ml of peroxide into the test tube 3 during the first trial the reaction bubbles spilled into tube 4 affecting the result slightly, because it made it to start reacting before the 20ml of peroxide was put into test tube 4 . In test tube 6 during the first trial the liver was lifted from the surface about 2cm.The wring for test tubes 1-5 during all the sextette tr ials was light brown, but for tube six the color was dark brown. BEFORE SUBSTRATE AFTER SUBSTRATE arrangement RAW DATAPROCESSING RAW DATA Amount of Solute concentration (ml) Repeat Reaction time (s)(+/-0. 5s) 5 1 130 2 129 3 130 4 132 5 128 6 123 10 1 100 2 110 3 92 4 98 5 95 6 101 15 1 87 2 87 3 84 4 88 5 82 6 84 20 1 63 2 70 3 78 4 71 5 74 6 75 25 1 59 2 58 3 60 4 60 5 58 6 59 0 1 39 2 42 3 37 4 41 5 40 6 38 Amount of Solute concentration (ml) Repeat Reaction time (s)(+/-0. 5s) Mean (s)(+/-0. 5s) 5 1 130 128. 6 2 129 3 130 4 132 5 128 6 123 10 1 100 99. 3 2 110 3 92 4 98 5 95 6 101 15 1 87 85. 3 2 87 3 84 4 88 5 82 6 84 20 1 63 71. 8 2 70 3 78 4 71 5 74 6 75 25 1 59 59. 0 2 58 3 60 4 60 5 58 6 59 30 1 39 39. 5 2 42 3 37 4 41 5 40 6 38 *Sample Calculation of mean sum of reaction time for tube/ of trials 39+42+37+41+40+38=237 237/6= 39. 5 PRESENTING PROCESSED DATA CONCLUDING My possible action was supported based on my data. The data suggests that as the hydrogen peroxide concentration increases the rate of reaction increased. It took slight time for it to react consort to figure 1. The general trend that was in this experiment was that the numbers for each amount of hydrogen were in the same range e. g. 15ml (87 87 84 88 82 84).My prediction was correct the more substrate was added the less time it used to react hence a faster reaction rate. There were no anomalous results. The data in this experiment suggests that the change in amount of substrate creates a faster reaction rate. EVALUATING PROCEDURES heretofore though the experiment and the outcome of the experiment support my hypothesis there are some weakness in this experiment that would have enabled a better outcome. The weaknesses that were present in the in the method of chosen for this investigation was the size of liver.The last weakness the arrangement in the steps taken. meliorate THE INVESTIGATION To imp rove the results of this investigation is the size of liver should have been smaller, so that more reaction would have taken place and the color of the liver would have changed more for all of the tubes. Another improvement would be in the arrangement of steps taken. To avoid the spillover of the reaction bubbles into test tube 4, the amount of hydrogen peroxide should have been in the test tubes first thusly the liver should have been dropped in after.

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