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Table of Contents
1. Title
2. Introduction
3. Principle
4. Materials
5. Procedure
6. Results7. Graph
8. Deduction
9. Discussion
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10.Precautions
11.Conclusion
DETERMINE THE Km and vmax OF THE
ACIDIC PHOSPHATASE
INTRODUCTION:
Catalysts are agents the increase the rate of chemical processes; those in cells are called
enzymes. There are literally hundreds of enzymes in each cell. Enzymes are involved in
catabolic and anabolic reactions, reactions that break down macromolecules and those that
build macromolecules, respectively. The generic equation for the mechanism of enzyme
action is familiar to you:
Enzyme + Substrate -- Enzyme-Substrate Complex - Enzyme + Product
There are three important features of this reaction that are important. First, enzymes
display a great degree of substrate specificity. That is, they catalyze a single chemical
reaction in the cell. Second, the binding of enzyme and substrate is like that of a hand and
glove. This model is called the induced fit model of enzyme action and describes well the
interaction of enzyme and substrate. Therefore, the enzyme will act upon only substratesthat fit into the active site of the enzyme. Third, the enzyme is not destroyed or even
modified in this reaction. Rather, it is released and is available to react with more
substrate molecules. This feature allows enzymes to be very efficient in catalytic
reactions and explains why small quantities of enzymes are adequate for cellular reactions.
The velocity or rate of a reaction can be determined by measuring either one of two things:
(1) substrate concentration, which should decrease as a reaction proceeds, or
(2) product formation, which should increase from an initial concentration of zero as the reactionproceeds.
PRINCIPLE:
Phosphatases are enzymes that hydrolyze phosphate monoesters and release inorganic
phosphate. Alkaline phosphatases (orthophosphoric monoester phosphohydrolases) are the
phosphate hydrolases that have a maximum activity at a relatively high pH (>7.0). This enzyme
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is widespread and occurs in both eukaryotic and prokaryotic cells. InEscherichia coli, its
physiological role is to cleave phosphoryl groups providing the cell with a source of inorganic
phosphate.
Phosphatases catalyzes the hydrolysis of phosphate groups from phosphoesters. They are widely
distributed in any organism. Many phosphatases are highly substrate-specific, like those enzymes
involved in signal transduction.
A number of phosphatases, however, cleave virtually any phosphate ester. Such unspecific
enzymes function mainly in the catabolic breakdown of metabolites or nutrients.
Depending on the pH at which such phosphatases have optimal activity, between acidic
phosphatases (also called acid phosphatases) and alkaline phosphatases can be
distinguished. Acidic phosphatases are widely distributed in many organisms, including
plants. They work optimally at approximately pH 5 without additional cofactors. In this
experiment, we will extract an acidic phosphatase from bean sprout.
To measure its activity, we used a substrate called disodium phenylphosphate. The more
activity of acidic phosphatase has, the more phenol is produced. So the content of phenolvaries in proportion with the activity of the acidic phosphatase. The amount of phenol is
determined by Folin-phenol method.
Figure 4-1 Acidic phosphatase catalyzes the reaction
Because of the hyperbolic shape of Vo against [S] plots, Vmax can only be determined from
an extrapolation of the asymptotic approach of Vo to some limiting value as [S] increases
indefinitely; and Km is derived from that value of [S] giving Vo = Vmax/2.
However, several rearrangements of the Michaelis-Menten equation transform it into a
straight-line equation. The best known of these is the Lineweaver-Burk double-reciprocal
plot. The Lineweaver-Burk plot is one way of visualizing the effect of inhibitors and
determining the Michaelis Constant Km and the Maximum Velocity Vmax from a set of
measurements of velocity at different substrate concentrations.
Vmax and Km are the two parameters which define the kinetic behavior of an enzyme as a
function of [S].
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If 1/Vo is plotted against 1/[S], a straight line is obtained where the slope is equal to
Km/Vmaxthe y-intercept is equal to 1/Vmax and x-intercept is equal to -1/ Km.
Figure 4-2 The Lineweaver-Burk double-reciprocal plot, depicting extrapolations that allow the
determination of the x- and y-intercepts and slope.
Where:
V0= initial velocity of the reactionVmax= maximum velocity of the reaction
[S]= substrate concentration
Km= the substrate concentration at which 1/2 Vmax is achieved
MATERIALS:
Apparatus: Petri dish, scissors, 5g of bean sprout, grinding pestle, mesh silk, beaker, water,
Eppendorf tube, test tubes, homogenizer, centrifuge, spectrophotometer, vortex
Mixer, incubator, marker, Gloves and watch.
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Solution : 1mL HAC(acetate) buffer (pH 5.6), 0.4mM phenol standard solution, H2O, 1 M
Na2CO3, Folin-phenol reagent, 5mol/L disodium benzene phosphate, 0.2 M acetate
Buffer, acid phosphatase solution.
PROCEDURE:
A. Preparation of the acidic phosphatase
1. Weigh 5g of bean sprout.
2. Add 1mL HAC buffer (pH 5.6) and then grind the bean sprout into homogenization.
Then place it for 30min at room temperature.
3. Pour the resulting homogenization through the mesh silk into a 2mL tube then
centrifuge at 6000rpm for 20min.
4. Transfer the resulting supernatant which containing the acidic phosphatase into a fresh
tube.
5. Dilution the supernatant for 40 times with HAC buffer (pH 5.6).
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B. Determine the Km and Vmax of the acidic phosphatase
1. Plot a standard curve of phenol content
2. Select 9 tubes and mark them as 0-8, #0 tube is used as blank
Additions (mL)tube number
0 1 2 3 4 5 6 7 8
0.4mM phenol
standard solution0
0.
1
0.
2
0.
3
0.
4
0.
5
0.
6
0.
7
0.
8
H2O 10.
9
0.
8
0.
7
0.
6
0.
5
0.
4
0.
3
0.
2
1M Na2CO3 2 2 2 2 2 2 2 2 2
Folin-phenol
reagent
0.
5
0.
5
0.
5
0.
5
0.
5
0.
5
0.
5
0.
5
0.
5
3. Mix well then incubate at 35 for 10 min
4. Measure the A680 of the samples and the blank tube is used for the zero setting.
5. A680 is plotted against phenol content.
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C. Determine the Km and Vmax of the acidic phosphatase
1. Select 7 tubes and mark them as 0-6, #0 tube is used as blank
Additions (mL)tube number
0 1 2 3 4 5 6
5mmol/L disodium
benzene
phosphate
0.5 0.10.1
50.2
0.2
50.3 0.5
0.2M acetate
buffer0 0.4 0.3
50.3 0.2
50.2 0
incubate at 35 for 2 min
acidic
phosphatase
solution
0 0.5 0.5 0.5 0.5 0.5 0.5
incubate at 35 for 15min
1M Na2CO3 2 2 2 2 2 2 2
Folin-phenol
reagent0.5 0.5 0.5 0.5 0.5 0.5 0.5
acidic
phosphatase
solution
0.5
2. Incubate at 35 for 10min.
3. Measure the A680 of the samples and the blank tube is used for the zero setting.
4. Calculate V0 and [S] the content of the phenol in each tube.
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1/Vo is plotted versus 1/[S], a straight line is obtained where the slope is equal to
Km/Vmaxthe y-intercept is equal to 1/Vmax and x-intercept is equal to -1/ Km.
RESULTS:
(B) :
Tube number 0 1 2 3 4 5 6 7 8
Absorbance/ (A680) 0.00 0.14 0.247 0.346 0.449 0.562 0.657 0.767 0.876
Mass of Phenol
/mol
0.00 0.04 0.08 0.12 0.16 0.20 0.24 0.28 0.32
(C) :
From Graph (B), using y= 0.355x,
(i) When x= 0.134, y= 0.0476. Amount of phenol=0.0476 mol.
(ii) When x= 0.165, y= 0.0586. Amount of phenol=0.0586 mol
(iii) When x= 0.212, y= 0.0753. Amount of phenol=0.0753 mol
(iv) When x= 0.211, y= 0.0749. Amount of phenol=0.0749 mol
(v) When x= 0.291, y= 0.1033. Amount of phenol=0.1033 mol
(vi) When x=0.338, y=0.120. Amount of phenol=0.120 mol
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From equation: Vo = Amount of phenol
Time
(i) Vo = 0.0476 1/Vo = 1
15 3.17 x 10-3
= 3.17 x 10-3 ms-1 = 315.3 m-1s
(ii) Vo = 0.0586 1/Vo = 1
15 3.91 x 10-3
= 3.91 x 10-3 ms-1 = 256.1 m-1s
(iii) Vo = 0.0753 1/Vo = 1
15 5.02 x 10-3
= 5.02 x 10-3 ms-1 = 199.3 m-1s
(iv) Vo = 0.0749 1/Vo = 1
15 4.99 x 10-3
= 4.99 x 10-3 ms-1 = 200.3 m-1s
(v) Vo = 0.1033 1/Vo = 1
15 6.89 x 10-3
= 6.89 x 10-3 ms-1 = 145.2 m-1s
(vi) Vo = 0.120 1/Vo = 1
15 8.00 x 10-3
= 8.00 x 10-3 ms-1 = 125.0 m-1s
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Tube number 0 1 2 3 4 5 6
Absorbance 0.00 0.134 0.165
0.212 0.211 0.291 0.338
[S] /mmol/L 5.0 1.0 1.5 2.0 2.5 3.0 5.0
1/ [S] /mmol-1L 0.20 1.0 0.667 0.50 0.40 0.333 0.20
Vo /(x10
-3
)ms-1 - 3.17 3.91 5.02 4.99 6.89 8.00
1/Vo / m-1s - 315.3 256.1 199.3 200.3 145.2 125.0
GRAPH:
(B) : Graph of A680 against phenol content
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(C) : Graph of 1/Vo against 1/[S]
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DEDUCTION:
(i) From graph (c), using equation y = 242.3 x +81.63,
Where line cuts the x-axis, y=0.
Therefore, 0 = 242.3 x + 81.63,
242.3 x = - 81.63,
x = -81.63
242.3
= -0.337
Hence, x-intercept = - 0.337 mmol-1L.
As x-intercept is -1/Km,
-1/Km = -0.337
Km = 2.97 mmol/L
(ii) From graph (c), using equation y = 242.3 x +81.63,
Where line cuts the y-axis, x=0.
Therefore, y = 81.63
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Hence, y-intercept = 81.63 m-1s.
As y-intercept is 1/Vmax,
1/Vmax = 81.63
Vmax = 0.01225 ms-1
DISCUSSION:
There are four factors that affect enzyme activity. The first is the amount of enzyme. The
initial velocity is proportional to the amount of enzyme molecules. The more enzyme, the
greater the initial velocity will be since more product is being formed. Another factor
that greatly influences enzyme activity is temperature. Proteins are usually denatured by
temperatures above 50oC. Any temperature lower than that causes an increase in enzyme
activity, until the freezing point is reached. Here, freezing an enzyme often denatures itand results in a loss of catalytic activity. However, for every enzyme, there is an optimal
temperature that results in the greatest Vo. This temperature is usually in the range of
20oC to 40oC.
The third factor that influences enzyme activity is pH. Excesses of pH, either solutions
that are too acidic or too alkaline, cause denaturation of the enzyme. Hence, all enzyme
activity is lost and the Vo equals zero. Most enzymes in plants and animals operate most
efficiently at near neutral pH. However the pH optimum of the enzyme you will study
today is 4.5. The name of the enzyme is acid phosphatase, whose name is indicative of
the pH optimum of this enzyme.
Finally, substrate concentration also influences the Vo of an enzyme-catalyzed reaction.
At low substrate concentration, the active sites on the enzymes are not saturated by
substrate and the enzyme is not working at maximal capacity. As the concentration of
substrate increases, more and more enzyme molecules are working. At the point of
saturation, no more active sites are available for substrate binding; at this point, the
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enzyme reaches its maximal velocity, designated Vmax. The following graph illustrates
this.
The entire relationship is described by a hyperbolic curve. The initial velocity of an enzyme
increases in a linear manner as the substrate concentration is increased. As substrate
concentration increases beyond this point, the Vmax occurs because the enzyme is saturated with
substrate. The substrate concentration required to yield half the maximal velocity (Vmax/2) can
also be determined from the figure below. This number is known as the Michaelis constant andis abbreviated Km. The Km is a measure of enzyme affinity.
For example, a Km of 0.2 mole/l of substrate would indicate that the substrate-binding site
would be half-saturated when the substrate is present in that concentration. Such an
enzyme would have a low affinity for its substrate. In contrast, a Km of 10-7mole/l
indicates that the enzyme has a high affinity for its substrate, since it is half saturated at
this low concentration of substrate.
The effect of substrate concentration on the velocity of an enzyme-catalyzed reaction can
be described by the Michaelis-Menten equation.
Vo = Vmax[S]
Km +[S]
Rearrangement of the equation to resemble that of a straight line (y=mx+c) by taking theinverse of both sides yields:
1 = Km 1 + 1
Vo Vmax [S] Vmax
Vmax
[S]
V0
Km
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This double-reciprocal plot is known as the Lineweaver-Burk plot and allows us to
determine exactly what the Vmax and Km of a particular enzyme-catalyzed reaction are by
solving for each in the equation.
PRECAUTIONS:
There may have been errors due to:
- Misuse of pipettes.
- Test tubes being wet or having some dirt leading to inaccurate results.
- Absorbance may have been disturbed as some of the light might have been absorbed by
the glass sample of the spectrophotometer itself or by fingerprints lying on the sample
glass leading to systematic errors.
- Maybe more than 2/3 of the solution was in the glass sample leading to overflow of liquid,
thus affecting absorbance results
- Or perhaps less than 2/3 of the solution was in the glass sample leading to UV light
passing over the solution hence affecting the absorbance results.
- The fact that different groups were using the centrifuge at the same time, the eppendorf
tubes might be of different weights and they might have been arranged in the wrong
position.
- Use clean glass wear and supplies
- Make sure cuvettes are clean of all residues
- Become familiar with spectrophotometry before proceeding
Slope = Km/Vmax1/V0
1/[S]
1/Vmax
-1/Km
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- Always let the spectrophotometer warm up for 15-20 minutes before using
- Know the limits of the spectrophotometer which is being used as most
spectrophotometers cannot linearly read absorbance values beyond 2.0 units. Thus, the
protein sample must be diluted to work within this range
- Arrange the eppendorf tubes diagonally in opposite directions so as to keep weight
balance
CONCLUSION:
From the experiment, the
Maximum velocity of the reaction, Vmax = 0.0123 ms-1
and the
Substrate concentration at which Vmax is achieved, Km = 2.97 mmol/L
Enzymes increase the rate of spontaneous reactions, not changing their
direction.
They do this by their ability to bind specific substrates to form transition
state complexes.
Km is related to the ability of the enzyme to bind its substrate.
A higher Km means poorer binding.
The catalytic ability of an enzyme can be characterized by these two
parameters.
Virtually every chemical reaction in the cell is catalyzed by an enzyme.
The enzyme binds its substrates with great specificity and it usually aids in
the chemical reaction that takes place.
However, the enzyme itself emerges unchanged.