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By lowering the activation energy, an enzyme affects the rate at which reaction occurs. Enzyme-
boosted reactions may proceed from 100,000 to 10 million times faster than they would without the
enzyme. In an enzyme-catalyzed reaction, the reactant (the substance being acted upon) is called the
substrate. Substrate molecules combine with enzyme molecules to form a temporary enzyme-substrate
complex. Products are formed, and the enzyme molecule is released unchanged. Thus, the enzyme is
not used up in the process and is capable of catalyzing the same reaction again and again. This can be
summarized as follows:
Before we proceed, let’s visualize an enzyme. Look at Figure 8-2. Using common, everyday items, think
of an enzyme as a key that unlocks a lock. Imagine that you have a number of locks, and all use the same
key. You would only need one key to unlock them. Changing the shape of the key just a tiny bit may still
allow the key to function in the lock, but you may have to fumble with the key a bit to get the lock open.
Changing the key more results in an inability to open the lock. Similarly, a change in the shape of an
enzyme alters its function. The structure of an enzyme is altered due to changes on cellular pH and body
temperature changes.
Proteases are enzymes commonly found in the supermarket, such as contact cleaner and meat
tenderizer. As their name suggests, proteases are enzymes with the specific ability to break up proteins
into smaller polypeptides. Major digestive proteases in humans are pepsin, trypsin, and chymotrypsin.
Pepsin is found in the stomach of animals and helps begin the digestion of meat, fish, cheese, and other
ingested proteins. Digestion of ingested proteins in our stomach and small intestines releases individual
amino acids to the blood stream for other metabolic processes including synthesis of our required
proteins.
Proteases digest various proteins in all organisms including plants. Plant proteases of particular
interest are found in tropical plants such as papaya and pineapple. Proteases are used commercially in
some soaps, stain removers, carpet cleaners, and detergents to dissolve protein stains such as grass and
bloodstains. The most abundant commercially available protease is papain extracted from papaya plants.
Papain is used in most meat tenderizers and in some contact lens cleaners.
In this activity we will compare different proteases ability to digest jello gelatin proteins. Gelatin
is extracted from dead animal skin and bones as collagenous material, which is then treated to produce the
final gelatin. Gelatin has a unique sequence of amino acids which bind to form a repeating sequence of
the triplet glycine-proline-hyroxyproline, which gives gelatin its triple helical structure. This helical
structure is responsible for trapping water molecules and forming gels.
Materials:
Cranberry Jello
Canned Pineapple Juice
Fresh Pineapple
Distilled Water
Teacher Notes:
The day before the lab, the jello needs to be made. Boiled pineapple juice and frozen pineapple
juice are made from fresh pineapple juice, then boiled or frozen. You may need to warm up your
spectrophotometer as much as 24 hours prior to the lab.
In this experiment, the starting solution will be clear, allowing nearly 100% of light to be
transmitted through the sample tube. If the enzyme produces the product, the sample will darken,
permitting less light to be transmitted through the cuvette. The change in transmittance will be directly
proportional to the amount of product. If the transmittance readings are recorded over time, the rate of the
enzymatic reaction can be calculated.
6. Measure the absorbance of your solution at 500 nm and record your results below.
7. Immediately pour back the solution into your beaker.
8. Repeat your measurements every five minutes for a total of thirty minutes.
9. Construct a data table that includes all of the tested variables in the experiment.
10. Enter your group results in the spreadsheet on the board. Be sure to get the other groups results.
11. Calculate the rate of enzyme activity by subtracting the absorbance at 5 minutes from your final
absorbance reading and record above. (Tf - Ti = Rate of activity)
Analysis:
1. Is the release of pigment from the gelatin the same in all the samples? How do you know?
2. Identify the active site on the jello for the pineapple enzyme. Explain what might have
caused the differences in enzyme digestion between your tests.
3. The spec. 20 helps you to measure the amount of light absorbed by your samples. Explain
how the spec 20 allows you to know which enzyme performed the best. Then bar graph
your change in absorbance for each sample, use a different color for each sample.