Enzymes - GRE Subject Test: Biochemistry, Cell, and Molecular Biology
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A researcher is studying the rate of an enzyme-catalyzed reaction by placing increasing amounts of substrate into a solution containing the enzyme. After a certain concentration, the rate of the reaction plateaus and does not go any higher. What has happened?
A researcher is studying the rate of an enzyme-catalyzed reaction by placing increasing amounts of substrate into a solution containing the enzyme. After a certain concentration, the rate of the reaction plateaus and does not go any higher. What has happened?
If the reaction rate has plateaued, this indicates that the enzyme has reached saturation. At this point, every active site on every molecule of enzyme is actively catalyzing the reaction as quickly as it can. The only way to change the reaction rate, at this point, would be to increase the concentration of the enzyme in the solution. Further increasing substrate concentration will have no effect.
We know that the enzyme has not become denatured because the reaction is still occurring. The rate of the reaction is constant during the plateau, and does not drop to zero.
If the reaction rate has plateaued, this indicates that the enzyme has reached saturation. At this point, every active site on every molecule of enzyme is actively catalyzing the reaction as quickly as it can. The only way to change the reaction rate, at this point, would be to increase the concentration of the enzyme in the solution. Further increasing substrate concentration will have no effect.
We know that the enzyme has not become denatured because the reaction is still occurring. The rate of the reaction is constant during the plateau, and does not drop to zero.
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In a Lineweaver-Burk plot, what quantity determines the y-intercept?
In a Lineweaver-Burk plot, what quantity determines the y-intercept?
A Lineweaver-Burk plot is a way to graphically represent enzyme kinetics. It is convenient because several portions of the graph readily display important information, such as rate constants. The y-intercept in particular is useful because it represents the reciprocal of the maximum velocity. The x-intercept describes the negative reciprocal of the Michaelis constant. The slope is the quotient of the Michaelis constant over the maximum velocity.
A Lineweaver-Burk plot is a way to graphically represent enzyme kinetics. It is convenient because several portions of the graph readily display important information, such as rate constants. The y-intercept in particular is useful because it represents the reciprocal of the maximum velocity. The x-intercept describes the negative reciprocal of the Michaelis constant. The slope is the quotient of the Michaelis constant over the maximum velocity.
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What information is contained in a Lineweaver-Burk plot that is not present in a standard Michaelis-Menten plot?
What information is contained in a Lineweaver-Burk plot that is not present in a standard Michaelis-Menten plot?
The two plots contain the same information. A Michaelis-Menten plot shows the relationship between initial reaction rate concentration of substrate (
versus 
). A Lineweaver-Burk plot shows the relationship between the inverses of these same two variables, however, it is much easier to visualize important data on a Lineweaver-Burk plot. The x-intercept, the y-intercept, and the slope all contain points of interest. A downside of the Lineweaver-Burk plot, however, is that it is more susceptible to inaccuracy if there is some flaw in the accumulated data.
The two plots contain the same information. A Michaelis-Menten plot shows the relationship between initial reaction rate concentration of substrate (
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Which of the following changes will alter 
of an enzyme-catalyzed reaction?
Which of the following changes will alter
The only option that will alter the 
is to add a non-competitive inhibitor. The addition of this inhibitor will affect the amount of free enzyme available to catalyze the reaction, and thus lower the 
by reducing the effective enzyme concentration.
Addition of a competitive inhibitor will alter the 
, but not the 
. Increasing the substrate concentration will have no effect once saturation has been reached.
The only option that will alter the
Addition of a competitive inhibitor will alter the
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A catalyst is an enzyme that promotes a reaction. In terms of free energy, what does a catalyst change about the reaction to promote the reaction proceeding?
A catalyst is an enzyme that promotes a reaction. In terms of free energy, what does a catalyst change about the reaction to promote the reaction proceeding?
During a reaction, the reactants must pass through high-energy transition states before they evolve into the products. The catalyst reduces the free energy of this transition state, thus making it 'easier' for the reactant to undergo the chemical reaction since the activation energy has been lowered.
During a reaction, the reactants must pass through high-energy transition states before they evolve into the products. The catalyst reduces the free energy of this transition state, thus making it 'easier' for the reactant to undergo the chemical reaction since the activation energy has been lowered.
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What is the primary mechanism by how enzymes increase the rate of a reaction?
What is the primary mechanism by how enzymes increase the rate of a reaction?
Enzymes exert their effect on the reaction rate by decreasing the energy needed for the reaction to proceed. As a result, the enzyme will decrease the activation energy. It should be noted that the forward reaction rate and reverse reaction rate are both increased by an enzyme. If this were not the case, more product would be made compared to the uncatalyzed reaction, and enzymes do not affect equilibrium constants for reactions.
Enzymes exert their effect on the reaction rate by decreasing the energy needed for the reaction to proceed. As a result, the enzyme will decrease the activation energy. It should be noted that the forward reaction rate and reverse reaction rate are both increased by an enzyme. If this were not the case, more product would be made compared to the uncatalyzed reaction, and enzymes do not affect equilibrium constants for reactions.
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Which of the following types of enzymes is responsible for joining molecules by forming new chemical bonds?
Which of the following types of enzymes is responsible for joining molecules by forming new chemical bonds?
Ligases are enzymes that catalyze the formation of new bonds between molecules. A classic example is DNA ligase, an enzyme that synthesizes phosphodiester bonds in the DNA backbone.
Transferases move small molecules from one molecule to another, sometimes altering the functional groups of a compound. Isomerases convert molecules from one isomer to another. Lyases are enzymes that break bonds through a means other than hydrolysis (typically by formation of a double bond).
Ligases are enzymes that catalyze the formation of new bonds between molecules. A classic example is DNA ligase, an enzyme that synthesizes phosphodiester bonds in the DNA backbone.
Transferases move small molecules from one molecule to another, sometimes altering the functional groups of a compound. Isomerases convert molecules from one isomer to another. Lyases are enzymes that break bonds through a means other than hydrolysis (typically by formation of a double bond).
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Chymostrypsin cleaves a polypeptide into two smaller subunits by using water in order to make the new amino and carboxyl termini. Based on this mechanism, what type of enzyme is chymostrypsin?
Chymostrypsin cleaves a polypeptide into two smaller subunits by using water in order to make the new amino and carboxyl termini. Based on this mechanism, what type of enzyme is chymostrypsin?
Since chymotrypsin uses a water molecule in order to cleave the polymer, it is considered a hydrolase enzyme.
Since chymotrypsin uses a water molecule in order to cleave the polymer, it is considered a hydrolase enzyme.
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During glycolysis, glucose-6-phospate is rearranged in order to form fructose-6 phosphate. The enzyme that accomplishes this does not change the intermediate's chemical formula in any way, but simply alters the shape of the molecule.
Based on this action, what type of enzyme is involved in this step in glycolysis?
During glycolysis, glucose-6-phospate is rearranged in order to form fructose-6 phosphate. The enzyme that accomplishes this does not change the intermediate's chemical formula in any way, but simply alters the shape of the molecule.
Based on this action, what type of enzyme is involved in this step in glycolysis?
Since the enzyme has changed the shape of the molecule without altering its chemical formula, the enzyme has simply made a new isomer of the molecule. This action is accomplished by isomerase enzymes.
Since the enzyme has changed the shape of the molecule without altering its chemical formula, the enzyme has simply made a new isomer of the molecule. This action is accomplished by isomerase enzymes.
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Which of the following is not a class of enzymes that alter epigenetic states?
Which of the following is not a class of enzymes that alter epigenetic states?
All answer choices fit the description. Epigenetics (above the gene) are heritable modifications of chromatin and DNA that affect gene expression. Pioneer transcription factors are able to bind DNA in heterochromatin and recruit enzymes that promote euchromatin formation which allows other transcription factors to bind and effect gene expression. Histone methyltransferases and acetyltransferases methylate and acetylate histones, respectively, to alter gene expression. DNA methyltransferases are also enzymes that confer epigenetic changes to DNA by methylation, which usually represses gene expression.
All answer choices fit the description. Epigenetics (above the gene) are heritable modifications of chromatin and DNA that affect gene expression. Pioneer transcription factors are able to bind DNA in heterochromatin and recruit enzymes that promote euchromatin formation which allows other transcription factors to bind and effect gene expression. Histone methyltransferases and acetyltransferases methylate and acetylate histones, respectively, to alter gene expression. DNA methyltransferases are also enzymes that confer epigenetic changes to DNA by methylation, which usually represses gene expression.
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Which of the following are not enzymes that act on DNA?
Which of the following are not enzymes that act on DNA?
The correct answer is acetylases. DNA can be directly methylated by methylases, mended during DNA repair by ligases, uncoiled by topoisomerases, and replicated by polymerases. However, DNA cannot be acetylated. Epigenetic associated-acetylation occurs only on histones to determine the chromatin state of a specific region.
The correct answer is acetylases. DNA can be directly methylated by methylases, mended during DNA repair by ligases, uncoiled by topoisomerases, and replicated by polymerases. However, DNA cannot be acetylated. Epigenetic associated-acetylation occurs only on histones to determine the chromatin state of a specific region.
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What is the name of the class of enzymes that permit a phospholipid in the cellular membrane to move from facing the exoplasm (outside of the cell) to the cytosol (cellular interior)?
What is the name of the class of enzymes that permit a phospholipid in the cellular membrane to move from facing the exoplasm (outside of the cell) to the cytosol (cellular interior)?
Flippases use ATP to permit membrane lipids to reorient themselves in the cellular membrane, specifically in the direction from extracellular to intracellular facing. Floppases catalyze the reverse movement: intracellular to extracellular. Migratases are not a class of enzyme. Phospholipases and kinases catalyze other types of reactions and certainly can act on lipids, but not this particular lipid movement.
Flippases use ATP to permit membrane lipids to reorient themselves in the cellular membrane, specifically in the direction from extracellular to intracellular facing. Floppases catalyze the reverse movement: intracellular to extracellular. Migratases are not a class of enzyme. Phospholipases and kinases catalyze other types of reactions and certainly can act on lipids, but not this particular lipid movement.
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Which of the following is an example of allosteric regulation of enzymes?
Which of the following is an example of allosteric regulation of enzymes?
The difference between the binding of cAMP and phosphorylation is that the latter is a covalent modification. Covalent modifications are a different way to regulate proteins, and do not fall under the category of allosteric regulation. Allosteric regulation only occurs outside of the active site, often simply called an allosteric site. The non-covalent binding of cAMP to a region of an enzyme outside of the active site thus qualifies as allosteric regulation.
The difference between the binding of cAMP and phosphorylation is that the latter is a covalent modification. Covalent modifications are a different way to regulate proteins, and do not fall under the category of allosteric regulation. Allosteric regulation only occurs outside of the active site, often simply called an allosteric site. The non-covalent binding of cAMP to a region of an enzyme outside of the active site thus qualifies as allosteric regulation.
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A researcher has designed a new type of inhibitor that binds at the active site of an enzyme. What type of inhibition does this molecule display?
A researcher has designed a new type of inhibitor that binds at the active site of an enzyme. What type of inhibition does this molecule display?
Because the inhibitor binds at the active site, it is actively competing with the ligand for access to the enzyme. This type of inhibitor displays competitive inhibition. Competitive inhibition can be overcome by adding excessive amounts of substrate. If the amount of substrate greatly out-measures the amount of inhibitor, then the substrate will still bind the enzyme very frequently and allow the reaction to proceed.
Noncompetitive inhibitors bind an enzyme at a spot that is not the active site. Uncompetitive inhibitors bind the enzyme-substrate complex, once the substrate has already entered the active site. Suicide inhibitors "kill" enzymes, typically by making permanent modifications to amino acids in the active site.
Because the inhibitor binds at the active site, it is actively competing with the ligand for access to the enzyme. This type of inhibitor displays competitive inhibition. Competitive inhibition can be overcome by adding excessive amounts of substrate. If the amount of substrate greatly out-measures the amount of inhibitor, then the substrate will still bind the enzyme very frequently and allow the reaction to proceed.
Noncompetitive inhibitors bind an enzyme at a spot that is not the active site. Uncompetitive inhibitors bind the enzyme-substrate complex, once the substrate has already entered the active site. Suicide inhibitors "kill" enzymes, typically by making permanent modifications to amino acids in the active site.
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Which of the following choices describes a way to graphically determine the type of inhibition being displayed by an inhibitor?
I. Plot initial reaction rate versus the concentration of substrate for the uninhibited enzyme, and then compare to the inhibited enzyme
II. Plot the inverse of the initial reaction rate versus the inverse of the substrate concentration for the uninhibited enzyme, and then compare to the inhibited enzyme
III. Plot the concentration of the inhibitor versus the concentration of substrate
Which of the following choices describes a way to graphically determine the type of inhibition being displayed by an inhibitor?
I. Plot initial reaction rate versus the concentration of substrate for the uninhibited enzyme, and then compare to the inhibited enzyme
II. Plot the inverse of the initial reaction rate versus the inverse of the substrate concentration for the uninhibited enzyme, and then compare to the inhibited enzyme
III. Plot the concentration of the inhibitor versus the concentration of substrate
Plotting the concentration of the inhibitor versus the concentration of the substrate will not give you any useful information because the reaction rate is essential in determining the type of inhibitor present.
Plotting initial reaction rate versus substrate concentration, or plotting the inverses, describes the graphical representation of Michaelis-Menten kinetics and a Lineweaver-Burk plot, respectively. Both of these are excellent methods to visually determine the type of inhibition displayed. On the graph, the line representing the inhibited enzyme will shift in predictable fashions depending on the type of inhibition.
Plotting the concentration of the inhibitor versus the concentration of the substrate will not give you any useful information because the reaction rate is essential in determining the type of inhibitor present.
Plotting initial reaction rate versus substrate concentration, or plotting the inverses, describes the graphical representation of Michaelis-Menten kinetics and a Lineweaver-Burk plot, respectively. Both of these are excellent methods to visually determine the type of inhibition displayed. On the graph, the line representing the inhibited enzyme will shift in predictable fashions depending on the type of inhibition.
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On a Lineweaver-Burk plot, an inhibited enzyme is shown to have a less negative x-intercept than the uninhibited enzyme, but the y-intercept remains the same. The type of inhibition displayed is __________ and the inhibited reaction has a __________ 
value.
On a Lineweaver-Burk plot, an inhibited enzyme is shown to have a less negative x-intercept than the uninhibited enzyme, but the y-intercept remains the same. The type of inhibition displayed is __________ and the inhibited reaction has a __________
The x-intercept on a Lineweaver-Burk plot tells us the negative reciprocal of 
.
Because the x-intercept is less negative, this tells us that the inhibited reaction has a larger 
. Having a different x-intercept but the same y-intercept is characteristic of competitive inhibition. The inhibitor and the substrate are competing for the same binding site.
The x-intercept on a Lineweaver-Burk plot tells us the negative reciprocal of
Because the x-intercept is less negative, this tells us that the inhibited reaction has a larger
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You have an enzyme solution and you add an inhibitor molecule and observe a marked decrease in enzyme activity. You increase the substrate concentration but this does not lead to any observable increase in enzyme activity. What can you conclude about your inhibitor?
You have an enzyme solution and you add an inhibitor molecule and observe a marked decrease in enzyme activity. You increase the substrate concentration but this does not lead to any observable increase in enzyme activity. What can you conclude about your inhibitor?
Noncompetitive inhibitors bind to enzymes away from the active site (allosteric) and distort it, reducing its affinity for substrate. Since they do not directly compete with substrate for enzyme binding, increasing the substrate concentration in the presence of a noncompetitive inhibitor will have no affect. While enzyme inhibitors include both organic and inorganic molecules, there is not enough information in the question stem to conclude the chemical classification of the inhibitor.
Noncompetitive inhibitors bind to enzymes away from the active site (allosteric) and distort it, reducing its affinity for substrate. Since they do not directly compete with substrate for enzyme binding, increasing the substrate concentration in the presence of a noncompetitive inhibitor will have no affect. While enzyme inhibitors include both organic and inorganic molecules, there is not enough information in the question stem to conclude the chemical classification of the inhibitor.
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How does a noncomeptitive inhibitor affect an enzyme?
How does a noncomeptitive inhibitor affect an enzyme?
A noncompetitive inhibitor acts to decrease how fast the enzyme can act on substrates. It accomplishes this by lowering the maximum rate at which it can create products. Noncompetitive inhibitors do not alter the enzyme's Michaelis constant.
A noncompetitive inhibitor acts to decrease how fast the enzyme can act on substrates. It accomplishes this by lowering the maximum rate at which it can create products. Noncompetitive inhibitors do not alter the enzyme's Michaelis constant.
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How do competitive inhibitors affect enzyme efficiency?
How do competitive inhibitors affect enzyme efficiency?
Competitive inhibitors can be overpowered by introducing excess substrate, so they do not affect the maximum rate of the enzyme. They do, however, make it so that more substrate is required in order to get the enzyme working at half of its maximum rate. As a result, competitive inhibitors act by raising the Michaelis constant of enzymes.
Competitive inhibitors can be overpowered by introducing excess substrate, so they do not affect the maximum rate of the enzyme. They do, however, make it so that more substrate is required in order to get the enzyme working at half of its maximum rate. As a result, competitive inhibitors act by raising the Michaelis constant of enzymes.
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Which of the following changes cannot be accomplished by an enzyme in a chemical reaction?
Which of the following changes cannot be accomplished by an enzyme in a chemical reaction?
An enzme is a biological catalyst that increases the rate of a reaction. This is accomplished by lowering the activation energy necessary to start the reaction. The equilibrium of the reaction, however, is not affected. This means that enthalpy and entropy are not affected by an enzyme's presence.
An enzme is a biological catalyst that increases the rate of a reaction. This is accomplished by lowering the activation energy necessary to start the reaction. The equilibrium of the reaction, however, is not affected. This means that enthalpy and entropy are not affected by an enzyme's presence.
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