Enzymes — MCQs
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Which of the following best describes the difference between glucokinase and hexokinase?
Enzymes that move a molecular group from one molecule to another are known as -
What are isoenzymes?
Aldehyde dehydrogenase requires NAD as ?
Selenocysteine is associated with ?
What are digestive enzymes classified as?
Type of inhibition of aconitase by trans-aconitate is?
What coenzyme is required by gulonate dehydrogenase for its activity?
Enzyme causing covalent bond cleavage without hydrolysis ?
Glucose oxidase converts glucose to?
Enzymes Indian Medical PG Practice Questions and MCQs
Question 531: Which of the following best describes the difference between glucokinase and hexokinase?
- A. Glucokinase has higher Km for glucose compared to hexokinase. (Correct Answer)
- B. Glucokinase is not inhibited by glucose-6-phosphate unlike hexokinase.
- C. Glucokinase has a low affinity for glucose.
- D. Glucokinase activity increases with glucose concentration while hexokinase remains saturated.
Explanation: ***Glucokinase has higher Km for glucose compared to hexokinase*** - **Glucokinase** has a **Km of ~10 mM** for glucose, while **hexokinase** has a **Km of ~0.1 mM**, making glucokinase's Km approximately **100-fold higher** - This **high Km** is the fundamental biochemical parameter that defines glucokinase's unique role as a **glucose sensor** in liver and pancreatic β-cells - The high Km means glucokinase activity is **proportional to blood glucose concentration** in the physiological range (5-15 mM), allowing it to regulate glucose metabolism in response to feeding - This is the **most precise biochemical descriptor** of the difference, from which other functional characteristics derive *Glucokinase has a low affinity for glucose* - While this statement is **correct** (high Km = low affinity), it is a **qualitative description** of what Km quantifies - Option stating "higher Km" is more specific and biochemically precise than simply stating "low affinity" *Glucokinase is not inhibited by glucose-6-phosphate unlike hexokinase* - This is a **correct and important regulatory difference** - **Hexokinase** is allosterically inhibited by its product **glucose-6-phosphate**, providing feedback regulation to prevent excessive glucose phosphorylation when cellular needs are met - **Glucokinase** lacks this product inhibition, allowing the liver to continue glucose uptake and storage even when G6P levels are high after meals - However, this describes a regulatory difference rather than the fundamental kinetic parameter *Glucokinase activity increases with glucose concentration while hexokinase remains saturated* - This statement is **correct** and describes the **functional consequence** of the different Km values - **Hexokinase** with its low Km (~0.1 mM) is saturated at normal blood glucose levels (5 mM), operating at Vmax - **Glucokinase** with its high Km (~10 mM) shows increasing activity as glucose rises from 5 to 15 mM postprandially - This is a physiological consequence rather than the fundamental biochemical parameter
Question 532: Enzymes that move a molecular group from one molecule to another are known as -
- A. Transferases (Correct Answer)
- B. Ligases
- C. Dipeptidases
- D. Oxido-reductases
Explanation: ***Transferases*** - **Transferases** are a class of enzymes that catalyze the transfer of a specific functional group (e.g., methyl, acetyl, phosphate) from one molecule (the donor) to another (the acceptor). - This broad category includes enzymes vital for many metabolic pathways, such as **kinases** (transferring phosphate groups) and **transaminases** (transferring amino groups). *Ligases* - **Ligases** are enzymes responsible for joining two large molecules together, typically by forming a new chemical bond. - This process usually involves the concomitant hydrolysis of a small, energy-rich molecule such as **ATP**, to provide the necessary energy for bond formation. *Dipeptidases* - **Dipeptidases** are a type of hydrolase enzyme that specifically cleaves the peptide bond within a **dipeptide**, releasing two free amino acids. - They are crucial for the final stages of protein digestion, breaking down small peptides into absorbable **amino acid units**. *Oxido-reductases* - **Oxido-reductases** are enzymes that catalyze **oxidation-reduction reactions** (redox reactions), where electrons are transferred from one molecule to another. - This class includes enzymes like **dehydrogenases** and **oxidases**, which play critical roles in cellular respiration and energy production.
Question 533: What are isoenzymes?
- A. Physically same forms of different enzymes
- B. Forms of same enzyme that catalyze different reactions
- C. Forms of different enzyme that catalyze same reactions
- D. Physically distinct forms of the same enzyme (Correct Answer)
Explanation: ***Physically distinct forms of the same enzyme*** - Isoenzymes are **multiple forms of an enzyme** that catalyze the **same reaction** but differ in their **physical or biochemical properties**, such as electrophoretic mobility, optimal pH, or kinetic parameters. - These differences usually arise from **genetic variations** (different genes encoding isoforms) or **post-translational modifications** (e.g., phosphorylation, glycosylation). *Physically same forms of different enzymes* - This statement is incorrect as isoenzymes are forms of the **same enzyme**, not different enzymes. - While different enzymes can catalyze similar reactions in certain pathways, they are not referred to as isoenzymes if they are structurally identical. *Forms of same enzyme that catalyze different reactions* - This describes enzymes with **broad substrate specificity** or those that act on different substrates but are not necessarily isoenzymes. - Isoenzymes specifically catalyze the **same chemical reaction**, but they may do so with different efficiencies or under different regulatory controls. *Forms of different enzyme that catalyze same reactions* - This describes a scenario where different enzymes might exhibit **catalytic promiscuity** or broad specificity, but not isoenzymes. - Isoenzymes are always derived from the **same parent enzyme** and catalyze the identical reaction.
Question 534: Aldehyde dehydrogenase requires NAD as ?
- A. None of the options
- B. Apoenzyme
- C. Coenzyme (Correct Answer)
- D. Cofactor
Explanation: ***Coenzyme*** - **NAD** (nicotinamide adenine dinucleotide) acts as a **coenzyme** for aldehyde dehydrogenase, serving as the **most specific and accurate classification** for its role. - As a coenzyme, **NAD** is an **organic, non-protein molecule** that binds reversibly to the enzyme and acts as a **transient carrier of electrons** (hydride ions, H⁻) during aldehyde oxidation. - **NAD⁺** accepts electrons from the aldehyde substrate, becoming reduced to **NADH**, which then dissociates and transfers electrons elsewhere in metabolism. - This is the **preferred answer** because coenzyme precisely describes NAD's organic nature, vitamin origin (niacin/B3), and its role as a mobile electron carrier. *Cofactor* - While technically **NAD is a type of cofactor** (cofactors include coenzymes, prosthetic groups, and metal ions), this term is **too general** for this context. - In biochemistry nomenclature, when both a general and specific term apply, the **more specific term (coenzyme) is preferred** to demonstrate precise understanding. - Choosing "cofactor" would be like calling a "cardiologist" a "doctor" - true but less specific. *Apoenzyme* - An **apoenzyme** is the **protein component** of an enzyme without its cofactor - it refers to the enzyme itself, not to NAD. - In this case, **aldehyde dehydrogenase** (the protein) is the apoenzyme, and **NAD** is the coenzyme that binds to it. - Together they form the active **holoenzyme** (apoenzyme + coenzyme = holoenzyme). *None of the options* - Incorrect because **coenzyme** is the accurate and specific term for NAD's role in aldehyde dehydrogenase function.
Question 535: Selenocysteine is associated with ?
- A. Carbonic anhydrase
- B. Catalase
- C. Transferase
- D. Deiodinase (Correct Answer)
Explanation: ***Deiodinase*** - Selenocysteine is a critical component of **iodothyronine deiodinases**, a family of enzymes that regulate **thyroid hormone metabolism**. - These enzymes catalyze the removal of iodine from thyroid hormones, converting **thyroxine (T4)** into the more active **triiodothyronine (T3)** or inactive forms. *Carbonic anhydrase* - This enzyme contains **zinc** as its essential metal cofactor and is involved in the interconversion of **carbon dioxide** and **bicarbonate**. - Its primary role is in pH regulation and CO2 transport, without any direct association with selenocysteine. *Catalase* - Catalase is an enzyme primarily found in **peroxisomes** and contains **iron-porphyrin** groups as its prosthetic group. - Its function is to convert **hydrogen peroxide** into water and oxygen, protecting cells from oxidative damage. *Transferase* - Transferases are a broad class of enzymes that catalyze the transfer of **functional groups** (e.g., methyl, glucose) from one molecule to another. - While essential for many metabolic processes, there is no inherent association of the general class of transferases with selenocysteine.
Question 536: What are digestive enzymes classified as?
- A. Hydrolases (Correct Answer)
- B. Oxidoreductases
- C. Transferases
- D. Ligases
Explanation: ***Hydrolases*** - Digestive enzymes like **amylase**, **lipase**, and **proteases** break down complex food molecules by adding water, a process known as **hydrolysis**. - This class of enzymes catalyzes the cleavage of a chemical bond with the concurrent addition of a water molecule. - All major digestive enzymes belong to this class according to the **EC enzyme classification system**. *Oxidoreductases* - These enzymes catalyze **redox reactions**, involving the transfer of electrons from one molecule to another. - Examples include **dehydrogenases** and **oxidases**, which are not primarily involved in breaking down food molecules in digestion. *Transferases* - Transferases catalyze the transfer of functional groups (such as methyl, acyl, or phosphate groups) from one molecule to another. - Examples include **kinases** and **transaminases**, which are involved in metabolic pathways but not in the digestive breakdown of food. *Ligases* - Ligases are enzymes that catalyze the joining of two large molecules by forming a new chemical bond, typically with the concomitant hydrolysis of ATP. - They are involved in **DNA repair** and **biosynthetic reactions**, not in the breakdown of food during digestion.
Question 537: Type of inhibition of aconitase by trans-aconitate is?
- A. Competitive (Correct Answer)
- B. Non-competitive
- C. Allosteric
- D. None of the options
Explanation: ***Competitive*** - **Competitive inhibition** occurs when the inhibitor (trans-aconitate) structurally resembles the enzyme's natural substrate (cis-aconitate) and binds to the **active site**, preventing the substrate from binding. - This type of inhibition can be overcome by increasing the concentration of the **substrate**. *Non-competitive* - **Non-competitive inhibitors** bind to a site on the enzyme other than the active site, causing a conformational change that reduces the enzyme's efficiency, regardless of substrate concentration. - Trans-aconitate's structural similarity to aconitate's substrate points away from a non-competitive mechanism. *Allosteric* - **Allosteric inhibition** involves an inhibitor binding to a regulatory site (allosteric site) on the enzyme, which is distinct from the active site, to alter enzyme activity. - While allosteric regulation is a type of non-competitive inhibition, trans-aconitate's direct structural resemblance to the substrate makes competitive inhibition the more specific and accurate description. *None of the options* - This option is incorrect because **competitive inhibition** accurately describes the mechanism by which trans-aconitate inhibits aconitase, given its structural similarity to the natural substrate. - The other options are less fitting due to the specific characteristics of trans-aconitate's action.
Question 538: What coenzyme is required by gulonate dehydrogenase for its activity?
- A. FAD
- B. FMN
- C. NADP
- D. NAD (Correct Answer)
Explanation: ***NAD*** - **Gulonate dehydrogenase** is an enzyme involved in the **uronic acid pathway**, specifically in the conversion of **L-gulonate to D-xylulose**. - This reaction is an **NAD-dependent oxidation**, meaning **NAD** acts as the electron acceptor, being reduced to **NADH**. *NADP* - **NADP** (nicotinamide adenine dinucleotide phosphate) is primarily involved in **anabolic pathways** like **fatty acid synthesis** and the **pentose phosphate pathway**, often in reduction reactions where it is converted to **NADPH**. - While structurally similar to NAD, it is generally not the direct coenzyme for gulonate dehydrogenase. *FAD* - **FAD** (flavin adenine dinucleotide) is a coenzyme derived from **riboflavin** (vitamin B2) and is typically involved in **redox reactions** where it repeatedly accepts and donates electrons, often in dehydrogenase reactions involving **carbon-carbon double bonds**. - Enzymes like **succinate dehydrogenase** (in the citric acid cycle) or acyl-CoA dehydrogenase (in fatty acid oxidation) utilize FAD, but not gulonate dehydrogenase. *FMN* - **FMN** (flavin mononucleotide) is another coenzyme derived from **riboflavin** and serves as a prosthetic group in various **flavoproteins**, often facilitating **single-electron transfers**. - It is frequently found in complexes like **NADH dehydrogenase** (Complex I of the electron transport chain) but is not the required coenzyme for gulonate dehydrogenase activity.
Question 539: Enzyme causing covalent bond cleavage without hydrolysis ?
- A. Lyase (Correct Answer)
- B. Ligase
- C. Hydrolase
- D. Transferase
Explanation: ***Lyase*** - **Lyases** are enzymes that catalyze the cleavage of **covalent bonds** (C-C, C-O, C-N, and others) by means other than hydrolysis or oxidation, often creating a new double bond or a ring structure. - They remove groups from substrates to form double bonds, or conversely, add groups to double bonds. - **Examples:** Aldolase (cleaves C-C bonds in glycolysis), carbonic anhydrase (reversible cleavage of C-O bond), fumarase (C-C bond cleavage in TCA cycle). *Ligase* - **Ligases** are enzymes that join two large molecules by forming a new chemical bond, usually accompanied by the **hydrolysis of ATP**. - They are involved in synthesis reactions, not the cleavage of bonds. *Hydrolase* - **Hydrolases** specifically catalyze the hydrolysis of a chemical bond, involving the **addition of water** across the bond. - They break down large molecules into smaller ones using water - this is the key difference from lyases. *Transferase* - **Transferases** catalyze the transfer of a **functional group** from one molecule (the donor) to another (the acceptor). - They do not cause covalent bond cleavage without hydrolysis but rather move existing groups between molecules.
Question 540: Glucose oxidase converts glucose to?
- A. Glucuronic acid
- B. Galactonic acid
- C. Gluconic acid (Correct Answer)
- D. Iduronic acid
Explanation: ***Gluconic acid*** - **Glucose oxidase** specifically catalyzes the oxidation of glucose, producing **gluconic acid** and hydrogen peroxide. - This reaction forms the basis for many common **glucose diagnostic tests**, such as those used in blood glucose monitors. *Glucuronic acid* - **Glucuronic acid** is formed from the oxidation of glucose at carbon 6, typically through the **uronic acid pathway**. - It is known for its role in **detoxification** and conjugation reactions in the liver, not as a direct product of glucose oxidase. *Galactonic acid* - **Galactonic acid** is an oxidized form of galactose, a different monosaccharide from glucose. - Its formation is not associated with the action of **glucose oxidase**, an enzyme specific to glucose. *Iduronic acid* - **Iduronic acid** is a C5 epimer of glucuronic acid and is a common component of various **glycosaminoglycans** like dermatan sulfate and heparan sulfate. - It is not produced by the action of **glucose oxidase** on glucose.
Practice by Chapter
Enzyme Classification and Nomenclature
Practice Questions
Enzyme Kinetics and Michaelis-Menten Equation
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Enzyme Inhibition: Competitive and Non-competitive
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Allosteric Regulation
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Coenzymes and Cofactors
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Isoenzymes and Clinical Significance
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Enzyme Regulation: Covalent Modification
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Enzyme Regulation: Zymogen Activation
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Enzyme Induction and Repression
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Ribozymes and Catalytic RNA
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Enzyme Diagnostic Applications
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Enzyme Therapy and Inhibitors as Drugs
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