Enzymes, Structure & Action

What Are Enzymes?

Enzymes are biological catalysts, proteins that speed up chemical reactions in living organisms without being consumed in the process. Virtually every metabolic reaction in cells requires an enzyme to proceed at a biologically useful rate.

Key Properties of Enzymes

Description

Speed up reactions without being used up

Each enzyme acts on specific substrates

Made of amino acid chains with 3D structure

Released unchanged after reaction

Can catalyse forward and reverse reactions

Significance

One enzyme molecule can catalyse thousands of reactions per second

Prevents unwanted side reactions; enables precise metabolic control

Structure determines function; sensitive to conditions affecting protein folding

Cells need only small amounts of each enzyme

Direction depends on substrate/product concentrations

The Catalytic Power of Enzymes

Enzymes can increase reaction rates by factors of 10⁶ to 10¹² compared to uncatalysed reactions. For example, the enzyme carbonic anhydrase converts CO₂ and H₂O to carbonic acid at a rate of 600,000 molecules per second, so fast that the reaction is essentially instantaneous in red blood cells.

Quick Check

Q: Why is it advantageous for cells to use enzymes rather than relying on heat or pressure to speed up reactions?

Enzyme Structure & The Active Site

Enzymes are globular proteins with a specific three-dimensional shape that is essential for their function. This shape is maintained by various bonds and interactions within the protein molecule.

Levels of Protein Structure in Enzymes

Primary structure: Linear sequence of amino acids linked by peptide bonds
Secondary structure: Local folding into α-helices and β-sheets, stabilised by hydrogen bonds
Tertiary structure: Overall 3D shape of the polypeptide, maintained by disulfide bridges, hydrogen bonds, ionic bonds, and hydrophobic interactions
Quaternary structure (some enzymes): Association of multiple polypeptide subunits (e.g., haemoglobin, DNA polymerase)

The Active Site

The active site is a specific region on the enzyme surface where substrate molecules bind and chemical transformation occurs. Key features include:

Specific pocket or cleft formed by the folding of the polypeptide chain
Complementary shape to the substrate molecule(s)
Specific amino acid residues that interact chemically with the substrate
Usually relatively small compared to the overall enzyme size (typically 3-12 amino acids)

The Importance of Tertiary Structure

The active site depends entirely on the correct tertiary structure of the enzyme. If this 3D shape is disrupted (denaturation), the active site is destroyed and the enzyme loses all catalytic activity, even though the primary structure (amino acid sequence) remains intact.

Cofactors and Coenzymes

Many enzymes require additional non-protein components to function:

Nature

Inorganic ions (metal ions)

Organic molecules (often vitamins)

Tightly bound cofactors/coenzymes

Examples

Zn²⁺ (carbonic anhydrase), Fe²⁺ (cytochromes), Mg²⁺ (DNA polymerase)

NAD⁺, FAD, coenzyme A, vitamins B1, B2, B3, B12

Haem group in catalase and peroxidase

Models of Enzyme Action

Two major models describe how enzymes interact with their substrates: the lock-and-key model and the induced fit model.

🔒 Lock-and-Key Model (1894)

Proposed by Emil Fischer, this model suggests that the active site has a rigid, pre-formed shape that exactly complements the substrate, like a lock and key.

Key points:

Active site shape is fixed
Only correctly shaped substrates fit
No change to enzyme structure during binding

🤲 Induced Fit Model (1958)

Proposed by Daniel Koshland, this model describes the active site as flexible, changing shape slightly to better fit the substrate upon binding.

Key points:

Active site is flexible and dynamic
Substrate binding induces conformational change
Better explains enzyme promiscuity and regulation

Modern Understanding

The induced fit model is now accepted as more accurate. Evidence from X-ray crystallography shows that enzymes do undergo conformational changes upon substrate binding. This flexibility is essential for:

Catalytic efficiency: Induced strain on substrate bonds lowers activation energy
Specificity: Only the correct substrate can induce the proper fit
Regulation: Allosteric modulators can bind away from the active site and affect its shape

HSC-Style Question

Q: Compare the lock-and-key and induced fit models of enzyme action. Explain why the induced fit model provides a better explanation of enzyme specificity. (4 marks)

The Enzyme Action Cycle

Enzyme-catalysed reactions follow a consistent cycle that can be summarised in several key steps:

Substrate binding: The substrate molecule(s) collide with the enzyme and bind to the active site, forming an enzyme-substrate (ES) complex. This involves weak interactions such as hydrogen bonds and ionic bonds.
Induced fit: The enzyme undergoes a conformational change that brings catalytic residues into optimal position and may place strain on substrate bonds.
Catalysis: The reaction occurs at the active site. The enzyme may facilitate the reaction by: (a) orienting substrates correctly, (b) straining substrate bonds, (c) providing a favourable microenvironment, or (d) participating directly in the reaction.
Product formation: The reaction reaches completion, converting substrate to product(s) within the enzyme-product (EP) complex.
Product release: The product(s) have lower affinity for the active site and are released, freeing the enzyme to bind another substrate molecule.

The Overall Reaction

E + S ⇌ ES → EP ⇌ E + P

Where E = enzyme, S = substrate, ES = enzyme-substrate complex, EP = enzyme-product complex, and P = product. The double arrows indicate that each step is reversible, though the overall direction depends on relative concentrations.

Activation Energy and the Transition State

Enzymes accelerate reactions by lowering the activation energy (Eₐ), the energy barrier that must be overcome for a reaction to proceed. They do this by:

Stabilising the transition state (the high-energy intermediate configuration)
Providing an alternative reaction pathway with lower Eₐ
Bringing reactants into close proximity and correct orientation

Key Point: Enzymes do NOT change the overall free energy change (ΔG) of a reaction, nor do they change the equilibrium position. They simply allow equilibrium to be reached faster by lowering the activation energy barrier.

Factors Affecting Enzyme Activity

Several environmental factors influence enzyme activity. Understanding these is crucial for both biological systems and industrial applications.

1. Temperature

As temperature increases, kinetic energy increases, leading to more frequent enzyme-substrate collisions
Rate approximately doubles for every 10°C rise (Q₁₀ ≈ 2), up to an optimum
Optimum temperature: Usually around 37°C for human enzymes (body temperature)
Above optimum: increased vibration disrupts weak bonds holding the tertiary structure; enzyme denatures
Thermophilic organisms have enzymes with higher optimum temperatures (e.g., 70-80°C)

2. pH

Affects ionisation of amino acid residues in the active site
Each enzyme has an optimum pH where activity is maximal
Most human enzymes: optimum pH ~7 (neutral), e.g., amylase in saliva
Pepsin (stomach): optimum pH ~2 (acidic environment)
Trypsin (small intestine): optimum pH ~8 (alkaline environment)
Extreme pH disrupts ionic bonds, causing denaturation

3. Substrate Concentration

At low [S], reaction rate is proportional to substrate concentration
As [S] increases, rate increases but progressively less
At high [S], rate plateaus, enzyme becomes saturated; all active sites occupied
Maximum rate = Vₘₐₓ; at half Vₘₐₓ, [S] = Kₘ (Michaelis constant, a measure of enzyme affinity)

4. Enzyme Concentration

Directly proportional to reaction rate (when substrate is not limiting)
More enzyme molecules = more active sites available

5. Inhibitors

Type	Mechanism	Effect	Example
Competitive	Reversible binding to active site	Competes with substrate; increased [S] can overcome	Malonate (inhibits succinate dehydrogenase)
Non-competitive	Binding to allosteric site	Changes enzyme shape; cannot be overcome by [S]	Cyanide (inhibits cytochrome oxidase)

Enzyme Denaturation

Denaturation is the irreversible loss of an enzyme's three-dimensional structure, resulting in loss of biological activity. Unlike inhibitors which temporarily block function, denaturation permanently destroys the active site.

⚠️ Causes of Denaturation

High temperature: Disrupts hydrogen bonds and hydrophobic interactions; thermal agitation exceeds bond strength
Extreme pH: Disrupts ionic bonds by changing charge states of amino acid side chains
Organic solvents: Disrupt hydrophobic interactions in the protein core
Heavy metal ions: Disrupt disulfide bonds (e.g., Hg²⁺, Pb²⁺, Ag⁺)
Detergents/surfactants: Disrupt hydrophobic interactions
High salt concentration: Can disrupt ionic bonds

Mechanism of Denaturation

Weak bonds maintaining tertiary structure are disrupted
Protein unfolds from its globular shape
The specific 3D shape of the active site is lost
Substrate can no longer bind effectively
Catalytic activity is abolished

Important Note on Reversibility

While most denaturation is irreversible, some enzymes can renature if conditions return to optimal before complete disruption. However, for HSC purposes, denaturation is generally considered irreversible. Ribonuclease is a classic example of an enzyme that can spontaneously renature when cooled.

Biological and Practical Significance

Example

High body temperature (>40°C)

Refrigeration, pasteurisation

Biological washing powders

PCR reactions

Application/Consequence

Can denature essential enzymes, leading to organ dysfunction

Low temperatures slow enzymes; high heat denatures microbial enzymes

Enzymes (lipases, proteases) work at moderate temperatures; hot water denatures them

Taq polymerase from thermophilic bacteria withstands high temperatures

Clinical & Industrial Applications

Understanding enzyme structure and function has led to numerous practical applications in medicine and industry.

Medical Applications

Enzyme Replacement Therapy

Lactase supplements: For lactose intolerance, oral lactase tablets provide the missing enzyme to digest dairy. Pancreatic enzyme replacement: For cystic fibrosis patients, pancreatic enzymes (lipase, protease, amylase) are given as medications.

Diagnostic Enzymes

Cardiac enzymes: Troponin, creatine kinase (CK-MB) are released during heart muscle damage, measured in blood tests for heart attack diagnosis. Liver enzymes: ALT, AST indicate liver damage when elevated.

Industrial Applications

Enzyme

Pectinase

Lactase

Amylase

Lipase, protease, amylase

Cellulase

DNA polymerase

Application

Clarifying fruit juices by breaking down pectin

Producing lactose-free milk

Breaking down starch in brewing and baking

Removing fat, protein, and starch stains

Stone-washing denim, softening fabrics

PCR for DNA amplification and analysis

HSC Connection

Q: Explain why enzymes used in biological washing powders work best at moderate temperatures (30-40°C) and why manufacturers warn against using very hot water. (3 marks)

Investigation: Effect of pH on Catalase Activity

This practical investigation explores how pH affects the activity of catalase, an enzyme that breaks down hydrogen peroxide into water and oxygen.

Background

Catalase is found in many living tissues, including liver and potato. It catalyses the decomposition of hydrogen peroxide (H₂O₂), a toxic byproduct of metabolism:

2H₂O₂ → 2H₂O + O₂

Materials

Fresh liver homogenate or potato extract (catalase source)
Hydrogen peroxide solution (3%)
Buffer solutions at pH 3, 5, 7, 9, 11
Test tubes, measuring cylinders, stopwatch
Gas syringe or inverted measuring cylinder for O₂ collection

Method

Add 5 mL of buffer solution to each of 5 test tubes (one for each pH)
Add 2 mL of liver homogenate to each tube and mix
Add 5 mL of H₂O₂ to each tube and immediately start timing
Measure oxygen production (volume of foam or gas collected) at 30-second intervals for 3 minutes
Record results in a table

Results Table

Rate of O₂ production (mL/min)

Relative enzyme activity

Discussion Questions

At which pH was enzyme activity highest? Why?
What happens to the enzyme at very low or very high pH?
Why is it important to use buffer solutions rather than simply adding acid or base?
How could you improve the reliability of your results?
What is the biological significance of catalase having an optimum pH around 7?

📝 Short Answer Questions

1. (3 marks) Describe the structure of an enzyme's active site and explain why the tertiary structure of the protein is essential for its function.

2. (4 marks) Explain how the induced fit model accounts for enzyme specificity, using the interaction between an enzyme and its substrate to illustrate your answer.

3. (5 marks) Describe the mechanism of enzyme denaturation and explain why high temperatures and extreme pH both result in loss of enzyme activity. Discuss the biological significance of this property.

4. (3 marks) Using your understanding of enzyme specificity, explain why people with lactose intolerance can often consume yoghurt without experiencing symptoms.

Clinical Scenario: Lactose Intolerance

🎯 Learning Intentions