Chapt. 8 Enzymes as catalysts - PowerPoint PPT Presentation

1 / 27

About This Presentation

Title:

Chapt. 8 Enzymes as catalysts

Description:

Chapt. 8 Enzymes as catalysts Ch. 8 Enzymes as catalysts Student Learning Outcomes: Explain general features of enzymes as catalysts: Substrate - Product – PowerPoint PPT presentation

Number of Views:374

Avg rating:3.0/5.0

Slides: 28

Provided by: Betz2

Category:

more less

Transcript and Presenter's Notes

Title: Chapt. 8 Enzymes as catalysts

1
Chapt. 8 Enzymes as catalysts

Ch. 8 Enzymes as catalysts
Student Learning Outcomes
Explain general features of enzymes as catalysts
Substrate -gt Product
Describe nature of catalytic sites
general mechanisms
Describe how enzymes lower activation energy of
reaction
Explain how drugs and toxins inhibit enzymes
Describe 6 categories of enzymes

2
Catalytic power of enzymes

Enzymes do not invent new reactions
Enzymes do not change possibility of reaction to
occur (energetics)
Enzymes increase the rate of reaction by factor
of 1011 or higher

Fig. 8.1 box of golfballs, effect of browning
enzyme
3
Enzymes catalyze reactions

Enzymes provide speed, specificity and
regulatory control to reactions
Enzymes are highly specific for biochemical
reaction catalyzed (and often particular
substrate)
Enzymes are usually proteins
(also some RNAs ribozymes)
E S ? ES binding substrate
ES ? EP substrate converted to bound product
EP ? E P release of product

4
Glucokinase is a typical enzyme

Glucokinase is typical enzyme
ATP D-glucose 6-phosphotransferase
Very specific for glucose
Not phosphorylate other hexoses
Only uses ATP, not other NTP
3D shape of enzyme critical for its function
(derived from aa sequence)

Fig. 8.2 glucokinase
5
A. Active site of enzyme

Enzyme active site does catalysis
Substrate binds cleft formed by aa of enzyme
Functional groups of enzyme, also cofactors bond
to substrate, perform the catalysis

Fig. 8.4
6
B. Binding site specificity

Substrate binding site is highly specific
Lock-and-key model 3D shape recognizes
substrate (hydrophobic, electrostatic, hydrogen
bonds)
Induced-fit model enzyme conformational change
after binding substrate
galactose differs from
glucose, needs separate
galactokinase

Fig. 8.5 glucokinase
7
Glucokinase conformational change

Conformation change of glucokinase on binding
glucose
Binding positions substrate to promote reactions
Large conformational change adjusts actin fold,
and facilitates ATP binding
Actin fold named for G-actin
(where first described Fig. 7.8)

Fig. 8.6 glucokinase (Yeast hexokinase)
8
Transition state complex

Energy Diagram substrates are activated to
react
Activation energy barrier to spontaneous
reaction
Enzyme lowers activation energy
Transition-state complex is stabilized by diverse
interactions

Fig. 8.7
9
Transition-state complex

Transition-state complex binds enzyme tightly
transition-state analogs are potent inhibitors
of enzymes (more than substrate analogs)
make prodrugs that convert to active analogs at
site of action
Abzymes catalytic antibodies that have aa in
variable region like active site of transition
enzyme
Artificial enzymes catalyze reaction
Ex. Abzyme to Cocaine esterase destroys cocaine
in body

10
II. Catalytic mechanism of chymotrypsin -
example enzyme

Chymotrypsin, serine protease, digestive enzyme
Hydrolyzes peptide bond (no reaction without
enzyme)
Serine forms covalent intermediate
Unstable oxyanion (O-) intermediate
Cleaved bond is
scissile bond

Fig. 8.8
11
B. Catalytic mechanism of chymotrypsin

1. Specificity of binding
Tyr, Phe, Trp on denatured proteins
Oxyanion tetrahedral intermediate
His57, Ser195, Asp
2. acyl-enzyme intermediate
3. Hydrolysis of acyl-enzyme intermediate

Fig. 8.9
12
Mechanism of chymotrypsin, cont.

3. Hydrolysis of acyl-enzyme intermediate
Released peptide product
Restores enzyme

Fig. 8.9
13
Energy diagram revisited with detail

Chymotrypsin reaction has several transitions
See several steps
Lower energy barrier to uncatalyzed

Fig. 8.10
14
III. Functional groups in catalysis

Functional groups in catalysis
All enzymes stabilize transition state by
electrostatic
Not all enzymes form covalent intermediates
Some enzymes use aa of active site (Table 1)
Ser, Lys, His - covalent links
His - acid-base catalysis
peptide backbone NH stabilize anion
Others use cofactors (nonprotein)
Coenzymes (assist, not active on own)
Metal ions (Mg2, Zn2, Fe2)
Metallocoenzymes (Fe2-heme)

15
Coenzymes assist catalysis

Activation-transfer coenzymes
Covalent bond to part of substrate enzyme
completes
Other part of coenzyme binds to the enzyme
Ex. Thiamine pyrophosphate is derived from
vitamin thiamine
works with many different enzymes
enzB takes H from TPP carbanion attacks keto
substrate, splits CO2

Fig. 8.11
16
Other activation-transfer coenzymes

Activation-transfer coenzymes
Specific chemical group binds enzyme
Other functional group participates directly in
reaction
Depends on enzyme for specificity of substrate,
catalysis

Fig. 8.12 A CoA forms thioesters with many acyl
groups acetyl, succinyl, fatty acids
17
Oxidation-reduction coenzymes

Oxidoreductase enzymes use other coenzymes
Oxidation is loss of electrons (loss H, or gain
O)
Reduction is gain electrons (gain H, loss of O)
Redox coenzymes do not form covalent bond to
substrate
Unique functional groups
NAD (and FAD) special
role for ATP generation
Ex. Lactate dehydrogenase
oxidizes lactate to pyruvate
transfers e- H to NAD
-gt NADH

Fig. 8.13 lactate dehydrogenase
18
Metal ions assist in catalysis

Positive metal ions attract electrons contribute
Mg2 often bind PO4, ATP ex. DNA polymerases
Some metals bind anionic substrates

Fig. 8.14
ADH alcohol dehydrogenase
oxidizes alcohol to acetaldehyde
and NAD to NADH
Zn2 assists with NAD
(In Lactate dehydrogenase, a His residue assisted
the reaction)

19
pH affects enzyme activity

Each enzyme has characteristic pH optimum
Depends on active-site amino acids
Depends on H bonds required for 3D structure
Each enzyme has optimum
temperature for activity
Humans 37oC
Taq polymerase
for PCR 72oC

Fig. 8.15 optimal pH for enzyme
20
V. Mechanism-based inhibitors

Inhibitors decrease rate of enzyme reaction
Mechanism-based inhibitors mimic or participate
in intermediate step of reaction
Covalent inhibitors
Transition-state analogs
Heavy metals

Fig. 8.2 organophosphate inhibitors include two
insecticides, and nerve gas Sarin
21
Covalent inhibitors

Covalent inhibitors form covalent or very tight
bonds with functional groups in active site

Fig. 8.16 DFP di-isopropylfluorophosphate
prevents acetylcholinesterase from degrading
acetylcholine
22
Transition state analogs

Transition-state analogs bind more tightly to
enzyme than substrate or product
Penicillin inhibits glycopeptidyl transferase,
enzyme that synthesizes cross-links in bacterial
cell wall.
Kills growing cells by inactivating enzyme

Fig. 8.17 penicillin
23
Allopurinol treats gout

Allopurinol is suicide inhibitor of xanthine
oxidase
Treatment for gout (decreases formation of
urate)

Fig. 8.18
24
Basic reactions and classes of enzymes

6 basic classes of enzymes
Oxidoreductases
Oxidation-reduction reactions (one gains, one
loses e-)
Transferases
Group transfer functional group from one to
another
Hydrolases cleave C-O, C-N and C-S bonds
addition of H2O in form of OH- and H
Lyases diverse cleave C-C, C-O, C-N
Isomerases rearrange, create isomers of starting
Ligases synthesize C-C, C-S, C-O and C-N bonds
Reactions often use cleavage of ATP or others

25
Some example enzymes

Example enzymes
Group transfer
transamination
transfer of amino group
Isomerase
rearranges atoms
ex. In glycolysis

Fig. 8.19
26
Key concepts

Enzymes are proteins (or RNA) that are catalysts
accelerate rate of reaction
Enzymes are very specific or substrate
Enzymes lower energy of activation to reach
high-energy intermediate state
Functional groups at active site (amino acid
residues, metals, coenzymes) cause catalysis
Mechanisms of catalysis include acid-base,
formation covalent intermediates, transition
state stabilization

27
Review questions