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Transcript
Structure and Mechanism II:
Ribonuclease A
Frazer Li
Outline
Introduction
– Some history of RNase A
– As well as the Function and Structure
Folding and Stability
– How RNase A binds to RNA
The Reaction Mechanism
Reaction Energetics and Homologues
Conclusion
History
Ribonucleolytic activity in the pancreas of ruminants is
high
– possibly to digest large amount of RNA produced by stomach
microorganisms.
This high level of activity has led to the discovery of
Ribonuclease A
RNase A is the first enzyme and third protein to have a
correct amino acid sequence
Was first crystallized over 50 years ago.
History
A variety of methods were used to determine the structure
of RNase A
1) Fast atom bombardment mass spectrometry
(FABMS) - assigns disulfide bonds of
a protein with RNase A.
2) Work on RNase A has yielded the first 3D
structure of a protein containing an
isoaspartyl residue, derived from
deamidation of an asparagine residue (Asn 67)
3) NMR spectroscopy in elaborating both protein
structure and protein folding pathways.
Function
2 Classes of enzyme that catalyze the synthesis or
degradation of RNA:
1) RNA polymerase – synthesis
2) RNA depolymerases or “ribonucleases” – degradation
RNase A has been the object of landmark work on the
folding stability and chemistry of proteins in enzymology
and in molecular evolution
RNA essential for life!
Structure
The size of RNase A is small
- Has 124 amino acid residues
- Contains 19 of the 20 natural amino acids, lacking only tryptophan
Has similar shape to a kidney with active site residues lying in the
cleft
Structure
Long four-stranded antiparallel β-sheet and three short α-helixes
- Cross-linked by four disulfide bonds involving all eight of its
cysteine residues
- peptide bonds preceding two of the four proline residues are in
the cis conformation
Folding and Stability
Four disulfide bonds:
– critical to stability on native enzyme
– more stability from Cys26-Cys84 and Cys58-Cys110 than from
Cys65-Cys72 and Cys40-Cys95 -two proline residues with cis
peptide bonds
The stability of RNase A is legendary
The two proline residues with cis peptide bonds, and the
three residues most important for catalysis is His12,
His119, and Lys41
RNA Binding
SUBSITES
B1, B2, and B3 interact with
the bases of a bound substrate
The B1 subsite bind only
pyrimidine bases
(demonstrates an
approximately 30-fold kinetic
preference for cytosinecontaining versus uracilcontaining substrates)
The B2 and B3 subsites bind
all bases, but B2 has a
preference for an adenine
base
B3 has a preference for a
purine base
RNA Binding
SUBSITES
Three other enzymic subsites
(P0, P1, and P2) interact with
the phosphoryl groups of a
bound substrate
The enzyme catalyzes the
cleavage of the P-O bond of a
phosphoryl group bound in the
P1 subsite, which is the active
site
RNA Binding
SUBSTRATE SPECIFICITY
RNase A catalyzes the cleavage of the P-O bond of an RNA strand
and the hydrolysis of the P-O bond of a nucleoside 2’,3’-cyclic
phosphodiester on the 3’-side of a pyrimidine residue
ONE-DIMENSIONAL DIFFUSION
The abilitiy to diffuse in one dimension can accelerate the formation
of a site-specific interaction within a linear biopolymer by up to 103fold.
Such facilitated diffusion is used by transcription factors and
restriction endonucleases to locate specific sites on double-stranded
DNA
Specifically, a uridine nucleotide is cleaved more quickly by RNase A
if it is flanked by a long stretch of poly(dA) than if it is flanked by a
short stretch
RNA Binding
PROCESSIVE CATALYSIS
In contrast, “processive” enzymes bind a polymeric substrate and
catalyze a series of identical chemical reactions along that polymer
before releasing it to solvent
For a substrate to be acted on processively, it must contain a
repeating structural motif
Reaction Mechanism
IT IS A GENERAL ACID-BASE
CATALYSIS
The side chain of His12 acts as a
base that abstracts a proton from
the 2’-oxygen of a substrate
molecule, and thereby facilitates
its attack on the phosphorus
atom
This attack displace a nucleoside
His119 acts as an acid that
protonates the 5’’-oxygen to
facilitate its displacement
Both products are released to
solvent
The side chain of Lys41 and the
main chain of Phe120 enhance
catalysis by stabilizing this
transition state
Reaction Mechanism
RNase A catalyze hydrolysis of RNA by a two-step process with the
intermediate formation of a 2’,3’-cyclic nucleotide
Important Residues for Catalysis
His12 and His 119
Only one histidine residue is alkylated in each molecule of RNase A.
The rate of the single enzymic carboxymethylation is nearly 104-fold
greater than that of free histidine
The alkylation, which causes a marked decrease in catalytic activity,
modifies only His12 or His119
Catalysis by RNase A has a classic bell-shaped pH rate profile
This profile is consistent with a mechanism that involves two
titratable residues, one protonated and the other unprotonated
Important Residues for Catalysis
His12 and His119
Eliminating the imidazole group of His12 decreases the affinity of the
enzyme for this transition state by 104-fold during cleavage of poly(C), UpA,
and UpOC6H4-p-NO2
Eliminating the imidazole group of His 119 decreased this affinity by 104-fold
during cleavage of UpA.
Therefore, the value of the imidazole group of His 119 to catalysis depends
on the pKa of the conjugate acid of the leaving groups
– pKa of CH3OCH2CH2OH is 14.8
– pKa of UpOC6H4-p-NO2 is 7.14
– Thus, the contribution of His119 to catalysis decreases when the pKa of the
conjugate acid of the leaving group decreases
His119 is proposed to both protonate a nonbridging oxygen of the
phosphate anion and deprotonate this same oxygen in the phosphorane
intermediate
Important Residues for Catalysis
Lys41
Lys41 contributes to catalytic
activity
– When Lys41 is replaced by an
arginine residue, the variant have
approximately 2% of the activity of
the wild-type enzyme in hydrolysis
Catalytic role of Lys41 is to
stabilize the excess negative
charge that accumulates on the
nonbridging phosphoryl oxygens
in transition state during RNA
cleavage
– Stabilized by Coulombic
interactions
– By short, strong hydrogen bond
involving the partial transfer of a
proton from Lys41
Lys41 is also used to donate a
single hydrogen bond to the
transition state during catalysis
Reaction Energetics
RNase catalyzes Exergonic reactions
Catalyzes both the reverse of transphosphorylation and hydrolysis
2’,3’-cyclic phosphodiester intermediate and hydrolysis of this cyclic
intermediate to form a 3’-phosphomonoester
NMR spectroscopy was used to monitor how this cyclic intermediate
accumulates during catalysis by RNase A and small molecules
The cyclic intermidiate does not accumulate during catalysis by hydroxide
ion or imidazole buffer
In the presence of these small-molecule catalysts, hydrolysis of the cyclic
intermediate is faster than transphosphorylation of RNA
These results suggest that RNase A has evolved primarily to catalyze
transphosphorylation rather than hydrolysis
Reaction Energetics
Therefore, RNase A is referred to RNA depolymerase
The imidazole group of His12 acts as a base in the transphosphorylation
reaction and an acid in the hydrolysis reaction
The imidazole group of His 119 has complementary role, acting as an acid
in the trasphosphorylation reaction and a base in the hydrolysis reaction
After catalysis of transphosphorylation, each histidine residue in the active
site of RNase A is protonated appropriately to catalyze hydrolysis of the
bound cyclic intermediate
RNase A short-curcuits this cycle by releasing rather than hydrolyzing the
cyclic intermediate.
Thus, RNase A has an iso mechanism in which the protonation states of the
unliganded enzyme are interconverted by a pathway that does not involve
substrate molecules
Reaction Energetics
RATE ENHANCEMENT
Replacing Lys41 with an alanine residue removes a potential
hydrogen-bond donor from the active site of RNase A
Enhances Catalysis
Similarly, replacing His12 or His119 the base and acid in catalysis
slows catalysis by 104 to 105 fold
B2 subsite provides a 104-fold rate acceleration
Homologues
Humans contain at least five homologues of RNase A
–
–
–
–
–
RNase 1 which is from human pancrease
RNase 4 which is from human liver are distinct enzymes
Angiogenin is a plasma enzyme that promotes neovasculariztion
Eosinopholic leukocytes contain RNase 2, which is neurotoxic
RNase 3 which has helinthotoxic and antibacterial activities
Conclusion
RNase A has been the most studied enzyme of the 20th century
Used to digest RNA produced by stomach microorganisms
Methods now exist to produce unlimited quantities of RNase A and
it’s homologues
Can be used to exploit further use of RNase A in biotechnology and
medicine
RNase A will continue to be used as a model system