Difference between revisions of "Structure-based mutation analysis BCKDHA"

Structure selection

The following table presents the PDB structures for BCKDHA to date:

The asteriks-marked values indicate that these structures were resolved with the asked experimental quality. As one can see, none of the structures fulfills all conditions.

Furthermode, we could not use any of the PDB structures for BCKDHA because all of them had gaps in the secondary structure which means that some residues were missing. So we took the structure which has the less gaps: 1U5B

• resultion: 1.83
  
• R-factor: 0.156
  
• ph-value: 5.8

This structure has to be modified with some programms to close the gaps. Additionally the first residues which are in BCKDHA misses in 1U5B thats why the start position corresponds to position 6 of the BCKDHA -PDB sequence.

As we can see none of the values corresponds to the demands because it was asked for a structure which has a very small R-factor, a pH of 7.4 and a high resolution.

Mapping of the mutations on the crystal structure

Structure of BCKDHA. Violet: mutations, orange: thiamine pyrophosphate binding sites, yellow: metal binding sites.

Showing hydrogen bonds with Pymol: A -> find -> polar contacts -> within selection The respective amino acids were colored by element, s.t. oxygen is red, nitrogen is blue, hydrogen is white and sulfur is yellow.

M82L

Hydrogen Bonds for methionine on pos 82 in the wild type structure

Hydrogen Bonds for leucine on pos 82 in the mutated type structure

Comparing the two figures for the wildtype and the mutated amino acid on position 82, no change in the hydrogen bonding network can be observed. This is due to the similar physiochemical properties of these two amino acids. No atom which could serve as additional hydrogen-bond donor or acceptor was introduced or removed.

Q125E

Hydrogen Bonds for glutamine on pos 125 in the wild type structure

Hydrogen Bonds for glutamic acid on pos 125 in the mutated type structure

The substitution from glutamine to glutamic acid changes the side chain properties completely. A NH2 group is substituted by a negatively charged oxygen. The NH2 which served in the wildtype structure as a hydrogen bond acceptor is not present any more, so the hydrogen bonding network changed for this substitution.

Y166N

Hydrogen Bonds for tyrosine on pos 166 in the wild type structure

Hydrogen Bonds for asparagine on pos 166 in the mutated type structure

Although tyrosine and asparagine both could play a role in the hydrogen bonding network, no hydrogen bond is formed for position 166. Therefore this substitution has no influence on the hydrogen bonding network of the protein.

G249S

Hydrogen Bonds for glycine 249 in the wild type structure

Hydrogen Bonds for serine on pos 249 in the mutated type structure

Introducing a serine on position 249 leads to the formation of several additional hydrogen bonds. Two of the newly established bonds are due to the new hydroxy group which is very likely to participate in hydrogen bonds. Another additional hydrogen bond is formed using the nitrogen atom as a hydrogen bond acceptor.

C264W

Hydrogen Bonds for cystein on pos 264 in the wild type structure

Hydrogen Bonds for tryptophan on pos 264 in the mutated type structure

R265W

Hydrogen Bonds for arginine on pos 265 in the wild type structure

Hydrogen Bonds for tryptophane on pos 265 in the mutated type structure

I326T

Hydrogen Bonds for isoleucine on pos 326 in the wild type structure

Hydrogen Bonds for threonine on pos 326 in the mutated type structure

F409C

Hydrogen Bonds for phenylalanine on pos 409 in the wild type structure

Hydrogen Bonds for cysteine on pos 409 in the mutated type structure

Y438N

Hydrogen Bonds for tyrosine on pos 438 in the wild type structure

Hydrogen Bonds for asparagine on pos 438 in the mutated type structure

Comparison energies

SCWRL

Before we could use SCWRL we first had to get the sequence of our model: repairPDB bckdha.pdb -seq >> bckdha.seq

When we have the sequence we have to make one file for each mutation. In these files we copied the bckdha.seq and changed the sequence to lower case letters. Then we add the mutation in an upper case letter.

To run SCWRL we used the command: scwrl -i bckdha.pdb -s mutation1.seq -o mutation1Model.pdb

Total minimal energy of the graph

foldX

To use foldX we first build a runscript. It is important to change values of <Temperature> and <pH> to the values of the used protein. These values can be found on the pdb side . Additionally we had to create one file with all PDB Ids each in a new line (list.txt). We used the command Foldx -runfile run.txt > Stout.txt to run the programm.

After using foldx we have the total energy for the wiltype protein and for each mutation. The value of the wildtype protein is 401.00 which is already a high value. This means that the protein is quite instabile. To find out which mutation has a high influence on the protein we look at the energies and especially on the difference between the energy of the mutated protein and the wildtype protein. All of the mutated proteins have a much higher energy than the unmutated protein which means that these proteins are less stable. We can see in the table that the proteins can be divided into two groups. The first group has an energy difference of about 31 and the other group has a much higher difference.

Minimise

It is important to remove the hydrogens and water before using the programm. For this we used the new version of repairPDB of the virtualbox. The programm can be started with the command: repairPDB bckdha.pdb -nosol out.pdb > Stout.txt
It is also possible to use the old version but then the command is: repairPDB bckdha.pdb -nosol -noh out.pdb > Stout.txt
It is useful to save the output in a file because it includes the energy.

Minimise calculates the energy for a mutation by building a new model for each mutation. And then it calculates the energy for the whole mutated model. To find out if there is a difference between the wildtype and the model that is calculated by Minimise. The aim by comparing the mutated models with the wildtype is to find out if there is a structural change caused by a mutation. We superposed each mutated protein with the wildtype and focused on the mutated position. In the pictures there are always the superposed structures. In the wildtype pictures the structure of the unmutated residue is bold and in the mutated pictures the structure of the mutated residue is bold. So we can compare the two pictures to see if there is a change in the structure caused by the mutation on this residue.

mutation	wildtype structure	mutated structure
M82L	wildtype	mutation M82L
Q125E	wildtype	mutation Q125E
Y166N	wildtype	mutation Y166N
G249S	wildtype	mutation G249S
C264W	wildtype	mutation C264W
R265W	wildtype	mutation R265W
I326T	wildtype	mutation I326T
F409C	wildtype	mutation F409C
Y438N	wildtype	mutation Y438N

Gromacs

The first part describes general background information for gromacs as well as how to run those programs. The second part contains the result description and analysis.

General

1. fetchpdb

The fetch-pdb script first checks, if it was called with an valid PDB-id. If the entered PDB code has 4letters, the script tries to download the pdb-file from the server. The successfully downloaded folder gets unzipped and everything except the actual pdb file is removed.

2. repairPDB

repairPDB bckdha_mod.pdb -noh -nosol > bckdha_clean.pdb

3. SCWRL

scwrl -i bckdha_mod.pdb -s extractedPDB.seq -o bckdha_scwrl.pdb

pdb including HEATOMS

4.pdb2gmx

use clean pdb without HEATOMS

pdb2gmx -f bckdha_clean.pdb -o bckdha.gro -p bckdha.top -water tip3p -ff amber03

5. MDP

6. grompp

grompp -v -f MDP_bckdha.mdp -c bckdha.gro -p bckdha.top -o bckdha.tpr

7. System Minimization

mdrun -v -deffnm bckdha 2> mdrun_out.txt

8. Analyzation

g_energy -f bckdha.edr -o energy_1.xvg

Analysis

Wildtype analysis: nsteps vs time

Wildtype analysis: force fields

The different force fields chosen for this task were:

• AMBER03

GROMACS Energy for the AMBER03 forcefield using the wildtype bckdha structure.

• CHARMM27

GROMACS Energy for the CHARMM27 forcefield using the wildtype bckdha structure.

• OPLS-AA

GROMACS Energy for the OPLS-AA forcefield using the wildtype bckdha structure.

Bond Analysis

Angle Analysis

Potential Analysis

Mutation analysis

M82L

Q125E

Y166N

G249S

C264W

R265W

I326T

F409C

Y438N

Links

go back to Maple syrup urine disease main page

go back to Task 6 Sequence based mutation analysis

go to Reference Sequence BCKDHA