Difference between revisions of "Structure-based mutation analysis"

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==General==
 
==General==
According to the [http://www.uniprot.org/uniprot/Q30201#section_x-ref UniProt] entry about HFE_HUMAN are three 3D-structures of the HFE_HUMAN available, which are listed below. We have chosen the '1A6Z' because it has the best resolution, a very good R-Value (it measures the quality of the model obtained from the crystallographic data), a pH near the physiological optimum and is as good as complete. '1DE4' has a slightly better R-Value and pH, but this PDB also includes the transferrin receptor, which we do not need and do not want in our structure. '1C42' is only a hypothetical model, so we exclude it from further research.
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According to the [http://www.uniprot.org/uniprot/Q30201#section_x-ref UniProt] entry about HFE_HUMAN are three 3D-structures of the HFE_HUMAN available, which are listed below. We have chosen the '1A6Z' because it has the best resolution, a very good R-Value (it measures the quality of the model obtained from the crystallographic data), a pH near the physiological optimum and is as good as complete. '1DE4' has a slightly better R-Value and pH, but this PDB also includes the transferrin receptor, which we do not need and do not want in our structure. Also the missing residues of chain A are the same as in the structure '1A6Z' which are only the first three positions. '1C42' is only a hypothetical model, so we exclude it from further research.
   
 
[[Image:1a6z_properties.PNG|thumb|stereochemistrical properties of 1a6z]]
 
[[Image:1a6z_properties.PNG|thumb|stereochemistrical properties of 1a6z]]

Revision as of 12:47, 1 July 2011

General

According to the UniProt entry about HFE_HUMAN are three 3D-structures of the HFE_HUMAN available, which are listed below. We have chosen the '1A6Z' because it has the best resolution, a very good R-Value (it measures the quality of the model obtained from the crystallographic data), a pH near the physiological optimum and is as good as complete. '1DE4' has a slightly better R-Value and pH, but this PDB also includes the transferrin receptor, which we do not need and do not want in our structure. Also the missing residues of chain A are the same as in the structure '1A6Z' which are only the first three positions. '1C42' is only a hypothetical model, so we exclude it from further research.

stereochemistrical properties of 1a6z

All stereochemistrical properties of the structure are shown in the figure to the right<ref>Lebrón JA, Bennett MJ, Vaughn DE, Chirino AJ, Snow PM, Mintier GA, Feder JN, Bjorkman PJ.: Crystal structure of the hemochromatosis protein HFE and characterization of its interaction with transferrin receptor.</ref>.

PDB Method Resolution (Å) Chain R-Value R-Free pH Temperature Completeness Missing residues (Chain:pos)
1A6Z X-ray 2.60 A/C 0.233 0.277 6.5 -150.15°C (123 k) 98.0 A:1-3 C:1-3 - - - -
1C42 model - A - - - - - - - - - - -
1DE4 X-ray 2.80 A/D/G 0.231 0.265 8.0 -173.15°C (100 k) 94.3 A:1-3 C:121,757-760 D:1-3 F:121,757-760 G:1-3 I:121,757-760

Mapping

Because we have no annotation about the active site so we just visualized the mutations at the '1A6Z' structure. Secondly we are using the same mutations as in Task 6 and have therefore the same problemes with their visualization (only 7 of 10 visualizeable).

All mutations are scattered accross the protein with no affinity to some special region or secondary structure element. Mutations shown in red are near glycosylation positions and mutations in yellow are near disulfidbonds.

1A6ZA with 7 of 10 visualized mutations taken from task 6

SCWRL

SCWRL predicts protein side-chain confirmations given a fixed backbone. We are using SCWRL version 4 released in 2009.

Usage:

  • use only chain A of backbone pdb: 1A6ZA.pdb
  • extract amino acid sequence and change it to lowercase: aa.txt
  • introduce each mutation into on seperated aa_x.txt file as capital
  • cmd: scwrl -i 1A6ZA.pdb -s aa_x.txt -o ./mutant_pdbs/1A6ZA_mutant_x.pdb > ./mutant_pdbs/1A6ZA_mutant_x.txt

Results:

Robert: currently working.

Mutation Position Energy
M/T 35 252.324
S/C 65 246.695
I/T 105 250.833
Q/H 127 252.368
A/V 176 280.381
T/I 217 260.189
C/Y 282a 389.539
C/S 282b 255.859

Energy comparison

FoldX

FoldX scores the importance of amino acid interactions according to the overall stability of the protein and calculates the energy.

Usage:

  • create a runfile tutorial and adjust all default parameters to known (if possible): runfile.txt
  • create a listfile of all pdb files that should be included in energy calculation: listfile.txt
  • cmd: sudo ./foldx -runfile runfile.txt > output.txt

Results:

Robert: currently working.

Minimise

Minimise is able to minimise the energy of an model.

Usage:

  • remove all hydrogen and water atoms from the pdb files with repairPDB: 1A6ZA_mutant_x_clean.pdb
  • cmd: repairPDB 1A6ZA_mutant_x.pdb -nosol 1A6ZA_mutant_x_clean.pdb > 1A6ZA_mutant_x_clean.txt
  • cmd: minimise inputpdb outputfile

Results: Robert: currently working.

Gromacs

Has to be done!

References

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