Difference between revisions of "Predicting the Effect of SNPs (PKU)"

Short Introduction

This week's task builds on the data gathered last week. We blindly choose 5 disease causing and 5 harmless SNPs and will try to predict their effect from the sequence change alone. You may find a detailed task description at the usual place and consult our task journal.

Our dataset

we propose the following dataset:

• GLU76GLY
• SER87ARG
• ARG158GLN
• GLN172HIS
• ARG243GLN
• LEU255SER
• MET276VAL
• ALA322GLY
• GLY337VAL
• ARG408TRP

You could check them, if you like.. I put them together 5 minutes ago and already forgot, which are which. ;-)

Investigated SNPS

In the following section, we present the information we gathered for each SNP individually. Summary comments on the methods we used, we placed at subsites. These include the PsiBlast Profile of our protein, PsiPred Predictions of the mutated sequences, the complete Alignment of 22 mammalian homologs to PAH and the SIFT, PolyPhen and SNAP predictions, but the conclusions are repeated below.

GLU76GLY

Prediction:

As this mutation results in a change from glutamic acid to glycine which have some differences in structure as can bee seen in <xr id="fig:mutationGLUGLY"/> we expect this change to be of rather minor effect. Of course glutamic acid is charged under biological conditions and glycine is not, but glycine could be a universal substitution, because it is neither hydrophobic nor hydrophilic. Additionally, as it is the smallest amino acid, it can not produce any sterical problems. Of course it might be that the glycine can not stabilize any structure, which should be present at this residue.We do not have any structural data for this point, but predictions suggest a position either in a helix or at the edge of a sheet structure. We only can rely on the physiochemical properties, for which we would say, that these changes are not drastic enough to cause the disease. If the mutation would have occurred rather near the catalytic site, our judgment would have been different with respect to the strong affinity of glutamic acid to ions, which plays a major role in PheOH-activity.

• Amino acid changes: [From negativly charged, polar, strongly hydrophilic, medium sized to neutral, non-polar, non-hydrophilic, small]
• BLOSUM62/PAM250/PAM1: -2(-4,+6)/9 (0,12)/4 (0,9865)
• PSSM: conserved
• Alignment of homologs: some variability
• SIFT: TOLERATED with a score of 0.18.
• PolyPhen: Benign
• SNAP: Non-neutral (low reliability)

<figure id="fig:mutationGLUGLY">

</figure>

2D structure projection of glutamic acid with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

2D structure projection of glycine with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

SER87ARG

Prediction

We expect that this mutation, which causes a change from serine to arginine, has a bigger effect on the protein, than the one above. With this mutation the strength of the effect depends completely on the location of the amino acid. Both of the amino acids are hydrophilic, but as arginine is one of the snorkeling, because of its rather hydrophobic stem, the changes can be rather serious(<xr id="fig:mutationSERARG"/>). It is predicted to be two positions N-terminal of a helix structure. As the overall change of size and the change in polarity from rather negative to positive and regarding the fact, that arginine is a rather seldom used amino acid (mostly appearing in the catalytic domain for phosphorylated substrates), we would say, that this is rather a disease causing mutation.

• Amino acid changes: [From neutral, polar, slightly hydrophilic to pos. charged, polar, strongly hydrophilic]
• BLOSUM62/PAM250/PAM1: 1(-3,+4)/11 (1,10(sic!))/6 (1,9840)
• PSSM: residue change appears often
• Alignment of homologs: some variability
• SIFT: TOLERATED with a score of 0.54.
• PolyPhen: Benign
• SNAP: Non-neutral (low reliability)

<figure id="fig:mutationSERARG">

</figure>

2D structure projection of serine with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

2D structure projection of arginine with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

ARG158GLN

Prediction:

From the secondary structure of both amino acids (<xr id="fig:mutationSERARG"/> left side), one would guess, that if an Arginine fits in this region, a Glutamine will fit there as well. But if one looks at the right side of this figure, in the close-up there are some small red discs, which indicate sterical collisions. These are due to the additional hydroxl-group, where the original amino acid only had hydrogen-atoms. Depending on the importance of this site and the collision's this mutation can have almost no or a very big effect. But since the sidechain collides in the inside of the protein, we would predict a rather serious effect.

• Amino acid changes: [From pos. charged, polar, strongly hydrophilic to neutral, polar, strongly hydrophilic]
• BLOSUM62/PAM250/PAM1: 1(-3,+5)/5 (1,17)/9 (0,9913)
• PSSM: residue change appears often
• Alignment of homologs: some variability
• SIFT: AFFECT PROTEIN FUNCTION with a score of 0.00.
• PolyPhen: Probably Damaging
• SNAP: Non-neutral (high reliability)

<figure id="fig:mutationSERARG">

</figure>

2D structure projection of Arginine with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

2D structure projection of Glutamine with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

Close-up of the mutated Glutamine at residue 158 in PheOH. The best fitting rotamer was chosen to minimize severe or smaller collisions (red to green discs) with neighboring residues. This rotamer appears in 1.7% of mutations according to the PyMol rotamer database.

Mutated Glutamine at residue 158 in PheOH. The residue is located in a helix region.

GLN172HIS

Prediction: This mutation is rather easy on the first sight. The general chemical properties are the same. The amino acids only differ in size and structure. As one can see in <xr id="mutationGLNHIS"/> on the right, there are some collisions with the structure. But due to the fact, that this amino acid is located on the outside of the protein and also located in a coiled region which only interferes with another coiled region, we are quite sure, that this mutation is not disease causing.

• Amino acid changes: [From neutral, polar, strongly hydrophilic to neutral, polar, strongly hydrophilic, ring-structure]
• BLOSUM62/PAM250/PAM1: 0(-3,+5)/7 (0,10)/23 (0,9876)
• PSSM: residue change appears often
• Alignment of homologs: highly conserved
• SIFT: AFFECT PROTEIN FUNCTION with a score of 0.03.
• PolyPhen: Benign
• SNAP: Neutral (high reliability)

<figure id="mutationGLNHIS">

</figure>

2D structure projection of glutamine with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

2D structure projection of histidine with the pK-values for each group. For a better referability the c-atoms are labeled according to the common nomenclature

Close-up of the mutated histidine at residue 172 in PheOH. The best fitting rotamer was chosen to minimize severe or smaller collisions (red to green discs) with neighboring residues. This rotamer appears in 18.9% of mutations according to the PyMol rotamer database.

Mutated histidine at residue 172 in PheOH. The residue is located in a coil region.

ARG243GLN

Prediction:

• Amino acid changes: From pos. charged, polar, strongly hydrophilic to neutral, polar, strongly hydrophilic.
• BLOSUM62/PAM250/PAM1: 1(-3,+5)/5 (1,17)/9 (0,9913)
• PSSM: conserved
• Alignment of homologs: highly conserved
• SIFT: AFFECT PROTEIN FUNCTION with a score of 0.00.
• PolyPhen: Probably damaging
• SNAP: Non-neutral (medium reliability)

<figure id="fig:mutationARG243GLN">

</figure>

Close-up of the mutated histidine at residue 243 in PheOH. The best fitting rotamer was chosen to minimize severe or smaller collisions (red to green discs) with neighbouring residues. This rotamer appears in 17.3% of mutations according to the PyMol rotamer database.

Mutated glutamine at residue 243 in PheOH. The residue is located in a sheet region.

LEU255SER

Prediction:

• Amino acid changes: From neutral, non polar, strongly hydrophobic to neutral, polar, slightly hydrophilic.
• BLOSUM62/PAM250/PAM1: -2(-4,+4)/4 (1,34)
• PSSM: position variable
• Alignment of homologs: highly conserved
• SIFT: AFFECT PROTEIN FUNCTION with a score of 0.00.
• PolyPhen: Probably damaging
• SNAP: Non-neutral (low reliability)

<figure id="fig:mutationLEU25SER">

Close-up of the mutated serine at residue 255 in PheOH. The best fitting rotamer was chosen to minimize severe or smaller collisions (red to green discs) with neighbouring residues. This rotamer appears in 42.9% of mutations according to the PyMol rotamer database.

Mutated serine at residue 255 in PheOH. The residue is located in a helix structure.

</figure>

MET276VAL

Prediction:

This mutation is located in a coil region at the outside of the protein (see <xr id="fig:mutationMET276VAL" />) and while the introduced valine is more hydrophobic than the previous methionine, the location of the residue appears to be uncritical enough for this mutation to have no effect on the protein structure. Indeed, the PSSM shows, that the mismatch valine is observed more often than the match methionine. The prediction methods agree for once and we also think this mutation to be likely not disease causing.

• Amino acid changes: From neutral, non-polar, hydrophobic to neutral, non-polar, strongly hydrophobic.
• BLOSUM62/PAM250/PAM1: neutral replacement
• PSSM: residue change appears often
• Alignment of homologs: highly conserved
• SIFT: TOLERATED with a score of 0.06.
• PolyPhen : Benign
• SNAP: Neutral (low reliability)

<figure id="fig:mutationMET276VAL">

Close-up of the mutated valine at residue 276 in PheOH. The best fitting rotamer was chosen to minimize severe or smaller collisions (red to green discs) with neighbouring residues. This rotamer appears in 94.5% of mutations according to the PyMol rotamer database.

Mutated valine at residue 276 in PheOH. The residue is located in a coil.

</figure>

ALA322GLY

Prediction:

While this residue is highly conserved in the mammalian analogs and in the PSSM, the replacement of alanine with glycine within the helix visible in <xr id="fig:mutationALA322GLY" /> appears possible. Both are small, non-polar amino acids allowed in helix formation and the now missing methyl group of alanine is unlikely to have a large effect on residues outside the helix. The prediction methods disagree again, but we judge this mutation to be neutral.

• Amino acid changes: From neutral, non-polar, hydrophobic, small to neutral, non-polar, slightly hydrophilic, small.
• BLOSUM62/PAM250/PAM1: good replacement
• PSSM: conserved
• Alignment of homologs: highly conserved
• SIFT: AFFECT PROTEIN FUNCTION with a score of 0.01.
• PolyPhen: Possibily damaging
• SNAP: Neutral (low reliability)

<figure id="fig:mutationALA322GLY">

Close-up of the mutated glycine at residue 322 in PheOH. There is only one rotamer and there can not be collisions with neighbouring residues as glycine is the smallest amino acid.

Mutated glycine at residue 322 in PheOH. The residue is located in a helix region.

</figure>

GLY337VAL

Prediction:

While the alignment shows some replacements in the region around GLY337 and the PSSM shows no high conservation, the residue itself is conserved in mammals. The position in the loop between two beta sheets (see <xr id="fig:mutationGLY337VAL" />) makes this likely a critical position, especially as the introduced valine is larger but has to fit in the loop, and is much more hydrophobic but lies at the outside of the protein. The prediction methods disagree on the effect of this SNP, but we deem it more likely that this is a disease causing mutation.

• Amino acid changes: From neutral, non-polar, slightly hydrophilic, small to neutral, non-polar, strongly hydrophobic, medium sized.
• BLOSUM62/PAM250/PAM1: Bad replacement
• PSSM: position variable
• Alignment of homologs: some variability
• SIFT: AFFECT PROTEIN FUNCTION with a score of 0.00.
• PolyPhen: Possibly damaging
• SNAP: Neutral (low reliability)

<figure id="fig:mutationGLY337VAL">

Close-up of the mutated valine at residue 337 in PheOH. The best fitting rotamer was chosen to minimize severe or smaller collisions (red to green discs) with neighbouring residues. This rotamer appears in 2.9% of mutations according to the PyMol rotamer database.

Mutated valine at residue 337 in PheOH. The residue is located in a loop between two sheet elements.

</figure>

ARG408TRP

Prediction:

Here, the mutation lies in a coil region, but the introduction of the large tryptophan is likely to cause steric clashes and might influence the helix and sheet structures nearby (see <xr id="fig:mutationARG408TRP" />). The predictions agree and all available information suggests, that this mutation causes a negative effect.

• Amino acid changes: From pos. charged, polar, strongly hydrophilic, medium sized to neutral, non-polar, slightly hydrophilic, large.
• BLOSUM62/PAM250/PAM1: Bad replacement
• PSSM: conserved
• Alignment of homologs: highly conserved
• SIFT: AFFECT PROTEIN FUNCTION with a score of 0.00.
• PolyPhen: Probably damaging
• SNAP: Non-neutral (medium reliability)

<figure id="fig:mutationARG408TRP">

Close-up of the mutated tryptophan at residue 408 in PheOH. The best fitting rotamer was chosen to minimize severe or smaller collisions (red to green discs) with neighbouring residues. This rotamer appears in 2.3% of mutations according to the PyMol rotamer database.

Mutated tryptophan at residue 408 in PheOH. The residue is located in a coil near a helix region.

</figure>

References