Difference between revisions of "Fabry:Homology based structure predictions"

Fabry Disease » Homology based structure predictions

The following analyses were performed on the basis of the α-Galactosidase A sequence. Please consult the journal for the commands used to generate the results.

Dataset preparation and target comparison

Datasets

We performed a HHpred as well as a COMA search, to generate three distinct datasets. Since COMA did not find any homologue structures with a similarity above 41% (see <xr id="tab:datasetCOMA"/>), we used the dataset created with the HHpred search and the script described in the journal. Hereby we found one structure with a similarity above 80%, one with a similarity between 40 and 80% and 15 with sequence similarity below 30%, of which 14 had a similarity of under 20% (see <xr id="tab:datasetHHpred" />). All HHpred matches had an E-value below 1e-15, for the COMA homologues we tried a less strict threshold of 0.002.
In most of the cases we used the structures 3hg3, 1ktb and 3cc1 for modelling, because either they are the only representatives in their class, or in the case od 3cc1, the sequence identity did not seem too low. For the Model MULTI 3 we also used the structures 3a24 and 3zss. The latter of those has an E-value of 0.00062. We added this structure to examine how a template with an E-value that is worse than the value of all our other structures, but still would fullfill the restrictions of an usual BLAST search (threshold of 0.003), would perform.
In this case it is important to mention, that although the identity of 3hg3 is 100%, it is not the pdb structure annotated for the AGAL protein, but the structure of the substrate bound catalytic mechanism, hence the high similarity.
1ktb is the X-ray structure for the already mentioned α-N-acetylgalactosiminidase in chicken, which in future might be used for enzyme replacement therapy in the treatment of Fabry Disease.
The last one of the frequently used structures, 3cc1, is the x-ray structure of a putative α-N-acetylgalactosiminidase in in Bacillus Halodurans.

Target comparison

<figtable id="tab:compare"> Comparison of apo and complex structure

Superimposed structures of 1R46 (blue) and 1R47 (green) in cartoon representation. Obviously, the structures do not differ much.

Comparison of the residues invoked in the binding of α-galactose in the apo structure (blue) and the complex structure (green)

</figtable>

<figure id="fig:GAL:1R47">

Residues involved in the binding of α-galactose in 1R47 source

</figure>

As an initial step of the evaluation, we compared the apo structure 1R46 and the complex structure (with bound α-galactose) 1R47. Since the alignment of both the chains A of 1R46 and 1R47 in Pymol (see <xr id="tab:compare"/>) revealed a RMSD value of 0.248 and the comparison of the position and direction of the residues involved in the binding of the sugar (see <xr id="fig:GAL:1R47"/>) do not differ significantly, we used only the 1R46 structure for vizualisation, but computed all values and statistics for both structures.
In the right figure in <xr id="tab:compare"/>, the residues Asp92A, Asp93A, LYS168A, ARG227A and ASP231A are depicted in sticks representation (thicker); they are responsible for the binding of the sugar in the complex structures, which is shown in magenta. Clearly, one can see not much difference in this region between 1R46 and 1R47.

Modeller

Calculation of models

With this command line tool, we created 10 models (see Journal). The first three were produced with the standard settings and workflow of Modeller. The subsequent four models were computed from multiple target files in different combinations and in the last three models we rearranged the alignment files in order to test the quality of the alignment and the influence of the two types of alignment.

Default settings

Model 1

<figtable id="tab:pics_1R46_3HG3"> Model 1, visual comparison

Model 1 (red), created with Modeller with the template 3HG3, superimposed on the x-ray structure of α-Galactosidase A (green)

Model 1 (red) superimposed on the x-ray structure of α-Galactosidase A (green) and the structure of 3HG3 (yellow)

</figtable>

For the first model we used the template with the highest sequence identity. According to HHPred, the identity is 100%, Modeller only calculates an identity of 96% (see <xr id="tab:Modeller_scores_3hg3_2"/>). This discrepancy might be due to the way of the comparison - 1R46 is completely inclosed in 3HG3, but 3HG3 has a longer sequence (404 residues) and thus only 96% of it can be congruent to 1R46 (398 residues without signal peptide). In the left picture in <xr id="tab:pics_1R46_3HG3"/> the superimposition of the computed Model 1 and the actual target structure are shown. The right picture additionally displays the template structure. One can see, that the three structure almost perfectly superimpose, which is underlined by the scores derived from Modeller (see <xr id="tab:Modeller_scores_3hg3_2"/>). The GA341 score of 1.0 indicates a "native like" model (see basic tutorial) and the Compactness <ref name="Compactness"> Foldit Wiki, Compactness (October 23, 2011), http://foldit.wikia.com/wiki/Compactness; May 26, 2012</ref> as well as the DOPE score (see basic tutorial) are the second highest and lowest of all calculated models, respectively.
The only parts that can not be modelled correctly are both ends of the sequence. Those parts are highlighted blue in the pictures. From our background knowledge we know that the first 31 residues form the signal peptide, that is cleaved off and thus can not be found in the tertiary structure of the target protein. This can not be modelled by the Modeller tool and thus it would be a good amendment to the modelling pipeline to add sequence based analyses like Signal peptide prediction, similiar to the predictions we made in Task 2. The lack of modellation of the last bit of the sequence can be pinned to the longer sequence of the 3HG3 structure, since the last 6 residues are craning and the template is 6 amino acids longer than the target.
Inspecting the problematic residues (see <xr id="tab:Modeller_scores_3hg3_1"/>), with a distance of more than 8 angstrom, manually in pymol, we discovered that two of them lie in loop regions (91 and 101) which are hard to model. On the other hand two of the residues are located in a helix (160 and 318) and seem to fit perfectly to the target.
For further evaluation of the model, please see Modeller Evaluation

Model 2

<figtable id="tab:pics_1R46_1KTB"> Model 2, visual comparison

Model 2 (red), created with Modeller with the template 1ktb, superimposed on the x-ray structure of α-Galactosidase A (green)

Model 2 (red) superimposed on the x-ray structure of α-Galactosidase A (green) and the structure of 1ktb (yellow)

</figtable>

For this model, we used the target 1KTB, which has a sequence identity of 53%. The superimposed structures of 1R46 and Model 2 are shown in <xr id="tab:pics_1R46_1KTB"/>, as well as the structural alignment of 1KTB with the model and the target. This model encounters only one of the problems of Model 1, namely the not modeled signal peptide for the same reasons mentioned above. The end of the sequence seems to be modeled just fine, although the template sequence is even longer (405 residues) than 3HG3. Despite the little worse Compactness and DOPE score (see <xr id="tab:Modeller_scores_1ktb_2"/>) , Model 2 seems to be really good, since there are no residues that have a distance greater than 8 Å (see <xr id="tab:Modeller_scores_1ktb_1"/>) and according to the GA341 score the model is also "native like" and a value greater than 0.7 generally indicates a reliable model, defined as ≥ 95% probability of correct fold. <ref name="Melo2002"> Melo F, Sánchez R, Sali A. (2002). Statistical potentials for fold assessment. Protein Sci. 2002 Feb;11(2):430-48. PMCID: PMC2373452</ref> .
For further evaluation of the model, please see Modeller Evaluation

Model 3

<figtable id="tab:pics_1R46_3CC1"> Model 3, visual comparison

Model 3 (red), created with Modeller with the template 3CC1, superimposed on the x-ray structure of α-Galactosidase A (green)

Model 3 (red) superimposed on the x-ray structure of α-Galactosidase A (green) and the structure of 3CC1 (yellow)

</figtable>

For the last of the basic models we used the structure 3CC1 as a template, which is rather far related with a sequence identity of roughly 25%. Here the emerging problems are obvious. Of course, the signal peptide can not be modelled again, but the real problem is that Model 3 is tilted approximately 90° compared to the target structure 1R46.
Additionally analyzing the quality scores of the model, we see that the model must be rejected. For example the GA341 score of 0.33 indicates that the model should be disarded, since any good model will give a score near 1.0, and according to Salilab any model with a score less than 0.6 should not be considered as helpfull <ref name="GA341"> Salilab - Modeller Usage, modeller ga341 score (February 21, 2006), http://salilab.org/archives/modeller_usage/2006/msg00060.html; May 26, 2012</ref>. By all means, the z-scores are also not good, because these statistical potentials contribute to the GA341 (see Modeller help).
For further evaluation of the model, please see Modeller Evaluation

Multiple templates

MULTI 1

<figtable id="tab:pics_1R46_multi1"> Model MULTI 1, visual comparison

Model MULTI 1 (red) (templates 3HG3 and 1KTB), superimposed on the x-ray structure of α-Galactosidase A (green)

Model MULTI 1 (red) superimposed on α-Galactosidase A (green) and the structure of 3HG3 (yellow) and 1KTB (orange)

</figtable>

Model 1, which is based on the structures 3HG3 and 1KTB is the subjectively second best of the Modeller computed models. The superimposition of the model and the target structure (see <xr id="tab:pics_1R46_multi1"/>) shows a similiar results to Model 1, but comparing the quality scores, we observe a slightly worse DOPE score a really bad Compactness value. According to Salilab the DOPE score is the score to distinguish between two good models <ref name="GA341"> Salilab - Modeller Usage, modeller ga341 score (February 21, 2006), http://salilab.org/archives/modeller_usage/2006/msg00060.html; May 26, 2012</ref>. This model has the second lowest score of all, as well as a almost 100% sequence identity to the target.
On the other hand, the Compactness seems to be really low, even smaller than the value of Model 3. Thus we think, that this quality score cannot really be considered reliable, in contrast to the DOPE score.
What also becomes obvious in this model, is that the more distant related 1KTB structure (orange) seems to fit better than the really close related 3HG3 (yellow), which can be seen in the visual comparison in the right picture of <xr id="tab:pics_1R46_multi1"/>.
For further evaluation of the model, please see Modeller Evaluation

MULTI 2

<figtable id="tab:pics_1R46_multi2"> Model MULTI 2, visual comparison

Model MULTI 2 (red), created with Modeller on basis of the templates 3HG3, 1KTB and 3CC1, superimposed on the x-ray structure of α-Galactosidase A (green)

Model MULTI 2 (red) superimposed on the x-ray structure of α-Galactosidase A (green) and the structure of 3HG3 (yellow), 1KTB (orange) and 3CC1 (lightorange)

</figtable>

Model 2 bases on Model 1, but has the additional structure 3CC1, which is rather distantly related to 1R46. Hence we have one structure of each sequence identity group. Thus we can observe a decrease in the model quality. In <xr id="tab:pics_1R46_multi2"/> one can see, that the signal peptide is somewhat nested inside the molecule. The DOPE score increased, thus indicating a less reliable model, although the Compactness has the highest level of all models (see <xr id="tab:Modeller_scores_MULTI2_2" />), underlining our above made statement, that this score is not really trustworthy.
Another sign for the bad quality of the model are the 556 residues with a distance greater than 6 angstrom shared among the three template structures in the alignment (see <xr id="tab:Modeller_scores_MULTI2_1" />).
For further evaluation of the model, please see Modeller Evaluation

MULTI 3

<figtable id="tab:pics_1R46_multi3"> Model MULTI 3, visual comparison

Model MULTI 3 (red), created with Modeller on basis of the templates 3CC1, 3ZSS and 3A24, superimposed on the x-ray structure of α-Galactosidase A (green)

Model MULTI 3 (red) superimposed on the x-ray structure of α-Galactosidase A (green) and the structure of 3CC1 (yellow), 3ZSS (orange) and 3A24 (lightorange)

</figtable>

This model combines three structures with a sequence identity of less than 30%, one of these has even a worse E-value than all the others (3ZSS - see section Datasets) to underline the need of a strict threshold in the dataset preparation.
In <xr id="tab:pics_1R46_multi3"/> demonstrates that there is an overhang of the Model 3 (red) on both sides of 1R46 and the signal peptide is again nested inside the structure. Looking at the right picture in the table, we find the explanation for this, because 3ZSS (orange) also takes up more space at the end than all other compared structures.
In this model the number of very distant residues is even more than in model MULTI 2, as we can see in <xr id="tab:Modeller_scores_MULTI3_1"/> there are 1488 bad aligned residues in the multiple sequence alignment of the four target structures. The quality scores, except for the Compactness, emphasize the bad quality of the model. Here, the GA341 score is especially low (0.004 - see <xr id="tab:Modeller_scores_MULTI3_2"/>).
For further evaluation of the model, please see Modeller Evaluation

MULTI 4

<figtable id="tab:pics_1R46_multi4"> Model MULTI 4, visual comparison

Model MULTI 4 (red), created with Modeller on basis of the templates 3CC1 and 3HG3, superimposed on the x-ray structure of α-Galactosidase A (green)

Model MULTI 4 (red) superimposed on the x-ray structure of α-Galactosidase A (green) and the structure of 3CC1 (yellow) and 3HG3 (orange)

</figtable>

The last member of the group of multiple template models is based on one structure of the best identity group (3HG3) and one of the worst group (3CC1). Here we can confirm our assumption, that 3CC1 increases the Compactness of the model by modeling the signal peptide inside the structure and hereby decreases the quality of the model (see <xr id="tab:pics_1R46_multi4"/>). This growth of Compactness comes on the expense of DOPE score (<xr id="tab:Modeller_scores_MULTI4_2"/>) and number of closely aligned residues (<xr id="tab:Modeller_scores_MULTI4_1"/>).
For further evaluation of the model, please see Modeller Evaluation

Edited Alignment input

CHAS and CHAS 2

<figtable id="tab:pics_1R46_3HG3_CHAS"> Models CHAS and CHAS 2, visual comparison

Model CHAS (red), with active site shifted right to next D (7 and 1 positions) in 2d alignment file, superimposed on the x-ray structure of α-Galactosidase A (green); active site highlighted in blue (target) and cyan (model)

For comparison with Model CHAS and CHAS 2, Model 1 (orange) which was basis for the edited alignments, superimposed on α-Galactosidase A (green); active site highlighted in blue (target) and cyan (model)

Model CHAS 2 (red), with active site shifted right to next D (7 and 1 positions) in both alignment files, superimposed on the x-ray structure of α-Galactosidase A (green); active site highlighted in blue (target) and cyan (model)

</figtable>

In these two models we tried to eluminate the influence of both alignment types in the model creation process. In order to do so, we changed the alignment of the active site in the 2d alignment such that each of the two Aspartic acid residues (position 170 and 231) is aligned with the next subsequent Asp in the template sequence. From this, we created model CHAS.
As a second step, we performed the same adjustment in the normal alignment and created CHAS 2.
Comparing the results with Model 1, we see that there is absolutely no difference between Model 1 and CHAS in any score or value, but a huge difference to CHAS 2. Leading to the conclusion, that the way we perform the model creation, the 2d alignment has absolutely no influence and making this step dispensable.
In the pictures in <xr id="tab:pics_1R46_3HG3_CHAS"/> a visual comparison of Model 1, CHAS and CHAS 2 was performed, with special attention to the modelling of the active site, highlighted in blue (target) and cyan (model).

CHAS 3

<figtable id="tab:pics_1R46_3HG3_CHAS3"> Model CHAS 3, visual comparison

Model CHAS 3 (red), with active site shifted right to next D (7 and 1 positions) in both alignment files and the substrate binding region (position 203-207, highlighted in blue and cyan) forced to be consecutive, superimposed on of α-Galactosidase A (green)

For comparison with Model CHAS 3, Model 1 (orange) which was basis for the edited alignments, created with Modeller on basis of the templates 3HG3, superimposed on the x-ray structure of α-Galactosidase A (green); binding region highlighted in blue and cyan

</figtable>

In the last model, we tried to improve the quality of a subjectively bad aligned region, the substrate binding region (position 203-207, highlighted in <xr id="tab:pics_1R46_3HG3_CHAS3"/>) by forcing it to be consecutive in the alignment. Taking a look at the comparison of Model 1 and the 1R46 structure in the right picture in <xr id="tab:pics_1R46_3HG3_CHAS3"/>, we see that the regions despite the "poor" alignment is modelled nearly perfct, but adjusting the alignment produces a very bad modelled substrate binding site, as one can see in the left picture.
Surprisingly, the calculated quality scores are not deviant from those of CHAS 2 (the adjustment in the alignment of the active site was maintained), although the binding site looks different.

Evaluation

TM-score

RMSD with SAP

<figure id="fig:RMSD_1ktb">

Depiction of the RMSD (green) of Model 1 (magenta) from Modeller and 1R46 (cyan)

</figure> <figure id="fig:RMSD_1ktb">

Depiction of the RMSD (green) of MULTI 1 (magenta) from Modeller and 1R46 (cyan)

</figure> <figure id="fig:RMSD_1ktb">

Depiction of the RMSD (green) of Model 2 (magenta) from Modeller and 1R46 (cyan)

</figure>

High values in Pymol in certain models: lot of unrecognized residues like EDO. Using repairPDB did not help.

DOPE score

<figure id="fig:DOPE_Model">

Per residue DOPE score comparison of 1R46 (green) with Model 1, 2 and 3 (red, orange and pink)

</figure> <figure id="fig:DOPE_MULTI">

Per residue DOPE score comparison of 1R46 (green) with MULTI 1-4 (red, orange, pink and purple)

</figure> <figure id="fig:DOPE_CHAS">

Per residue DOPE score comparison of 1R46 (green) with CHAS 1, 2 and 3 (red, orange and pink)

</figure> <figure id="fig:DOPE_Best2">

Per residue DOPE score comparison of 1R46 (green) with the two subjectively best models Model 1 and MULTI 1 (red and orange)

</figure>

Swissmodel

Calculation of models

Evaluation

TM-score

RMSD with SAP

iTasser

3D-Jigsaw

References

<references/>