Difference between revisions of "Task alignments 2012"
m (→Sequence searches) |
m (moved Task alignments to Task alignments 2012) |
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* multiple alignments (e.g. ClustalW, Probcons, Mafft, Muscle, T-Coffee, Cobalt) and MSA editors (e.g. Jalview) |
* multiple alignments (e.g. ClustalW, Probcons, Mafft, Muscle, T-Coffee, Cobalt) and MSA editors (e.g. Jalview) |
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with special attention to advantages and limitations of theses methods. |
with special attention to advantages and limitations of theses methods. |
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+ | |||
+ | == Where to run the analyses == |
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+ | * You can run the analyses on your own computers. |
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+ | * You can also use the student computer pool: <code>i12k-biolab0n.informatik.tu-muenchen.de</code>, where ''n'' goes from 1 to 9 (or more?). The file server does not have blast etc. installed! |
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== Sequence searches == |
== Sequence searches == |
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− | + | For every native protein sequence for every disease employ different tools for database searching and multiple sequence alignment in the "big80" database. |
|
The methods to employ (minimally) are: |
The methods to employ (minimally) are: |
||
− | * Searches of the non-redundant sequence database big_80 (to be found in /mnt/project/pracstrucfunc12/data/big/): |
+ | * Searches of the non-redundant sequence database big_80 (to be found in <code>/mnt/project/pracstrucfunc12/data/big/</code>): |
** Blast |
** Blast |
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** PSI-Blast using standard parameters with all combinations of |
** PSI-Blast using standard parameters with all combinations of |
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*** default E-value cutoff (0.002) |
*** default E-value cutoff (0.002) |
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*** E-value cutoff 10E-10 |
*** E-value cutoff 10E-10 |
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− | ** HHblits |
+ | ** HHblits (HHsearch) using standard parameters, since there is no big_80 for HHblits, search against Uniprot |
+ | '''Note:''' |
||
− | '''Note:''' Check the outcome of your simple blast search. If there are many significant hits, increase the number of reported hits (-v, -b or max_target_seqs depending on blast version and output format) until no more relevant hits are found. Use that parameter also for the PSI-Blast searches and use a similar setting for HHblits / HHsearch. (Think about why we ask you to do this.) |
||
+ | * Check the outcome of your simple blast search. If there are many significant hits, increase the number of reported hits (-v, -b or max_target_seqs depending on blast version and output format) until no more relevant hits are found. Use that parameter also for the PSI-Blast searches and use a similar setting for HHblits / HHsearch. (Think about why we ask you to do this.) |
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+ | *'' If your PSI-Blast search hits the limit (and your blast search didn't), also increase the number of reported hits!'' [[User:Andrea|andrea]] 10:31, 3 May 2012 (UTC) |
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+ | * Mentioning HHsearch here seems to be confusing. Sorry! Do a HHblits search. You can use HHsearch to solve the pdb structures problem mentioned below. |
||
'''CAVE''': If your data set gets large, the PSI-Blast searches will take a while. |
'''CAVE''': If your data set gets large, the PSI-Blast searches will take a while. |
||
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* compare the result lists (e.g. how much overlap, distribution of %identity and E-values) |
* compare the result lists (e.g. how much overlap, distribution of %identity and E-values) |
||
* validate the result lists -- e.g. |
* validate the result lists -- e.g. |
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− | ** using COPS (/mnt/project/pracstrucfunc12/data/COPS/) to check whether found pdb entries fall into the same fold class |
+ | ** using COPS (<code>/mnt/project/pracstrucfunc12/data/COPS/</code>) to check whether found pdb entries fall into the same fold class |
** using GO to check whether sequences have common GO classifications |
** using GO to check whether sequences have common GO classifications |
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** If you compare the representatives against a PSI-Blast result for big_80, you will get more hits for big_80. |
** If you compare the representatives against a PSI-Blast result for big_80, you will get more hits for big_80. |
||
** If you compare the representatives plus the cluster members against big_80, you will get fewer hits for big_80. |
** If you compare the representatives plus the cluster members against big_80, you will get fewer hits for big_80. |
||
− | ** Come up with a way to generate comparable results. (There is also a complete database "big" which you can use for searching -- reusing the profiles from your big_80 search. |
+ | ** Come up with a way to generate comparable results. (There is also a complete database "big" which you can use for searching -- reusing the profiles from your big_80 search. -- Think about why we don't ask you to start out with a search against big.) |
* big_80 is generated with [http://weizhong-lab.ucsd.edu/cd-hit/ CD-HIT], which prefers long sequences over shorter ones. Hence the number of pdb hits in your big_80 search is going to be low. Likewise, the Uniprot database for hhblits does not contain pdb structures. So, if you want to do the quality check using COPS data, come up with a way to generate comparable results. |
* big_80 is generated with [http://weizhong-lab.ucsd.edu/cd-hit/ CD-HIT], which prefers long sequences over shorter ones. Hence the number of pdb hits in your big_80 search is going to be low. Likewise, the Uniprot database for hhblits does not contain pdb structures. So, if you want to do the quality check using COPS data, come up with a way to generate comparable results. |
||
== Multiple sequence alignments== |
== Multiple sequence alignments== |
||
− | + | For calculating multiple sequence alignments, create a dataset of 20 sequences from the database search. |
|
+ | Ideally this dataset would include 5 sequences each from these ranges: |
||
* 99 - 90% sequence identity |
* 99 - 90% sequence identity |
||
* 89 - 60% sequence identity |
* 89 - 60% sequence identity |
||
* 59 - 40% sequence identity |
* 59 - 40% sequence identity |
||
* 39 - 20% sequence identity |
* 39 - 20% sequence identity |
||
+ | Ideally there should be at least one pdb-structure in each range. -- This will only be possible in rare cases! |
||
− | + | But generate at least three groups of 10 sequences where |
|
* one contains only sequences with low sequence identity (<40%) |
* one contains only sequences with low sequence identity (<40%) |
||
* one contains only sequences with high sequence identity (>60%) |
* one contains only sequences with high sequence identity (>60%) |
||
− | * one contains sequences |
+ | * one contains sequences covering the whole range of sequence identity. |
The alignment methods to use on each of these groups are: |
The alignment methods to use on each of these groups are: |
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** default parameters ("t_coffee your_sequences.fasta) |
** default parameters ("t_coffee your_sequences.fasta) |
||
** use of 3D-Coffee |
** use of 3D-Coffee |
||
+ | '''Note''': ClustalW should be on your path on the student machines, there is a version of T-Coffee on <code>/mnt/opt/T-Coffee/bin/</code>. If you include that in your path, you also have muscle. |
||
+ | |||
Compare your alignments (qualitatively). Things to look for are: |
Compare your alignments (qualitatively). Things to look for are: |
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* Are functionally important residues conserved? |
* Are functionally important residues conserved? |
||
* Are there gaps in secondary structure elements? |
* Are there gaps in secondary structure elements? |
||
+ | * Where do functionally important residues stand out most? |
||
Points for discussion: |
Points for discussion: |
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* Do all methods cope with low similarity? |
* Do all methods cope with low similarity? |
||
* Does the incorporation of structural information (3D Coffee) help? |
* Does the incorporation of structural information (3D Coffee) help? |
||
+ | * Overall, what would be your criteria for a good alignment? |
||
+ | * Based on your experience, which method would you like to use in the future? |
||
+ | |||
+ | == What to put on the Wiki == |
||
+ | |||
+ | The wiki entry referring to this task has several purposes: |
||
+ | * Use it as a lab journal to document what you did (make your results reproducible): e.g. collect what your command line looked like, which files your results are stored in, etc. |
||
+ | * Document your results: Describe what you observed. |
||
+ | * Discuss the outcome: Try to make sense of what you observed. Would you have expected that outcome? Why / why not? |
||
+ | |||
+ | We recommend to separate the "lab journal" part from the Results and Discussion part. |
Latest revision as of 08:17, 23 April 2013
Most prediction methods are based on comparisons to related proteins. Therefore, the search for related sequences and the alignment to other proteins is a prerequisite for most of the analyses in this practical. Hence we will investigate the recall and alignment quality of different alignment methods.
Contents
Theoretical background talks
The introductory talks should given an overview of
- pairwise alignments and high-throuput profile searches (e.g. Fasta, Blast, PSI-Blast, HHsearch)
- multiple alignments (e.g. ClustalW, Probcons, Mafft, Muscle, T-Coffee, Cobalt) and MSA editors (e.g. Jalview)
with special attention to advantages and limitations of theses methods.
Where to run the analyses
- You can run the analyses on your own computers.
- You can also use the student computer pool:
i12k-biolab0n.informatik.tu-muenchen.de
, where n goes from 1 to 9 (or more?). The file server does not have blast etc. installed!
Sequence searches
For every native protein sequence for every disease employ different tools for database searching and multiple sequence alignment in the "big80" database. The methods to employ (minimally) are:
- Searches of the non-redundant sequence database big_80 (to be found in
/mnt/project/pracstrucfunc12/data/big/
):- Blast
- PSI-Blast using standard parameters with all combinations of
- 2 iterations
- 10 iterations
- default E-value cutoff (0.002)
- E-value cutoff 10E-10
- HHblits (HHsearch) using standard parameters, since there is no big_80 for HHblits, search against Uniprot
Note:
- Check the outcome of your simple blast search. If there are many significant hits, increase the number of reported hits (-v, -b or max_target_seqs depending on blast version and output format) until no more relevant hits are found. Use that parameter also for the PSI-Blast searches and use a similar setting for HHblits / HHsearch. (Think about why we ask you to do this.)
- If your PSI-Blast search hits the limit (and your blast search didn't), also increase the number of reported hits! andrea 10:31, 3 May 2012 (UTC)
- Mentioning HHsearch here seems to be confusing. Sorry! Do a HHblits search. You can use HHsearch to solve the pdb structures problem mentioned below.
CAVE: If your data set gets large, the PSI-Blast searches will take a while.
For evaluating the differences of the search methods:
- compare the result lists (e.g. how much overlap, distribution of %identity and E-values)
- validate the result lists -- e.g.
- using COPS (
/mnt/project/pracstrucfunc12/data/COPS/
) to check whether found pdb entries fall into the same fold class - using GO to check whether sequences have common GO classifications
- using COPS (
Note: Make sure that your result lists are comparable. There are a few catches:
- HHblits searches against the clustered Uniprot version. In the output the cluster representatives are listed together with the cluster members.
- If you compare the representatives against a PSI-Blast result for big_80, you will get more hits for big_80.
- If you compare the representatives plus the cluster members against big_80, you will get fewer hits for big_80.
- Come up with a way to generate comparable results. (There is also a complete database "big" which you can use for searching -- reusing the profiles from your big_80 search. -- Think about why we don't ask you to start out with a search against big.)
- big_80 is generated with CD-HIT, which prefers long sequences over shorter ones. Hence the number of pdb hits in your big_80 search is going to be low. Likewise, the Uniprot database for hhblits does not contain pdb structures. So, if you want to do the quality check using COPS data, come up with a way to generate comparable results.
Multiple sequence alignments
For calculating multiple sequence alignments, create a dataset of 20 sequences from the database search. Ideally this dataset would include 5 sequences each from these ranges:
- 99 - 90% sequence identity
- 89 - 60% sequence identity
- 59 - 40% sequence identity
- 39 - 20% sequence identity
Ideally there should be at least one pdb-structure in each range. -- This will only be possible in rare cases!
But generate at least three groups of 10 sequences where
- one contains only sequences with low sequence identity (<40%)
- one contains only sequences with high sequence identity (>60%)
- one contains sequences covering the whole range of sequence identity.
The alignment methods to use on each of these groups are:
- ClustalW
- Muscle
- T-Coffee with
- default parameters ("t_coffee your_sequences.fasta)
- use of 3D-Coffee
Note: ClustalW should be on your path on the student machines, there is a version of T-Coffee on /mnt/opt/T-Coffee/bin/
. If you include that in your path, you also have muscle.
Compare your alignments (qualitatively). Things to look for are:
- How many conserved columns?
- How many gaps?
- Are functionally important residues conserved?
- Are there gaps in secondary structure elements?
- Where do functionally important residues stand out most?
Points for discussion:
- Observe how the sequence identity in the groups of sequences influences the alignments.
- Do all methods cope with low similarity?
- Does the incorporation of structural information (3D Coffee) help?
- Overall, what would be your criteria for a good alignment?
- Based on your experience, which method would you like to use in the future?
What to put on the Wiki
The wiki entry referring to this task has several purposes:
- Use it as a lab journal to document what you did (make your results reproducible): e.g. collect what your command line looked like, which files your results are stored in, etc.
- Document your results: Describe what you observed.
- Discuss the outcome: Try to make sense of what you observed. Would you have expected that outcome? Why / why not?
We recommend to separate the "lab journal" part from the Results and Discussion part.