Difference between revisions of "BIO Assignment 2 2011"

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Assignment 2 - Search, retrieve and annnotate
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Assignment 2 (last: 2011) - Search, retrieve and annotate
 
</div>
 
</div>
  
Note: This assignment is currently inactive. Unannounced changes may be made at any time.
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care=Be sure you have understood all parts of the assignment and cover all questions in your answers! Sadly, we always get assignments back in which important aspects have simply been overlooked and marks are unnecessarily lost. Sadly, we always get assignments back in which important aspects have simply been overlooked and marks are unnecessarily lost. If you did not notice that the above sentence was repeated, you are not reading carefully enough.|
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num=2|
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ord=second|
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due = Monday, October 24 at 12:00 noon (before the quiz)}}
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 +
 
 +
;Your documentation for the procedures you follow in this assignment will be worth 1 mark.
 +
 
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 +
&nbsp;
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&nbsp;
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<div style="padding: 2px; background: #F0F1F7;  border:solid 1px #AAAAAA; font-size:125%;color:#444444">
 
Introduction
 
Introduction
 
</div>
 
</div>
Baker's yeast, ''Saccharomyces cerevisiae'', is perhaps the most important model organism since it is a eukaryote that has been studied genetically and biochemically in great detail for many decades and it is easily manipulated with high-throughput experimental methods. We will use information from this model organism to study the conservation of function and sequence in other fungi whose genomes have been completely sequenced. This and the following assignments will revolve around a transcription factor that plays an important role in the regulation of the cell cycle: Mbp1, a key component of the MBF complex (Mbp1/Swi6) that regulates gene expression at the crucial G1/S-phase transition of the mitotic cell cycle and has been shown to bind to the regulatory regions of more than a hundred target genes.
+
Baker's yeast, ''Saccharomyces cerevisiae'', is perhaps the most important [http://en.wikipedia.org/wiki/Model_organism model organism]. It is a eukaryote that has been studied genetically and biochemically in great detail for many decades, and it is easily manipulated with high-throughput experimental methods. We will use information from this model organism to study the conservation of function and sequence in other fungi whose genomes have been completely sequenced; the assignments are an exercise in model-organism reasoning: the transfer of knowledge from one, well-studied organism to others.  
  
One would assume that such control machinery would be conserved in other fungi and it will be your task in these assignments to collect evidence whether related molecular machinery is present in some of the newly sequenced fungal genomes.
+
This and the following assignments will revolve around a transcription factor that plays an important role in the regulation of the cell cycle: '''Mbp1''' is a key component of the MBF complex (Mbp1/Swi6). This complex regulates gene expression at the crucial G1/S-phase transition of the mitotic cell cycle and has been shown to bind to the regulatory regions of more than a hundred target genes.
  
(If you need to brush up on the concepts mentioned above, you could study the corresponding chapter in [http://www.ncbi.nlm.nih.gov/entrez/query.fcgi?cmd=Search&db=books&doptcmdl=GenBookHL&term=MBF+AND+106229%5Buid%5D&rid=mcb.section.3531 Lodish's Molecular Cell Biology]. It is not strictly necessary to understand the details of the yeast cell-cycle to complete the assignments, but highly recommended, if this all is to make some sense.)
+
One would speculate that such central control machinery would be conserved in other fungi and it will be your task in these assignments to collect evidence whether related molecular machinery is present in some of the newly sequenced fungal genomes. Throughout the assignments we will use freely available tools to conduct bioinformatics investigations of questions such as:
 +
*What functional features can we detect in Mbp1?
 +
*Do homologous proteins exist in other organisms?
 +
*Do we believe these homologues may bind to similar sequence motifs?
 +
*Do we believe they may function in a similar way?
 +
*Do other organisms appear to have related cell-cycle control systems?
  
In this particular assignment you will go on a search and retrieve mission for information and annotation of Mbp1 homologues in a fungal genome, using common public databases and Web resources.
 
  
 +
&nbsp;<br><div style="padding: 5px; background: #EEEEEE;">
 +
*Access the [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=mbp1 information page on Mbp1] at the ''Saccharomyces'' Genome Database and read the summary paragraph on the protein's function!
 +
</div>
  
<div style="padding: 2px; background: #F0F1F7;  border:solid 1px #AAAAAA; font-size:125%;color:#444444">
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(If you would like to brush up on the concepts mentioned above, you could study the corresponding chapter in [http://www.ncbi.nlm.nih.gov/books/bv.fcgi?rid=mcb.chapter.3432 Lodish's Molecular Cell Biology] and./or read Nobel laureate [http://www.cumc.columbia.edu/dept/eukaryotic/nurse.pdf Paul Nurse's review (pdf)] of the key concepts of the eukaryotic cycle. It is not strictly necessary to understand the details of the yeast cell-cycle to complete the assignments, but recommended, since it's obviously more fun to work with concepts that actually make some sense.)
Preparation, submission and due date
+
 
 +
In this particular assignment you will go on a search and retrieve mission for information on yeast Mbp1, using common public databases and Web resources.
 +
 
 +
 
 +
<div style="padding: 5px; background: #BDC3DC;  border:solid 1px #AAAAAA;">
 +
==Search==
 
</div>
 
</div>
  
Read carefully. Be sure you have understood all parts of the assignment and cover all questions in your answers! Sadly, we always get assignments back in which important aspects have simply been overlooked and marks are unnecessarily lost. Sadly, we always get assignments back in which important aspects have simply been overlooked and marks are unnecessarily lost. If you did not notice that the above sentence was repeated, you are not reading carefully enough.
 
  
Prepare a Microsoft Word document with a title page that contains:
 
*your full name
 
*your Student ID
 
*your e-mail address
 
*the organism name you have been assigned (see below)
 
  
Follow the steps outlined below. You are encouraged to write your answers in short answer form or point form, '''like you would document an analysis in a laboratory notebook'''. However, you must
+
<div style="padding: 5px; background: #BDC3DC; border:solid 1px #AAAAAA;">
*document what you have done,
+
==Retrieve==
*note what Web sites and tools you have used,
+
</div>
*paste important data sequences, alignments, information etc.
+
 
  
If you do not document the process of your work, we will deduct marks. Try to be concise, not wordy! Use your judgement: are you giving us enough information so we could exectly reproduce what you have done?
+
Much useful information on yeast Mbp1 is compiled at the [http://db.yeastgenome.org/cgi-bin/locus.pl?locus=mbp1 SGD information page on Mbp1]. However we don't always have the luxury of such precompiled information. Let's look at the protein and it's features "the traditional way".
  
Write your answers into separate paragraphs and give each its title. Save your document with a filename of:
 
<code>A2_{lastname}.{firstname}.doc</code>
 
<small>(for example my first assignment would be named: A2_steipe.boris.doc - and don't include the brackets this time, please!)</small>
 
  
Finally e-mail the document to [boris.steipe@utoronto.ca] before the due date.
+
<div style="padding: 5px; background: #EEEEEE;  border:solid 1px #AAAAAA;">
 +
*Navigate to the NCBI homepage (you probably have bookmarked it anyway) and enter <code>Mbp1 AND "saccharomyces cerevisiae"[organism]</code> as an Entrez query.
 +
*Click on '''Protein''' and find the RefSeq record for the protein sequence.
 +
*From the NCBI RefSeq record, obtain a FASTA sequence of the protein and paste it into your assignment.
 +
</div>
  
Your document must not contain macros. Please turn off and/or remove all macros from your Word document; we will disable macros, since they pose a security risk.
 
  
With the number of students in the course, we have to economize on processing the assignments. '''Thus we will not accept assignments that are not prepared as described above.''' If you have technical difficulties, contact me.
+
There are several sources for functional domain annotations of proteins. The NCBI has the [http://www.ncbi.nlm.nih.gov/Structure/cdd/cdd.shtml Conserved Domain Database], in Europe, the [http://smart.embl-heidelberg.de/ SMART database] provides such annotations. In terms of domains, both resources are very comparable. But SMART also analyses more general features such as low-complexity sequences and coiled coils. In order to use SMART however, we need the '''Uniprot accession number''' that corresponds to the refseq identifier. In a rational world, one would wish that such important crossreferences would simply be provided by the NCBI ... well, we have been wishing this for many years now. Fortunately ID-mapping services exist.
  
'''The due date for the assignment is Thursday, October 19. at 10:00 in the morning.'''
 
  
<div style="padding: 2px; background: #F0F1F7; border:solid 1px #AAAAAA; font-size:125%;color:#444444">
+
<div style="padding: 5px; background: #EEEEEE;">
Grading
+
*Navigate to the [http://www.uniprot.org/?tab=mapping UniProt ID-Mapping service]. Enter the RefSeq identifier for the yeast Mbp1 protein and retrieve the corresponding UniProtKB Accession number. If this does not work, try the same mapping at the [http://pir.georgetown.edu/pirwww/search/idmapping.shtml PIR ID-mapping service]. Note the Uniprot accession number you find. (Should this work equally on both sites?)
 
</div>
 
</div>
  
Don't wait until the last day to find out there are problems! Assignments that are received past the due date will have one mark deducted at the first minute of every twelve hour period past the due date. Assignments received more than 5 days past the due date will not be assessed.
 
  
Marks are noted below in the section headings for of the tasks. A total of 10 marks will be awarded, if your assignment answers all of the questions. A total of 2 bonus marks (up to a maximum of 10 overall) can be awarded for particularily interesting findings, or insightful comments. A total of 2 marks can be subtracted for lack of form or for glaring errors. The marks you receive will
+
Now navigate to [http://www.uniprot.org '''Uniprot'''], enter the ID you have found into the search field and select [Sequence Clusters(UniRef)] as the database to search in. There should be two sequences in the '''[UniRef100 ... (100% identical)]''' cluster. Compare them. One of them is a highly annotated Swiss-Prot record, the other is practically unannotated data that has been imported from a "third party" to UniProt. Unfortunately, that one is the sequence that the ID mapping service had found. No cross-references to the NCBI are included with Swiss-Prot records, nor do NCBI RefSeq records cross-reference NCBI holding. I consider this a sorry state of affairs. Therefore most of us actually run BLAST searches to find equivalent sequences in other databases and this is the most wasteful way imaginable to address the problem.
* count directly towards your final marks at the end of term, for BCH441 (undergraduates), or
 
* be divided by two for BCH1441 (graduates).
 
  
&nbsp;
+
 
&nbsp;
+
<div style="padding: 5px; background: #EEEEEE;">
 +
*Note down the SwissProt ID and the UniProtKB Accession Number for yeast Mbp1.
 +
</div>
  
  
 
<div style="padding: 5px; background: #BDC3DC;  border:solid 1px #AAAAAA;">
 
<div style="padding: 5px; background: #BDC3DC;  border:solid 1px #AAAAAA;">
==Key databases==
+
 
 +
==Annotate==
 
</div>
 
</div>
 
&nbsp;
 
&nbsp;
 
&nbsp;
 
&nbsp;
 +
  
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
=== The NCBI (1 mark)===
+
 
 +
=== ''saccharomyces cerevisiae'' Mbp1 - domain annotations===
 
</div>
 
</div>
Visit the NCBI website at http://www.ncbi.nlm.nih.gov/
 
  
Look for the site-map and explore the contents of this site, the databases, the services and its other offerings. Browse across the different sections and set yourself a specific objective so you are confident you know what this part is and does. Expect to spend more than two hours on this task.
 
  
For example, you might have:
+
Now we can analyse Mbp1's domain in SMART, and use this information to annotate the sequence in detail.
* looked at least at two Coffee Break tutorials and know what the others contain
+
 
* familiarized yourself with the search field tags in PubMed to the degree that you know how to formulate a specific search, for example to retrieve review articles that mention the cell cycle in their title, which are about saccharomyces cerevisiae , that are not more than two years old
+
 
* tried searching for crossreferences to the YER111C gene using the Entrez system
+
<div style="padding: 5px; background: #EEEEEE;">
* used the map viewer to explore the region between 370 and 400 KB on yeast chromosome V
+
*Navigate to the [http://smart.embl-heidelberg.de/ SMART database], use "Normal Mode", then in the "Sequence Analysis" form enter the UniProtKB yeast Mbp1 accession number, check the checkboxes for the aditional analyses that SMART offers and carefully review the results. <small>By that I mean I might ask at some point what a particular section of the result means and how it is interpreted re. its biological significance. If parts are not obvious to you: &rarr; mailing list.</small>
* etc.
+
*In your assignment, in the actual, full-length sequence, highlight or otherwise clearly identify the features that SMART has annotated. Minimally you should include '''KilA-N''', '''low complexity''', '''coils''', and '''Ankyrin domains''', taking the sequence coordinates from the SMART annotations. Make sure you highlight the whole length of the feature and get the boundaries right. <small>If features overlap, you could eg. highlight one red, the other green and the overlap yellow. Or underline one, format the other in italics... And don't forget to label ''''what''' you have highlighted.</small>
 +
</div>
 +
 
  
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
=== The EBI (1 mark) ===
+
 
 +
=== APSES (KilA-N) domains ===
 
</div>
 
</div>
Visit the EBI website at http://www.ebi.ac.uk/
 
  
Look for the site-map and explore the contents of this site, the databases, the services and its other offerings. Browse across the different sections and set yourself specific objectives so you are confident you know what each section is and does. Expect to spend more than two hours on this task.
 
  
For example, you might have:
+
As you see from the annotations, Mbp1 is a large protein comprising several domains; it binds DNA through a small domain called the APSES domain (this is reported as the KilA-N domain superfamily). Many organisms have transcription factors that have a domains homologous to other APSES domains. Since we are interested in related proteins, and all functional relatives would be expected to share such a DNA binding domain, we should define this domain in more detail in order to be able to use it later to search for homologous proteins in diverse organisms.
* browsed through the tutorials (e.g. the lectin tutorial) in the education section of the Macromolecular Structure Database (MSD)group
+
 
* used the e! Ensembl browser to compare your experience in exploring yeast chromosomeV:370000-400000
+
 
* explored crossreferences to the yeast Swi4 protein using the SRS system
+
Use the NCBI Entrez system to search for the string "apses" in the "Conserved Domains" database and access the entry for the KilA-N domain superfamily. You should find 10 aligned sequences on that page, each with their own GI identifier. To find the actual boundaries of the domain annotation, do the following:
* browsed through the Interpro Molecule of the Month articles and read the article on TATA-box binding protein
+
 
* looked at the 2can tutorial pages and explored the tutorial on database browsing
+
 
* etc.
+
<div style="padding: 5px; background: #EEEEEE;">
 +
*Navigate back to the RefSeq Protein record <small>(You did record that link in your documentation, right?).</small> In the right-hand menu, find the section "Related information" and click on CDD Search results.
 +
* Click on the colored box for one of the annotated domains to appreciate the level of detailedinformation thatnis available here.
 +
*Back in the CDD annotation window, click on the [+] next to KilA-N super family to access the actual alignment of the PFAM domain definition with the MBP1 sequence.
 +
*Check and record (e.g. by highlighting) whether the NCBI and the SMART definition of the APSES domain in Mbp1 coincide exactly. If they don't, explain briefly what that means.
 +
*Make sure you understand how the sequences displayed on the CDD page and the actual domain sequences differ. <small>Hint: not all sequences are displayed in their full-length.</small>
 +
</div>
 +
 
  
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
===The PDB (1 mark) ===
+
 
 +
=== APSES domain structure ===
 
</div>
 
</div>
Visit the PDB website at http://www.pdb.org/
 
  
Browse across the different sections and set yourself a specific objective so you are confident you know what this part is and does. Look for the "About PDB" page and explore the page. Explore the links on the "Education" page to see where you might fill in gaps in your knowledege of structural molecular biology. From the homepage, find a protein of your choice (eg. the yeast Swi6 or Mbp1 protein) and explore the information that is available for it. Expect to spend more than an hour on this task.
+
We can expect that the structures of all homologous APSES domains should be similar, i.e. if the structure of one is known, we should be able to conclude the approximate three-dimensional structure of any APSES domain. Indeed, structural information ''is'' available for APSES domains!
 +
 
 +
 
 +
There are several possible approaches you could pursue to identify candidate files:
 +
 
 +
*there may be cross references to structures/PDB on any of the pages you have visited;
 +
*you could search the PDB itself for the keyword Mbp1;
 +
*you could use the domain sequence you have defined and ;
 +
**BLAST it against the database of PDB sequences (select it as an option on the BLAST form);
 +
**perform an "advanced serach" for similar sequences on the PDB Website.
 +
 
 +
 
 +
In any case, you should find more than one coordinate files that contain MBP1-like structures. Therefore you need to make a choice which one is the "best" for further analysis. Your choice of the "best" file for study could be based on:
 +
*experimental method (X-ray or NMR);
 +
*quality of the structure (resolution, refinement);
 +
*size (coverage) of the structure (number of amino acids for which structure coordinates have been determined).
 +
 
 +
&nbsp;<br><div style="padding: 5px; background: #EEEEEE;">
 +
*Record how you have identified the file you consider the "best" and what criteria you have used to define whether it is better suited for analysis than others.
 +
</div>
  
For example, you might have:
 
* worked through the PDB query tutorial
 
* browsed through the Molecule of the Month articles and studied the entry on TATA-box binding proteins
 
* and explored structures entries for 1SW6, 1E0B and 1BM8
 
* etc.
 
  
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
 
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
=== BioMart (1 mark) ===
 
</div>
 
Data integration across a variety of databases is a major challenge for the data-management side of bioinformatics. You have come across two solutions above: the NCBI Entrez system and the EBI SRS system. Here is another solution to this problem: the EBI BioMart system.
 
* Access the BioMart server at http://www.biomart.org
 
* Follow at least two links into BioMart databases (e.g. ensembl and HapMap)
 
* Explore
 
  
<div style="padding: 5px; background: #BDC3DC;  border:solid 1px #AAAAAA;">
+
=== DNA binding site ===
==Rasmol (3 marks)==
 
 
</div>
 
</div>
Access the Rasmol tutorial at http://biochemistry.utoronto.ca/steipe/bioinformatics/tutorials/rasmol_tutorial.html
 
Install Rasmol(Linux), RasMac (Macintosh), or RasTop(Windows) on your computer.
 
  
Work through the tutorial.
 
  
<div style="padding: 5px; background: #BDC3DC;  border:solid 1px #AAAAAA;">
+
The Mbp1 APSES domain has been shown to bind to DNA and the residues involved in DNA binding have been characterized. ([http://www.ncbi.nlm.nih.gov/pubmed/10747782 Taylor ''et al.'' (2000) ''Biochemistry'' '''39''': 3943-3954] and [http://www.ncbi.nlm.nih.gov/pubmed/18491920 Deleeuw ''et al.'' (2008) Biochemistry. '''47''':6378-6385]) . In particular the residues between 50-74 have been proposed to comprise the DNA recognition domain.
== Stereo vision (3 marks):==
+
 
 +
 
 +
<div style="padding: 5px; background: #FFCC99;">
 +
;Analysis (0.5 marks)
 +
 
 +
* Using VMD, generate a parallel stereo view of the protein structure that clearly shows the proposed Mbp1 DNA recognition domain, distinctly coloured differently from the rest of the protein. Use a representation that includes the sidechains.
 +
 
 +
* Generate a second VMD stereo image as above, but use a representation that emphasizes the secondary structure of the structure (tube or cartoon representation, colouring by structure).
 +
 
 +
* Generate a third VMD stereo image  that shows three representations combined: (1) the backbone, (2) the sidechains of residues that presumably contact DNA, distinctly colored, and (3) a transparent surface of the entire protein. This image should show whether residues annotated as DNA binding form a contiguous binding interface. '''Note:''' VMD makes smart use of GPU capabilities of your computer. Try setting your graphics parameters to visualize with GLSL - your transparent surface may look '''much''' better.
 +
 
 +
 
 +
Include the images into your assignment but be careful not to exceed the width and size restrictions I have defined in the submission guidelines. Include your "selections statements" (e.g. <code>protein and not resid 23 to 34</code>) so that it is easy for you to reproduce what you have done. Also note any important parameters you have changed from the default.
 
</div>
 
</div>
Use the hints given in the stereo vision section of the Rasmol tutorial and practice viewing molecules in stereo. Make sure that you use the Rasmol command
 
set stereo -5
 
to display molecules for divergent ("wall-eyed", not "cross-eyed") stereo view. Practice at least ...
 
* two times daily,
 
* for 3-5 minutes each session,
 
* for at least twelve days (twentyfour sessions) between now and the due date of the assignment.
 
Keep up your practice after the assignment. '''Stereo viewing will be required in the final exam.'''
 
  
You will receive 1 mark for every 8 sessions (4 days) of practice you have completed (max. 3 marks). Use different molecules and try them with different colouring and renderings. You will find a list suggesting interesting molecules on the tutorial page.
 
  
Record your progress on a sheet of paper. Make sure you also record the information for the supplementary questions you need to turn in (see below).
+
DNA binding interfaces are expected to comprise a number of positively charged amino acids, that might form salt-bridges with the phosphate backbone.  
  
'''Note: do not go through this assignment mechanically. If you are not making any progress, contact me so we can help you on the right track.'''
 
  
<div style="padding: 5px; background: #BDC3DC;  border:solid 1px #AAAAAA;">
+
<div style="padding: 5px; background: #FFCC99;">
==Assessment==
+
;Analysis (1 mark)
 +
 
 +
 
 +
*Report whether this is the case here and which residues might be included.
 +
*Do the DNA binding residues form a contiguous surface that is compatible with a binding interface? Justify your conclusions.
 
</div>
 
</div>
 +
<small>Be '''specific''' in your analysis: write exactly which residue does what. For example don't write
 +
:''there are many lysines...''
 +
but write something like
 +
:''K33, R35 and K76 form a patch of positively charged residues close to the C-terminus of the putative recognition helix.''
 +
This is the '''interpretation''' of results and therefore the '''most important step''' of your entire analysis.</small>
  
&nbsp;
 
  
&nbsp;
+
<div style="padding: 5px; background: #BDC3DC;  border:solid 1px #AAAAAA;">
  
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
+
== More statistics with R==
Copy and paste from the following for your submission. Copy the most appropriate phrase for each section, fill in the blanks and answer the questions truthfully.</div>
+
</div>
&nbsp;
 
  
'''NCBI:'''
 
I have explored the NCBI Web site in detail, familiarized myself
 
with its contents and am confident that I will find information
 
that I am  looking for. A part of the site that I found particularily
 
interesting or useful is ________________________ (1 mark).
 
or
 
I did not find the time to explore the NCBI site in detail (0 marks).
 
&nbsp;
 
&nbsp;
 
  
'''EBI:'''
+
Time for a break:
I have explored the EBI Web site in detail, familiarized myself
 
with its contents and am confident that I will find information
 
that I am looking for. A part of the site that I found particularily
 
interesting or useful is ________________________ (1 mark).
 
or
 
I did not find the time to explore the EBI site in detail (0 marks).
 
&nbsp;
 
&nbsp;
 
  
'''PDB:'''
 
I have explored the PDB Web site in detail, familiarized myself
 
with its contents and am confident that I will find information
 
that I am looking for. A part of the site that I found particularily
 
interesting or useful is ________________________ (1 mark).
 
or
 
I did not find the time to explore the PDB site in detail (0 marks).
 
&nbsp;
 
&nbsp;
 
  
'''BioMart:'''
+
<div style="padding: 5px; background: #FFCC99;">
I have accessed the BioMart Web site and familiarized myself with
+
;Second step (0.5 marks)
the functionality of at least two BioMart databases. I understand
 
some of the issues of data integration and how they are addressed
 
through BioMart.  (1 mark).
 
or
 
I did not find the time to explore the seqhound site (0 marks).
 
&nbsp;
 
&nbsp;
 
  
  
<div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
+
Access the [http://www.cyclismo.org/tutorial/R/ Clarkson University R tutorial]. Work through part two of the tutorial (Data types).
Copy and paste from the following statements the one that best characterizes your situation:
 
 
</div>
 
</div>
  
'''Rasmol:'''
 
I have successfully completed the Rasmol tutorial;
 
I understand the purpose and command syntax of
 
all the commands used in the scripted tutorial
 
examples and can confidently use all of these for
 
my own visualization tasks (3 marks).
 
or
 
I have worked with the Rasmol tutorial. Nevertheless,
 
I am not confident with the purpose and command
 
syntax of some of the commands used in the scripted
 
tutorial examples. I have changed some parameters
 
and achieved predictable results (2 marks).
 
or
 
The command syntax of some of the commands used
 
in the scripted tutorial examples is challenging; I have
 
worked with the program, but before I can use it for my
 
own purposes I will need additional training (1 marks).
 
or
 
I have not done this part of the assignment (0 marks).
 
&nbsp;
 
&nbsp;
 
  
 +
<!-- div style="padding: 5px; background: #E9EBF3;  border:solid 1px #AAAAAA;">
 +
 +
== Onward: the Genome of Interest ==
 +
</div -->
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The systematic name and strain of a fungus is listed with the [[Group project|project group]] that you have been assigned to. Navigate to the NCBI homepage &rarr; "Genomic Biology" &rarr; "Fungal Genomes Central" &rarr; "Genome Sequencing Projects". This should take you to a tabular view of ongoing and completed fungal genome sequencing projects. Find your organism name in this table. There may be one or more sequencing projects associated with the organism, but there should be only one project for the specific strain.
Copy the following statement into your assignment and fill in the blanks truthfully.
 
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Stereo Vision:
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Click on the organism name to navigate to the Genome Project information page.
I have practiced stereo viewing twice daily on _____ days
 
for a total of _____ practice sessions (maximum 3 marks for 24 sessions).
 
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*Review the status of the data you are working with - such as
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**whether the entire genome is available or only a partial sequence;
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**How many chromosomes does this genome have?
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**What is the status of its genome assembly and annotation?
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**Has the mitochondrial genome been sequenced as well?
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**Why is this organism deemed important enough to be sequenced?
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I have been able to visualize a 3D image in focus for the first time on day ___.
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I have been able to view molecules in stereo comfortably since day ___.
 
 
Currently I am able to view molecules in stereo on screen and on
 
paper with ease / with some effort / with difficulty / rarely / not at all.
 
  
  
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If you have any questions at all, don't hesitate to mail me at [mailto:boris.steipe@utoronto.ca boris.steipe@utoronto.ca] or post your question to the [mailto:bch441_2011@googlegroups.com Course Mailing List]

Latest revision as of 23:31, 21 September 2012

Note! This assignment is currently active. All significant changes will be announced on the mailing list.

 
 


   


   

Assignment 2 (last: 2011) - Search, retrieve and annotate

   


Preparation, submission and due date

Read carefully.
Be sure you have understood all parts of the assignment and cover all questions in your answers! Sadly, we always get assignments back in which important aspects have simply been overlooked and marks are unnecessarily lost. Sadly, we always get assignments back in which important aspects have simply been overlooked and marks are unnecessarily lost. If you did not notice that the above sentence was repeated, you are not reading carefully enough.

Review the guidelines for preparation and submission of BCH441 assignments.

The due date for the assignment is Monday, October 24 at 12:00 noon (before the quiz).

   


Your documentation for the procedures you follow in this assignment will be worth 1 mark.


   


Introduction

Baker's yeast, Saccharomyces cerevisiae, is perhaps the most important model organism. It is a eukaryote that has been studied genetically and biochemically in great detail for many decades, and it is easily manipulated with high-throughput experimental methods. We will use information from this model organism to study the conservation of function and sequence in other fungi whose genomes have been completely sequenced; the assignments are an exercise in model-organism reasoning: the transfer of knowledge from one, well-studied organism to others.

This and the following assignments will revolve around a transcription factor that plays an important role in the regulation of the cell cycle: Mbp1 is a key component of the MBF complex (Mbp1/Swi6). This complex regulates gene expression at the crucial G1/S-phase transition of the mitotic cell cycle and has been shown to bind to the regulatory regions of more than a hundred target genes.

One would speculate that such central control machinery would be conserved in other fungi and it will be your task in these assignments to collect evidence whether related molecular machinery is present in some of the newly sequenced fungal genomes. Throughout the assignments we will use freely available tools to conduct bioinformatics investigations of questions such as:

  • What functional features can we detect in Mbp1?
  • Do homologous proteins exist in other organisms?
  • Do we believe these homologues may bind to similar sequence motifs?
  • Do we believe they may function in a similar way?
  • Do other organisms appear to have related cell-cycle control systems?


 

  • Access the information page on Mbp1 at the Saccharomyces Genome Database and read the summary paragraph on the protein's function!

(If you would like to brush up on the concepts mentioned above, you could study the corresponding chapter in Lodish's Molecular Cell Biology and./or read Nobel laureate Paul Nurse's review (pdf) of the key concepts of the eukaryotic cycle. It is not strictly necessary to understand the details of the yeast cell-cycle to complete the assignments, but recommended, since it's obviously more fun to work with concepts that actually make some sense.)

In this particular assignment you will go on a search and retrieve mission for information on yeast Mbp1, using common public databases and Web resources.


Search


Retrieve


Much useful information on yeast Mbp1 is compiled at the SGD information page on Mbp1. However we don't always have the luxury of such precompiled information. Let's look at the protein and it's features "the traditional way".


  • Navigate to the NCBI homepage (you probably have bookmarked it anyway) and enter Mbp1 AND "saccharomyces cerevisiae"[organism] as an Entrez query.
  • Click on Protein and find the RefSeq record for the protein sequence.
  • From the NCBI RefSeq record, obtain a FASTA sequence of the protein and paste it into your assignment.


There are several sources for functional domain annotations of proteins. The NCBI has the Conserved Domain Database, in Europe, the SMART database provides such annotations. In terms of domains, both resources are very comparable. But SMART also analyses more general features such as low-complexity sequences and coiled coils. In order to use SMART however, we need the Uniprot accession number that corresponds to the refseq identifier. In a rational world, one would wish that such important crossreferences would simply be provided by the NCBI ... well, we have been wishing this for many years now. Fortunately ID-mapping services exist.


  • Navigate to the UniProt ID-Mapping service. Enter the RefSeq identifier for the yeast Mbp1 protein and retrieve the corresponding UniProtKB Accession number. If this does not work, try the same mapping at the PIR ID-mapping service. Note the Uniprot accession number you find. (Should this work equally on both sites?)


Now navigate to Uniprot, enter the ID you have found into the search field and select [Sequence Clusters(UniRef)] as the database to search in. There should be two sequences in the [UniRef100 ... (100% identical)] cluster. Compare them. One of them is a highly annotated Swiss-Prot record, the other is practically unannotated data that has been imported from a "third party" to UniProt. Unfortunately, that one is the sequence that the ID mapping service had found. No cross-references to the NCBI are included with Swiss-Prot records, nor do NCBI RefSeq records cross-reference NCBI holding. I consider this a sorry state of affairs. Therefore most of us actually run BLAST searches to find equivalent sequences in other databases and this is the most wasteful way imaginable to address the problem.


  • Note down the SwissProt ID and the UniProtKB Accession Number for yeast Mbp1.


Annotate

   


saccharomyces cerevisiae Mbp1 - domain annotations


Now we can analyse Mbp1's domain in SMART, and use this information to annotate the sequence in detail.


  • Navigate to the SMART database, use "Normal Mode", then in the "Sequence Analysis" form enter the UniProtKB yeast Mbp1 accession number, check the checkboxes for the aditional analyses that SMART offers and carefully review the results. By that I mean I might ask at some point what a particular section of the result means and how it is interpreted re. its biological significance. If parts are not obvious to you: → mailing list.
  • In your assignment, in the actual, full-length sequence, highlight or otherwise clearly identify the features that SMART has annotated. Minimally you should include KilA-N, low complexity, coils, and Ankyrin domains, taking the sequence coordinates from the SMART annotations. Make sure you highlight the whole length of the feature and get the boundaries right. If features overlap, you could eg. highlight one red, the other green and the overlap yellow. Or underline one, format the other in italics... And don't forget to label 'what you have highlighted.


APSES (KilA-N) domains


As you see from the annotations, Mbp1 is a large protein comprising several domains; it binds DNA through a small domain called the APSES domain (this is reported as the KilA-N domain superfamily). Many organisms have transcription factors that have a domains homologous to other APSES domains. Since we are interested in related proteins, and all functional relatives would be expected to share such a DNA binding domain, we should define this domain in more detail in order to be able to use it later to search for homologous proteins in diverse organisms.  

Use the NCBI Entrez system to search for the string "apses" in the "Conserved Domains" database and access the entry for the KilA-N domain superfamily. You should find 10 aligned sequences on that page, each with their own GI identifier. To find the actual boundaries of the domain annotation, do the following:


  • Navigate back to the RefSeq Protein record (You did record that link in your documentation, right?). In the right-hand menu, find the section "Related information" and click on CDD Search results.
  • Click on the colored box for one of the annotated domains to appreciate the level of detailedinformation thatnis available here.
  • Back in the CDD annotation window, click on the [+] next to KilA-N super family to access the actual alignment of the PFAM domain definition with the MBP1 sequence.
  • Check and record (e.g. by highlighting) whether the NCBI and the SMART definition of the APSES domain in Mbp1 coincide exactly. If they don't, explain briefly what that means.
  • Make sure you understand how the sequences displayed on the CDD page and the actual domain sequences differ. Hint: not all sequences are displayed in their full-length.


APSES domain structure

We can expect that the structures of all homologous APSES domains should be similar, i.e. if the structure of one is known, we should be able to conclude the approximate three-dimensional structure of any APSES domain. Indeed, structural information is available for APSES domains!


There are several possible approaches you could pursue to identify candidate files:

  • there may be cross references to structures/PDB on any of the pages you have visited;
  • you could search the PDB itself for the keyword Mbp1;
  • you could use the domain sequence you have defined and ;
    • BLAST it against the database of PDB sequences (select it as an option on the BLAST form);
    • perform an "advanced serach" for similar sequences on the PDB Website.


In any case, you should find more than one coordinate files that contain MBP1-like structures. Therefore you need to make a choice which one is the "best" for further analysis. Your choice of the "best" file for study could be based on:

  • experimental method (X-ray or NMR);
  • quality of the structure (resolution, refinement);
  • size (coverage) of the structure (number of amino acids for which structure coordinates have been determined).

 

 

  • Record how you have identified the file you consider the "best" and what criteria you have used to define whether it is better suited for analysis than others.


DNA binding site


The Mbp1 APSES domain has been shown to bind to DNA and the residues involved in DNA binding have been characterized. (Taylor et al. (2000) Biochemistry 39: 3943-3954 and Deleeuw et al. (2008) Biochemistry. 47:6378-6385) . In particular the residues between 50-74 have been proposed to comprise the DNA recognition domain.


Analysis (0.5 marks)
  • Using VMD, generate a parallel stereo view of the protein structure that clearly shows the proposed Mbp1 DNA recognition domain, distinctly coloured differently from the rest of the protein. Use a representation that includes the sidechains.
  • Generate a second VMD stereo image as above, but use a representation that emphasizes the secondary structure of the structure (tube or cartoon representation, colouring by structure).
  • Generate a third VMD stereo image that shows three representations combined: (1) the backbone, (2) the sidechains of residues that presumably contact DNA, distinctly colored, and (3) a transparent surface of the entire protein. This image should show whether residues annotated as DNA binding form a contiguous binding interface. Note: VMD makes smart use of GPU capabilities of your computer. Try setting your graphics parameters to visualize with GLSL - your transparent surface may look much better.


Include the images into your assignment but be careful not to exceed the width and size restrictions I have defined in the submission guidelines. Include your "selections statements" (e.g. protein and not resid 23 to 34) so that it is easy for you to reproduce what you have done. Also note any important parameters you have changed from the default.


DNA binding interfaces are expected to comprise a number of positively charged amino acids, that might form salt-bridges with the phosphate backbone.


Analysis (1 mark)


  • Report whether this is the case here and which residues might be included.
  • Do the DNA binding residues form a contiguous surface that is compatible with a binding interface? Justify your conclusions.

Be specific in your analysis: write exactly which residue does what. For example don't write

there are many lysines...

but write something like

K33, R35 and K76 form a patch of positively charged residues close to the C-terminus of the putative recognition helix.

This is the interpretation of results and therefore the most important step of your entire analysis.


More statistics with R


Time for a break:


Second step (0.5 marks)


Access the Clarkson University R tutorial. Work through part two of the tutorial (Data types).



[End of assignment]

If you have any questions at all, don't hesitate to mail me at boris.steipe@utoronto.ca or post your question to the Course Mailing List