Difference between revisions of "Application Exam Questions"
(→2002) |
|||
Line 18: | Line 18: | ||
<small>Comment</small> | <small>Comment</small> | ||
+ | |||
+ | ==2003 - Domains and Homology== | ||
+ | [[Image:CDART.jpg|frame|none|Following an Entrez-provided links to "sh3" domains may ultimately bring you to the CDART entry for a protein. This screenshot shows the first of ten pages of results for the eukaryotic SH3 domains. ]] | ||
+ | |||
+ | |||
+ | <div style="padding: 5px; background: #DDDDDD; border:solid 1px #000000;"> | ||
+ | *'''Briefly define homologs, orthologs and paralogs.''' | ||
+ | *'''Are the proteins depicted above homologs ?''' | ||
+ | *'''Briefly explain the contents, implications and use of this CDART entry.''' | ||
+ | </div> | ||
+ | |||
+ | <small>''(By now, "contents, implications and use" would be too vague and general for my taste for an exam question.)''</small> | ||
+ | |||
+ | |||
+ | ==2003 - Expression Analysis== | ||
+ | |||
+ | In order to study the coordination of gene expression in the yeast cell cycle, you have created a synchronized, growing culture of ''Saccharomyces cerevisiaea'' cells and harvested mRNA at ten successive time points along one replication cycle. You now plan to perform two-color microarray (spotted array) experiments. | ||
+ | |||
+ | <div style="padding: 5px; background: #DDDDDD; border:solid 1px #000000;"> | ||
+ | *'''Describe the principle and key steps of this experiment, from mRNA samples to a series of scanned images. ''' | ||
+ | *'''Describe the key steps involved in going from a scanned image to expression profiles of individual genes. ''' | ||
+ | *'''After clustering genes according to similarity of expression profiles, you will have sets of genes with correlated expression profiles. You hypothesize that these may be coregulated genes. What bioinformatics procedure(s) can you suggest to help you annotate shared functions for your clusters of genes ? ''' | ||
+ | *'''What bioinformatics procedure(s) can you suggest to pursue the question whether these genes may be coregulated ? ''' | ||
+ | </div> | ||
+ | |||
+ | <small>Comment</small> | ||
+ | |||
+ | |||
+ | ==2003 - Integrated processes== | ||
+ | |||
+ | Read the following abstract: | ||
+ | |||
+ | :'''Structure of TCTP reveals unexpected relationship with guanine nucleotidefree chaperones''' | ||
+ | |||
+ | :Paul Thaw, Nicola J. Baxter, Andrea M. Hounslow, Clive Price, Jonathan P. Waltho and C. Jeremy Craven: ''Nature Struct Biol'' '''8''': 701–704 (2001) | ||
+ | |||
+ | :The translationally controlled tumor-associated proteins (TCTPs) are a highly conserved and abundantly expressed family of eukaryotic proteins that are implicated in both cell growth and the human acute allergic response but whose intracellular biochemical function has remained elusive. We report here the solution structure of the TCTP from Schizosaccharomyces pombe, which, on the basis of sequence homology, defines the fold of the entire family. We show that <u>TCTPs form a structural superfamily with the Mss4/Dss4 family of proteins</u>, which bind to the GDP/GTP free form of Rab proteins (members of the Ras superfamily) and have been termed guanine nucleotide-free chaperones (GFCs). Mss4 also acts as a relatively inefficient guanine nucleotide exchange factor (GEF). We further show that the Rab protein binding site on Mss4 coincides with the region of highest sequence conservation in the TCTP family. This is the first link to any other family of proteins that has been established for the TCTP family and suggests the presence of a GFC/GEF at extremely high abundance in eukaryotic cells. | ||
+ | |||
+ | |||
+ | This abstract reports several pieces of data and mentions several pieces of prior information. | ||
+ | |||
+ | <div style="padding: 5px; background: #DDDDDD; border:solid 1px #000000;"> | ||
+ | *'''List the most important data and information entities and databases that have been used in this study.''' | ||
+ | *'''Summarize on approximately one-half page or less the essential steps of how these entities were related to each other in this study. You may use any representation that is reasonable such as pseudocode, a flowchart, or other type of sketch.''' | ||
+ | </div> | ||
+ | Note that you are not required to understand the biochemical processes that are described here, nor are you required to comment on the cell-biological implications. One of the key steps has been underlined by me - you must understand how such a conclusion can be drawn in the situation that is described. You are to summarize the flow of data: the entities that are being referred to, and the experimental and computational procedures. | ||
+ | |||
==2002== | ==2002== |
Revision as of 14:52, 11 December 2006
- Bioinformatics and computational biology are huge and growing areas of active research with a dynamic array of subspecialities - phylogenetic analysis has advanced in leaps and bounds with the availablity of molecular data, genomic-, transcriptomic-, proteomic and other cross-sectional views are slowly beginning to unravel some of the intricacies of the cell's inner workings, predictive models for molecular medicine and bioengineering may help shape our society's future. These tasks are what motivates bioinformatics worldwide, seeking to develp novel ways to reason about biology.
2003 - Consequences of Homology
A bacterial genome has been sequenced. Comparison with tRNA synthetase COGs has failed to turn up an annotation for a Glutaminyl tRNA synthetase gene. Assume that the genome sequence is complete, has been assembled without frameshift errors and all gene models are correct. The sequence for Glutaminyl tRNA synthetase has not simply been overlooked. Answer the following questions briefly.
- What is a COG ?
- State two reasons why the endpoint of a biochemical pathway could be present in an organism but a gene on the pathway would fail to be found in a COG analysis.
- Briefly(!) state what wet-lab experiments you would propose to confirm (or disprove) the hypotheses you have stated above ?
Comment
2003 - Domains and Homology
- Briefly define homologs, orthologs and paralogs.
- Are the proteins depicted above homologs ?
- Briefly explain the contents, implications and use of this CDART entry.
(By now, "contents, implications and use" would be too vague and general for my taste for an exam question.)
2003 - Expression Analysis
In order to study the coordination of gene expression in the yeast cell cycle, you have created a synchronized, growing culture of Saccharomyces cerevisiaea cells and harvested mRNA at ten successive time points along one replication cycle. You now plan to perform two-color microarray (spotted array) experiments.
- Describe the principle and key steps of this experiment, from mRNA samples to a series of scanned images.
- Describe the key steps involved in going from a scanned image to expression profiles of individual genes.
- After clustering genes according to similarity of expression profiles, you will have sets of genes with correlated expression profiles. You hypothesize that these may be coregulated genes. What bioinformatics procedure(s) can you suggest to help you annotate shared functions for your clusters of genes ?
- What bioinformatics procedure(s) can you suggest to pursue the question whether these genes may be coregulated ?
Comment
2003 - Integrated processes
Read the following abstract:
- Structure of TCTP reveals unexpected relationship with guanine nucleotidefree chaperones
- Paul Thaw, Nicola J. Baxter, Andrea M. Hounslow, Clive Price, Jonathan P. Waltho and C. Jeremy Craven: Nature Struct Biol 8: 701–704 (2001)
- The translationally controlled tumor-associated proteins (TCTPs) are a highly conserved and abundantly expressed family of eukaryotic proteins that are implicated in both cell growth and the human acute allergic response but whose intracellular biochemical function has remained elusive. We report here the solution structure of the TCTP from Schizosaccharomyces pombe, which, on the basis of sequence homology, defines the fold of the entire family. We show that TCTPs form a structural superfamily with the Mss4/Dss4 family of proteins, which bind to the GDP/GTP free form of Rab proteins (members of the Ras superfamily) and have been termed guanine nucleotide-free chaperones (GFCs). Mss4 also acts as a relatively inefficient guanine nucleotide exchange factor (GEF). We further show that the Rab protein binding site on Mss4 coincides with the region of highest sequence conservation in the TCTP family. This is the first link to any other family of proteins that has been established for the TCTP family and suggests the presence of a GFC/GEF at extremely high abundance in eukaryotic cells.
This abstract reports several pieces of data and mentions several pieces of prior information.
- List the most important data and information entities and databases that have been used in this study.
- Summarize on approximately one-half page or less the essential steps of how these entities were related to each other in this study. You may use any representation that is reasonable such as pseudocode, a flowchart, or other type of sketch.
Note that you are not required to understand the biochemical processes that are described here, nor are you required to comment on the cell-biological implications. One of the key steps has been underlined by me - you must understand how such a conclusion can be drawn in the situation that is described. You are to summarize the flow of data: the entities that are being referred to, and the experimental and computational procedures.
2002
- Task
Comment