Protein Complex Discovery Who: identity of proteins in complex? What: biological process involved? Where: is the complex localized? When: are proteins involved in the complex? How much: stoichiometry of proteins in complex quantity- relative vs absolute Regulation: modifications
Direct Analysis of a Complex: The Kinetochore The kinetochore is the structure on chromosomes where the spindle fibers attach during cell division to pull the chromosomes apart Microtubules are green, chromosomes are blue, and kinetochores pink
Tandem Affinity Purification 5’ gene� 3’ Tag� Clone gene and add tag code to N or C terminal Express tagged protein in cell Bait Protein Calmodulin TEV cleavage site Protein A
Tandem Affinity Purification (i) The cell extract is passed over an IgG column. This binds the ProteinA tag on the protein. The column is then washed.
Tandem Affinity Purification (ii) TEV protease is added to cleave the ProtA tag away. The target is eluted and bound to a phenylsepharose column since the CaM tag binds this in the presence of calcium. The column is washed and the tagged protein released by removing calcium with EDTA
Cell-Map Proteomics –Tandem Affinity Purification
Systematic Complex pull-downs
Final verified complex
Zooming the Picture Out
The Big Picture
Yeast two-hybrid method Goal: Determine how proteins interact with each other Method Use yeast transcription factors Gene expression requires the following: A DNA-binding domain An activation domain A basic transcription apparatus Attach protein1 to DNA-binding domain (bait) Attach protein2 to activation domain (prey) Reporter gene expressed only if protein1 and protein2 interact with each other The yeast two-hybrid method exploits the gene transcription machinery of yeast to study interactions between proteins in vivo. Gene transcription in S. cerevisiae, as in most eukaryotic cells, requires a DNA-binding domain, an activation domain, and the basic transcription apparatus. A protein of interest (call it protein1) is attached to the DNA-binding domain of a well-characterized transcription factor such as Gal4. This protein is called the “bait.” Protein2 is attached to the activation domain from the same transcription factor. The protein2-activation domain complex is called the “prey.”If protein1 and protein2 interact with each other, then DNA binding and activation will occur and a reporter gene will be expressed. The yeast two-hybrid method is shown schematically in the next slide.
A schematic of the yeast two-hybrid method The figure in the slide shows in greater detail how the yeast two-hybrid method works. Two sets of yeast colonies are grown. In this example, the first set of colonies consists of all yeast open reading frames (ORFs) attached to the DNA-binding domain. The second set of colonies consists of all ORFs attached to the activation domain. Yeast from the two sets of colonies are mated with each other to produce every possible protein–protein interaction in the offspring. Cells expressing the reporter gene are selected, and their ORFs are identified by DNA sequencing to reveal the precise protein–protein interaction. This method has been successfully applied to determine all protein–protein interactions in the yeast Saccharomyces cerevisiae, as shown in the next slide. © 2005 Prentice Hall Inc. / A Pearson Education Company / Upper Saddle River, New Jersey 07458
Drosophila interaction map Recently a group of researchers from CuraGen Corporation, a biotechnology company, completed an extensive protein-interaction map of Drosophila, using the yeast two-hybrid system. The image in this slide shows the entire interaction map as well as close-up of a particular region. The nodes of the interaction map are coded to indicate the likely function of the protein they represent. Black stars around a node indicate a gene implicated in human disease. For this map, the 3,000 interactions with the highest confidence values were chosen, and they link 3,522 proteins.
Attaching a Green Flurescent Protein to an ORF PCR product GFP HIS3MX6 Homologous recombination Chromosome ORF1 ORF2 As in the case of protein–protein interactions, the yeast genome was used to determine the subcellular location of products of all ORFs. This was done by inserting the sequence for the green fluorescent protein (GFP) together with a marker gene (HIS3MX6) that makes it possible to select transformed yeast strains in histidine-free medium. Oligonucleotide primers corresponding to each ORF were used to generate ORF-specific sequences flanking the GFP and selectable marker. This approach permits the sequence to be incorporated into the chromosomal DNA via homologous recombination. The fusion protein resulting from this insertion has the GFP attached at the C-terminus of the ORF protein. Inside the living cell, the precise location of the protein can be determined by localizing the protein’s fluorescence. Fusion protein NH2 protein GFP COOH
Location of proteins revealed 75% of yeast proteome localized > 40% of proteins in cytoplasm 67% of proteins were previously unlocalized Localizations correlate with transcriptional modules cytoplasm nucleus The image in this slide shows a tagged protein that was localized to the nucleus. Note the contrast between the glowing nucleus and the much fainter cytoplasm. This study was able to successfully localize 75% of the entire yeast proteome, with greater than 40% of the proteins being found in the cytoplasm, and other proteins being localized in 21 distinct subcellular regions, including the nucleus, mitochondria, and the endoplasmic reticulum. The researchers were also able to show that subcellular localizations frequently correlated with transcriptional modules. By comparing their data with previous work on protein–protein interactions, they were also able to show that proteins localized in different regions had different probabilities of interacting with each other. For example, proteins in the cytoplasm were only 1.3 times more likely to interact with each other by chance, while microtubule-bound proteins were 56 times more likely to do so. A protein localized to the nucleus © 2005 Prentice Hall Inc. / A Pearson Education Company / Upper Saddle River, New Jersey 07458
Subcellular localization of interacting proteins The Drosophila protein-interaction map was also organized to show where interactions are likely to occur in the cell. Proteins with known, or annotated, subcellular localizations were used to determine the sites of likely interactions. The nodes are color coded to indicate what cellular component each protein belongs to. In this map, there are 2,346 proteins and 2,268 interactions.
Molecular Machinary-Parts List