The Yeast Two-Hybrid System.ppt
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1、The Yeast Two-Hybrid System,Anne C. Luebke,What is the yeast two-hybrid system used for?,Identifies novel protein-protein interactions Can identify protein cascades Identifies mutations that affect protein-protein binding Can identify interfering proteins in known interactions (Reverse Two-Hybrid Sy
2、stem),How does it work?,Uses yeast as a model for eukaryotic protein interactions A library is screened or a protein is characterized using a bait construct Interactions are identified by the transcription of reporter genes Positives are selected using differential media,The Model,DNA-Binding Domain
3、,Bait Protein,Prey Protein,Transcription Activating Region,Reporter Gene,DNA-Binding Site,Steps to Screen a Library,Create the Bait Plasmid Construct from the gene of interest and the DNA binding domain of Gal4 or LexA or other suitable domain Transform with the bait construct a yeast strain lacking
4、 the promoter for the reporter genes and select for transformed yeast Transform the yeast again with the library plasmids Select for interaction,Sequence analysis,Isolate plasmid from yeast and transform E. coli Purify plasmid from E. coli and sequence Blast sequence against database for known prote
5、ins or construct a possible protein sequence from the DNA sequence and compare to other proteins,Reporter Genes,LacZ reporter - Blue/White Screening HIS3 reporter - Screen on His+ media (usually need to add 3AT to increase selectivity) LEU2 reporter - Screen on Leu+ media ADE2 reporter - Screen on A
6、de+ media URA3 reporter - Screen on Ura+ media (can do negative selection by adding FOA),Plasmid Constructs,Plasmids are constructed with the Gal4 DNA binding domain (or other suitable domain) in front of a Multiple Cloning Site (MCS) The plasmid contains genes that can be used for selection such as
7、 Amp, Leu2, Ura3, or Trp1,Sample Plasmid,From Golemis Lab Homepage,False Positives,False positives are the largest problem with the yeast two-hybrid system Can be caused by: Non-specific binding of the prey Ability to induce transcription without interaction with the bait (Majority of false positive
8、s),Elimination of False Positives,Sequence Analysis Plasmid Loss Assays Retransformation of both strain with bait plasmid and strain without bait plasmid Test for interaction with an unrelated protein as bait Two (or more) step selections,Advantages,Immediate availability of the cloned gene of the i
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