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Two-Hybrid Vector Systems Detection of Protein-Protein Interactions Protein-Protein Interactions • Essential role in most biological processes – – – – – – – – Signal transduction Cell growth and differentiation Gene expression Secretion Metabolishm DNA replication Transcription / translation / splictin Cell cycle control Functional Genomics • Protein kinases ( >2000); protein phosphatases (>1000); receptors; transcriptional regulators; signal transducers; etc.... • Signaling molecules play pivotal roles • Poor in vitro and in vivo function correlation's Protein-Protein Interaction Methods • Traditional biochemical methods – – – – Co-immunoprecipitation Protein crosslinking Co-purification Protein expression libraries • Two-Hybrid System – Protein folding and phosphorylation – No protein purification – Links genotype to phenotype Two-Hybrid Applications • Identify novel interacting proteins • Verify interactions determined by traditional methods • Drug screening • Functional mapping – domains / amino acids – post-translational modifications required Two-Hybrid Systems • Nuclear Yeast Systems – GAL4 – LexA • Membrane Yeast Systems – CytoTrap ….Sos recruitment system (SRS) Basics of Two-Hybrid Systems • cDNA vector – expresses random primed or oligo d(T) primed cDNA – expressed protein is the “PREY” or “Target” protein fused to a tranacriptional activation domain (GAL4 / LexA systems) or is myrstilated (Stratagene’s CytoTrap system) • Bait vector – expresses a known protein – expressed protein is chimeric, part is the known bait protein and part is a transcription factor DNA binding domain (GAL4 / Lex A systems), or hSos (CytoTrap) Nucleus 2. Target-AD hybrid protein binds to bait 1. Bait-DBD hybrid protein binds to DNA Bait DBD Target AD 3. Activation domain switches on transcription of reporter gene(s) HIS3 DNA Binding Site or b-gal 4. Yeast cells expressing target proteins that bind to bait grow on media lacking histidine and turn blue in the presence of X-gal GAL4 / LexA Considerations • Expression of hybrid proteins and localization to the nucleus • GAL4 fusion partner must not interfere with interactions • Neither hybrid can activate transcription of reporter gene without the other hybrid protein Limitations of GAL4 / LexA • Bait proteins which activate transcription of reporter genes in the absence of an interaction target protein can not be used. • Interactions must take place in the nucleus HybriZAP Vector System Advantages of l AD Vector • • • • Cloning efficiency is higher Background is lower No size bias with l (0 ~ 6 kb inserts) Pre-screening and screening for additional clones with traditional methods are easier • cDNA can be cloned directionally or nondirectional and random • In vivo excision to plasmid libraries is simple and fast HybriZAP EXCISION PROCESS HybriZAP XL1-Blue HybriZAP Packaged pAD-GAL4 Phagemid XLOLR Ex-Assist Helper Phage F pilus Ex-Assist Helper Phage F pilus a) Co-infection of XL1-Blue, SupE E.coli cells containing F’ episome coding for F pilus and bearing LamB receptors. b) Excision Process. HybriZAP, packaged pAD-GAL4 and packaged Helper Phage are produced. c) Infection of XLOLR, Su-, lr , F’ E.coli cells. Lambda phage cannot infect and Ex-Assist Helper Phage cannot replicate. d) Plate on Ampicillian plates. Resulting colonies contain pAD-GAL4 phagemid and insert DNA. Yeast YRG-2 Reporter Genes • LacZ • Histidine – GLA4 17 mer UAS – Sensitive – Easy and rapid assay • Filter lift • Quantitative liquid assay – Not selectable Endogenous GAL4 not expressed GAL 80 is mutated – – – – GAL1 UAS Very sensitive Selectable Not quantitative Frozen Competent Yeast Cells • thaw cells • add plasmid DNA • 30 minutes at 30oC, heat shock at 42oC for 8 min. • add SD broth, grow 1 hour at 30oC • pellet cells, resuspend, plate (3-7 days to get colonies) Stratagene’s GAL4 System • HybriZAP is l or plasmid based • Directional libraries, random nondirectional • Reporter genes integrated into YRG-2 • Vector kits, premade and custom cDNA libraries • Power of l, ease of plasmid • Increased relative size of the library • Available as high efficiency frozen cells • Flexible options /priced competitively Two-Hybrid Products (GAL4) • Complete HybriZAP 2.1 l kit – Digested l vector, Gigapack, competent E. coli, cDNA synthesis kit, control plasmids • Complete plasmid kit – Digested pAD-GAL4-2.1 vector, XL10-Gold Ultracompetent E. coli, cDNA synthesis kit, control plasmids, competent YRG-2 yeast • Custom and Premade libraries • Accessory kits CytoTrap Two-Hybrid System for the Detection of Protein-Protein Interactions CytoTrap customer • Is beginning a two-hybrid screen and isn’t sure if the bait needs glycosylation • Has wanted to screen with a protein that is a transcriptional activator or inhibitor....maybe a PathDetect customer? • Has been unsuccessful in a traditional two-hybrid screen Ras Activation Ras GTP Ras GDP P P SOS Greb2 In yeast, the Cdc25 protein has the same function as human SOS. Thus, hSOS can complement the yeast Cdc25 protein…. but if you remove the Greb-2 domain of SOS, it can not localize to the membrane to activate the Ras pathway CDC25H-2 Yeast Host • Genotype: MAT a, ura3, lys2, leu2, trp1, cdc25-2, his3D200, ade, Gal+ • Phenotype: Cdc25-2 yeast homologue of hSOS and is a guanyl nucleotide exchange factor (GEF) • cdc25-2 protein is thermostable at 25oC • cdc25-2 protein is not thermostable at 37oC 1. Target protein becomes anchored to cell membrane Myristylation Signal Target Cell Membrane GDP RAS Bait hSOS 2. Bait protein binds to target, localizing SOS to membrane GTP 3. SOS activates RAS by promoting GDP/GTP exchange 4. RAS activates signaling cascade that permits mutant yeast CDC25H-2 to grow at 37oC plasmid vector 5.6 kb U S pMyr EcoRI Srf I/I Sma Xho I Sal I Bait vector 11.3 kb S pSOS BamH I Nco I Srf I Aat I Sal I Mlu I BssH II Sac I Not I Sac II 2× Pac I Co-transform pADH-Sos Gal 4 AD Bait pGal1-Myr yeast cDNA library Select on -UL/Glu Plates @ 25oC 2 days Replica Plate on -UL/Gal Plates @37oC Patch “positive colonies” -UL/Glu 25oC 37oC No Interaction: Temp Revert: Interaction: + + + + - -UL/Gal 25oC + + + 37oC + 344+ 53 “positive” interaction clones selected Isolate pGal1 Myr yeast cDNA plasmid DNA Co-transform -UL/Gal 25oC 37oC pSOS GAL4: pSOS: + + + - Putative Positive Further Analysis CytoTrap products: • CytoTrap XR Library Construction Kit – – – – – – cDNA synthesis kit pMyr XR vector (Xho I and EcoRI digested) XL10-Gold ultracompetent cells pSos vector XL1-Blue subcloning competent cells cdc25H yeast strain CytoTrap products: • CytoTrap Vector Kit – – – – – • • • • pMyr vector (supercoiled) pSos vector (supercoiled) 2 positive control plasmids 2 negative control plasmids cdc25H yeast strain pMyr XR vector pMyr vector (supercoiled) pSos vector cdc25H yeast strain In Conclusion • Directional cloning / or random Eco RI cloning of cDNA • Exceptional premades available now • Brochure available • The CytoTrap system is the first is transcriptional activation independent yeast two-hybrid system Competition • Remember....CytoTrap is a completely different way to look for protein-protein interactions • Clontech Matchmaker systems – GAL4 and LexA • Invitrogen Hybrid Hunter – LexA • Other small companies...... Mammalian Two-Hybrid System More tools for functional genomics Why Mammalian? • Verification of mammalian interactions discovered in yeast • Proteins more likely to have native conformation • Results more likely to represent biologically significant interactions • Yeast do not phosphorylate tyrosine Nucleus Bait (X) Target (Y) NF-kB AD Gal4 BD pReporter Gal4 Gal4 Gal4 Gal4 Gal4 Figure 1 TATA Reporter Gene Why Nf-kB activation domain? pGal4BD NF-kB # 478 Gal4 (1-147) NF-kB (283-550) pGal4BD NF-kB # 476 Gal4 (1-147) NF-kB (364-550) pGal4BD NF-kB # 479 Gal4 (1-147) NF-kB (519-550) pGal4BD VP16 Gal4 (1-147) VP16 (411-455) Luciferase Activity (RLU) 18000000 16000000 14000000 12000000 10000000 8000000 6000000 4000000 2000000 0 Gal4BD-VP16 Gal4BD-NFkB 476 Gal4BD-NFkB 479 Gal4BD-NFkB 478 CHO 293 HeLa-luc CMV promoter ColE1 ori pAD NF-kB 4141 bps MCS AmpR SV40 poly(A) LoxP f1-ori BamHI SrfI EcoRI HindIII NotI Eco52I SalI XbaI XhoI CMV promoter Col E1 replication ori GAL4BD TK poly(A) signal MCS pBD 4598 bps SV40 poly (A) Neo/Kan f1(-) ori SV40 early promoter BamHI NheI SrfI SmaI XmaI EcoRI HindIII NotI AccI SalI XbaI PstI Ecl136II SacI Acc65I KpnI BglII HLR cell line 30000 25000 20000 15000 10000 5000 pBD-53 + pAD-TRAF2 pBD-CD40 + pAD-SV40 T pBD-53 + pAD-TRAF2 pBD-CD40 + pAD-SV40 T COS 2500000 2000000 1500000 1000000 500000 0 pBD-53 + pAD-TRAF2 pBD-CD40 + pAD-SV40 T pBD-53 + pAD-SV40 T Figure 4 293 2500000 2000000 1500000 1000000 500000 0 pBD-53 + pAD-SV40 T Luciferase Activity) 0 pBD-53 + pAD-SV40 T Luciferase Activity 0 CHO 14000000 12000000 10000000 8000000 6000000 4000000 2000000 Luciferase Activity Luciferase Activity Luciferase Activity ( Interaction between P53 and SV40T results in activation of luciferase activity pBD-53 + pAD-TRAF2 pBD-CD40 + pAD-SV40 T pBD-53 + pAD-SV40 T HeLa 60000 50000 40000 30000 20000 10000 0 pBD-53 + pAD-TRAF2 pBD-CD40 + pAD-SV40 T pBD-53 + pAD-SV40 T A Using different reporters SEAP SEAP Units 250000 200000 150000 100000 50000 0 pBD 53 + pAD TRAF2 pBD CD40 + pAD SV40 T pBD 53 + pAD SV40 T b-galactosidase Units b-Gal C 1.2 1 0.8 0.6 0.4 0.2 0 pBD 53 + pAD TRAF2 pBD CD40 + pAD SV40 T Figure 5 pBD 53 + pAD SV40 T Competition • Clontech – VP16 Activation Domain / CAT reporter • Promega CheckMate Mammalian TwoHybrid System – VP16 Activation Domain / dual Renilla and firefly Luciferase reporter • Stratagene Advantages – Increased activity of Nf-kB activator – Multiple reporter options Questions?