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Various Strategies Used to Obtain Proteins for Crystallization and Biostructural Studies Dorothee Ambrosius, R. Engh, F. Hesse, M. Lanzendörfer, S. Palme, P. Rüger Roche Pharmaceutical Research, Penzberg. Protein Classes. extracellular proteins p lasma protein concentration:
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Various Strategies Used to Obtain Proteins for Crystallization and Biostructural Studies Dorothee Ambrosius, R. Engh, F. Hesse, M. Lanzendörfer, S. Palme, P. Rüger Roche Pharmaceutical Research, Penzberg
Protein Classes • extracellular proteins • plasma protein concentration: • 70 mg/ml • transporter (albumin) • immuno-globulin • enzymes, enzyme-inhibitors • coagulation factors, lipoproteins • protein characteristics/ • stability • often monomeric proteins • contain disulfide bridges • protease resistant • stable fold • intracellular proteins • cytoplasma and organelles: • 300-800 mg/ml • multi-enzyme complexes • enzyme cascades • transcription complexes • focal adhesion/integrins • cytoskeleton, heat-shock proteins • protein characteristics/stability • often multimeric complexes • no disulfide bridges • very labile proteins; short half-life • require stabilization: interaction with • other proteins
Biological Function of Cytokines G-CSF Neutrophils Source: Herrmann/Lederle
Development Goals for Recombinant Human G-CSF Hu-G-CSF: hematopoietic growth factor (174 aa) 2 S-S bridges, one single Cys 17 Clinical use: patients with neutropenia: after chemotherapy improved haemotopoietic recovery reduction of infectious risks native sequence: without additional N-terminal Met reduction of immunogenicity risk potency: equal to Amgen´s Neupogen low production cost: E. coli as host strain in vitro refolding consistent quality: robust downstream scheme analytical methods established
Strategy: Development of Recombinant Human G-CSF Fusion Peptide Human G-CSF • Fusion Peptide • high level expression • improved refolding • efficient separation of cleaved and uncleaved protein • optimized cleavage site • Protease • specific • efficient • recombinant • consistent quality • rhG-CSF • low production costs • without N-terminal Met • equal potency/efficiency • consistent quality • improved quality Genetic engineering of an economic downstream process
Optimization of rhG-CSF Fusion Proteins Fusion Peptide Met G-CSF Met-Thr-Pro-Leu G-CSF Met-Thr-Pro-Leu-His-His G-CSF Met-Thr-Pro-Leu-Lys-Lys G-CSF Met-Thr-Pro-Leu-Glu-Glu-Gly G-CSF Met-Thr-Pro-Leu-Glu-Glu-Gly-Thr-Pro-Leu G-CSF Met-Lys-Ala-Lys-Arg-Phe-Lys-Lys-His G-CSF Expression (%) 100 30 100 100 25 10 100 Cleavage - ++ ++ + +++ ++ +++ Renaturation (%) 10 20 20 50 90 80 80 Cleavage Site (Pro-Arg-Pro-Pro) Source: EP 92102864.3 ; DE 4104580
Refolding Kinetics of rhG-CSF Fusion Protein Solubilization 6,0 M Gdn/HCl, pH 8.0 100 mM Tris,/HCl 100 mM DTE 1 mM EDTA Temperature: RT c= 20 mg/ml Renaturation 0,8 M Arginine/HCl 100 mM Tris/HCl, pH 8.0 0.5 / 0.5 mM = GSH / GSSG 10 mM EDTA Temperature: RT Protein conc. 0.5 -1.0 mg /ml Time: 1- 2 hours native Pellet SN denat. Source: EP 92102864.3 ; DE 4104580
Role of p53 in cell cycle control:“guardian of the genome” h cell cycle arrest: repair defective genes active p53 latent p53 cell type level of p53 extent of DNA damage genetic background activation accumulation stress factors or oncogenic proteins mdm2 apoptosis: kill harmful deregulated cells negative feedback loop !!
Engineering of MDM2 for biostructural purposes The MDM2 oncoprotein is a cellular inhibitorof the p53 tumor suppressor. Goal: Improvement of biophysical properties of HDM2 (human MDM2) by “crystal engineering” Known: XDM2 (Xenopus laevis MDM2): - better solubility, suitable for biostructural investigations - wrong species and reduced binding affinity HDM2 (25-108): - high binding affinity to p53 peptide - prone to aggregation, not suitable for biostructural studies Strategy: use XDM2 as scaffold and humanize its p53-binding site introduce point mutations in HDM2 to increase solubility remove flexible ends at both sides of structured p53-binding region
17-29 p53 mdm2 26-108 Structure of MDM2/p53-peptide complex Figures taken from Kussie et al., Science274 (1996) 948. Resolution X-ray structures: human MDM2/p53: 2.6 Å Xenopus MDM2/p53: 2.3 Å
MDM2 variants created by protein engineering 1 26 108 125 185 240 300 330 350 440 491 human MDM2 p53 binding HDM2 (17-125) X-ray published HDM2 (25-108) X-ray HDM2 (25-108) mutants X-ray XDM2 (13-119) X-ray published, NMR XDM2 (13-119) LHI NMR, X-ray XDM2 (21-105) LHI X-ray P92H I50L L95I
Human MDM2: Yields & Upscale Step 15N-labeled non-labeled (LB) (minimal medium) Fermentation 10 L 10 L E. coli (wet weight) 90 g 600 g Inclusion bodies (w.w.) 3.5 g 85 g IB total protein content 1.3 g 30 g MDM2 (50-70% yield) 0.8 g 18 g Renaturation (~25%) 0.2 g 4.5 g MDM2 (Purification) 0.16 g 3.6 g Final product 0.1 g 2.2 g
Crystals of hXDM/peptide Patience might be rewarded Some crystals comply withcorporate identity rules hXDM2/phage-peptide hXDM2/p53 peptide Conditions: 0.1 M MES pH 6.2, 4.0 M NaOOCH 3 days after micro seeding at 13 °C4 months at 4 °C
Protein Kinase Families (incomplete list) I: Ser/Thr-Kinase Families Subfamilies/Structures Ia: Non Receptor Ser/Thr-Kinase familiy cAPK: cAMP dependent protein kinase PKA, PKB, PKC cdks: Cyclin dependent kinase cdk2, cdk4, cdk6 MAPK: Mitogen activated protein kinase Erk, Erk2, Jnk,p38(,,) MLCK: Myosine light chain kinase Twitchin, Titin CK: Casein kinase Ck-1, Ck-2 PhK: Phosphorylase kinase (tetramer: , , , )PhK CaMK: Calcium/calmodulin dependen kinase CaMK Ib: Receptor Ser/Thr-Kinase family TGF1-R Kinase TGF1-ßR II: Tyr-Kinase Families Subfamilies/Structures IIa: Non receptor Tyr-Kinase family SRC-family SRC, c-SRC, CSK, HCK LCK: humam lymphocyte kinase: LCK, c-Abl IIb: Receptor Tyr-Kinase family EGFR-family: EGFR, ErbB2-4 InsR-family IRK, IGF1R, IRR PDGFR-, CSFR-, Met-, Ron-familiy, FGF1-R, VEGFR-K EphA1….EphB1, Trk A, B, C, etc.
PKA: 2 Å X-ray Structure Further details for crystallization see poster of Ch. Breitenlechner
PKA: cyclic AMP Dependent Protein Kinase Expression: E. coli, solubly expressed in phosphorylated, active form 20-50 mg purified protein (10 l fermentation) Purification: affinity chromatography with inhibitory peptide (PKI) mimicking substrate binding Ref.: R. Engh & D. Bossemeyer, Adv. Enz. Reg. 41, 2001 Binding Affinity: 20 nM of inhibitory peptide (PKI) Protein: MW: 35 kDa Ser/The kinase monomeric 2 domain (C- and N-lobe) protein without additional regulatory domains (SH2, SH3, etc.) extended structured C- and N-Terminus, which possibly stabilizes the overall kinase structure Ideal model: Ser/Thr protein kinase inhibitor studies generation of other Ser/The kinase (e.g. PKB, Aurora) structures
Major Components of the Cell Cycle Machinery G0 • mitogen induced progression • through the cell cycle requires • timely controlled activation of • different cyclin-dependent • kinases (CDKs) • cyclins (D, E, A, B), periodically • expressed throughout the • cycle, are the regulatory • subunits of CDKs (activation) • members of the p16(INK4)- and • p21(KIP)-protein family inhibit • CDKs and CDK-cyclin complexes • and arrest inappropriate cell • cycle progression CDC2 INK4 M cyclin B Mitosis CDK4/6 cyclin D Cell Cycle G2 G1 CDC2 Kip/ Cip DNA Replication cyc. A/B CDK2 S cyclin E CDK2 cyclin A Kip/ Cip
Cyclin Dependent Kinases: CDK2 and CDK4/6 N. Pavletich, JMB 287, 821-828, 1999
Summary Proteins show a tremendous diversity with respect to - biological function and cellular location - structure, conformation and stability E. coli is a very attractive expression system with respect to time, yield, costs and production of isotope labeled proteins Application of in vitro protein refolding is a powerful tool to generate native structured proteins and should be considered as alternative The protein kinase family is regulated by multiple mechanism and show conformational diversity of catalytic cores; high degree of flexibility - e.g. IRK(3P) and LCK (Tyr kinases) show structural homology to cAPK and cdks (Ser/Thr kinases) Until today, most kinases successfully applied for structural research are expressed as active P--enzyme in baculo/insect cells; exception PKA
Acknowledgement PEX: S. Kanzler, H. Brandstetter (MPI) MDM2: G. Saalfrank, Ch. Breitenlechner (MPI), U. Jacob (MPI) IL-16: B. Essig , P. Mühlhahn (MPI), T. Holak (MPI) MIA: G. Saalfrank, C. Hergersberg, R. Stoll (MPI), T. Holak (MPI) cAPK: G. Achhammer, E. Liebig, Ch. Breitenlechner (MPI) cdks: H. Hertenberger, J. Kluge, U. Jucknischke G-CSF: S. Stammler, M. Leidenberger, U. Michaelis, T. Zink (MPI), T. Holak (MPI)