Creating enzymes not found in nature

1. Creating enzymes not found in nature Burckhard Seelig University of Minnesota & Harvard Medical School

2. How to get new enzymes? • - Isolate enzymes from nature • - Enzyme engineering • Directed evolution, screen for modified properties • Design by computational methods • - Catalytic antibodies • Search in large libraries Library size ~ Probability of a hit

3. Outline: • Artificial ribozymes • Selection of proteins • De novo protein enzymes

4. RNA Genetic information & Catalytic properties (DNA / PCR) (Ribozymes) => Selections in RNA libraries possible

5. In vitro Selection of RNA (1014 molecules)

6. Diels-Alder Reaction * * - Central reaction in organic synthesis - Carbon - carbon bond formation / new stereo – centers *

7. Selection for Diels-Alderase Ribozymes - New selection scheme - Library of 2 x 1014 RNAs - 120 random nucleotides 10 cycles of selection and amplification

8. Diels-Alderase Ribozymes • 20,000 fold rate acceleration • Enantioselectivity > 95% ee • Minimal structural motif of 49 nucleotides Seelig B et. al. Angew. Chem. Int. Ed. 2000 (39) 4576-4579. Stucture: Serganov A et. al. Nat. Struct. Mol. Biol. 2005, 12,218-24.

9. Outline: • Artificial ribozymes • Selection of proteins • De novo protein enzymes Selection in Protein Libraries DNA => RNA => Protein

10. genotype phenotype Selections for Functional Proteins cell-based droplet-based phage- ribosome- mRNA- screen screen (IVC) display display display complexity~ 1013

11. P mRNA-Display Protein mRNA • Stable covalent link between protein and gene • Libraries of up to 1013 different proteins in a single tube • Selection of rare, functional molecules Roberts RW & Szostak JW, PNAS 1997(94) 12297.

12. P P Action of Puromycin messenger RNA ribosome Puromycin “Adenine” moiety “Tyrosine” moiety nascent protein P truncated protein

13. P P P P P mRNA-Display messenger RNA DNA Puromycin ribosome nascent protein P mRNA-displayed protein

14. Outline: • Artificial ribozymes • Selection of proteins • De novo protein enzymes How to Select for Enzymes ?

15. General Selection Scheme for Enzymes

16. Selection of RNA-RNA Ligases • No natural enzymes known • Artificial ribozymes and deoxyribozymes exist

17. Protein Library - Zinc-finger scaffold = common structural motif - Not taking part in catalysis in natural proteins - Library complexity: 3.9 x 1012 Library design & synthesis: Cho GS & Szostak JW, Chem. Biol. 2006 (13) 139.

18. Progress of in vitro Selection + Seelig B & Szostak JW, Nature 2007 (448) 228-31.

19. In vitro Evolution => 100 fold improvement

20. Induced Soluble FT Elution kDa: 45 30 20 14 Expression of Ligases in E.coli Ligases fused to maltose binding protein, purification on amylose column.

21. Activity of Free Enzyme 1 h 3 h 10 h No splint 5’-P 5’-HO * Product Substrate * Ligation of two RNA oligonucleotides by enzyme expressed in E.coli.

22. Rate Enhancement & Multiple Turnover Rate enhancements over uncatalyzed background rate > 2 x 106 fold.

23. Summary • Diels Alderase ribozymes from random RNA library • General scheme for selection of enzymes from • protein libraries > 1012 • Product formation as only selection criterion • Novel RNA-ligases from Zinc-finger library • Rate enhancements 2 x 106 fold + multiple turnover

24. Take home message: We can make new enzymes !

25. Acknowledgments Diels - Alderase Ribozyme Andres Jäschke and lab members DFG, BMBF Dept. ofBiochemistry, Free University of Berlin, Germany RNA - Ligase Jack W. Szostak and lab members, Glen Cho, Anthony D. Keefe, Glenn F. Short III, HHMI, NASA, DFG Dept. of Molecular Biology, Harvard Medical School