Abstract

Recent progress in this laboratory now makes it possible to attack some of the central questions of protein stability and function. How do weak bonding interactions form and stabilize protein structures? How do native proteins regulate their functions by making and breaking subsets of these same interactions. At present we know little about the parameters and principled involved. Advances in hydrogen exchange (HX)-based methods are uniquely able to probe these issues by resolving and measuring structural free energies and free energy changes. In the previous project period, we demonstrated the design and synthesis of a synthetic, stable, alpha-helical peptide that can see as a carrier onto which bonding interactions of various kinds can be built. We showed that the stabilization free energy of experimentally imposed interactions and their sites of action can then be determined from the NMR-detected hydrogen exchange behavior of the various peptide group NHs. We propose to use this system to evaluate, in a controlled context, the free energy of the many kinds of bonding interactions that proteins use to form and stabilize their structures. Proteins regulate their functions through structure change, i.e. by manipulating specific bonding interactions. For example, the archetypal allosteric protein, hemoglobin, controls the oxygen affinity of its heme groups by using part of the binding energy of its initial oxygen ligands to break bonding interactions that selectively stabilize its law affinity, T state. To understand how this energy interconversation process works, it will be necessary to locate the detailed changes in structure, measure their individual free energies, and quantify in free energy terms - how the different changes interact, how they add and subtract and transfer, to constitute the allosteric function. In the previous project period we demonstrated the unique ability of hydrogen exchange methods to locate and quantify site-resolved free energy and free energy, changes in hemoglobin. This work was limited by our available methodology to a small but important fraction of the protein. Work was done to develop the next generation of hydrogen exchange methods, involving both mass spectrometry and NMR, that will extend our HX labeling technology to the whole protein. We propose to complete this development and then to exploit these methods to learn how the allosteric machinery functions.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK011295-31
Application #
2443898
Study Section
Molecular and Cellular Biophysics Study Section (BBCA)
Project Start
1975-06-01
Project End
1999-06-30
Budget Start
1997-07-01
Budget End
1998-06-30
Support Year
31
Fiscal Year
1997
Total Cost
Indirect Cost

  Institution

Name
University of Pennsylvania
Department
Biochemistry
Type
Schools of Medicine
DUNS #
042250712
City
Philadelphia
State
PA
Country
United States
Zip Code
19104

  Publications

Englander, J J; Louie, G; McKinnie, R E et al. (1998) Energetic components of the allosteric machinery in hemoglobin measured by hydrogen exchange. J Mol Biol 284:1695-706
Milne, J S; Mayne, L; Roder, H et al. (1998) Determinants of protein hydrogen exchange studied in equine cytochrome c. Protein Sci 7:739-45
Englander, J J; Rumbley, J N; Englander, S W (1998) Signal transmission between subunits in the hemoglobin T-state. J Mol Biol 284:1707-16
Hiller, R; Zhou, Z H; Adams, M W et al. (1997) Stability and dynamics in a hyperthermophilic protein with melting temperature close to 200 degrees C. Proc Natl Acad Sci U S A 94:11329-32
Anni, H; Vanderkooi, J M; Mayne, L (1995) Structure of zinc-substituted cytochrome c: nuclear magnetic resonance and optical spectroscopic studies. Biochemistry 34:5744-53
Bai, Y; Englander, J J; Mayne, L et al. (1995) Thermodynamic parameters from hydrogen exchange measurements. Methods Enzymol 259:344-56
Sharp, K A; Englander, S W (1994) How much is a stabilizing bond worth? Trends Biochem Sci 19:526-9
Bai, Y; Englander, S W (1994) Hydrogen bond strength and beta-sheet propensities: the role of a side chain blocking effect. Proteins 18:262-6
Yu, K R; Hijikata, T; Lin, Z X et al. (1994) Truncated desmin in PtK2 cells induces desmin-vimentin-cytokeratin coprecipitation, involution of intermediate filament networks, and nuclear fragmentation: a model for many degenerative diseases. Proc Natl Acad Sci U S A 91:2497-501
Bai, Y; Milne, J S; Mayne, L et al. (1994) Protein stability parameters measured by hydrogen exchange. Proteins 20:4-14

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