Abstract

Protein homologues often have common functions, with variation evolving via amino acid substitutions at specificity determinants (SDs). These residues may be located in binding sites or other """"""""long-range"""""""" regions of the protein. Predicting SDs is a current target of bioinformatics sequence analyses. Our long- term goal is to experimentally identify long-range SDs in the Lacl/GaIR family;the proposed work focuses on SDs in the linker that connects the DMA-binding domain to the regulatory domain. Hypotheses are derived from 4 different prediction strategies, which are only in partial agreement with each other. The common function of the Lacl/GaIR proteins - transcription control - allows """"""""moderate through-put"""""""" assays of function so that all predictions may be compared. We will test hypotheses in multiple homologues to address the question: Do homologues utilize all SDs available to the common fold (a frequent assumption of prediction algorithms) or do different functions require only a subset of potential SDs? Further, the aspect of function affected by changing an SD cannot yet be reliably predicted, nor is it clear whether a functional change for one SD is the same in all homologues. Our experiments will monitor different aspects of Lacl/GaIR function, including DMA specificity, DNA affinity, and allosteric response to binding regulatory effector molecules. Proposed experiments utilize chimeras comprising the Lacl DMA-binding domain and regulatory domains from E. coli paralogues. Linkers come from Lacl or paralogues. Since each naturally-occurring Lacl/GaIR protein recognizes a different DNA ligand, the common DNA-binding domain allows us to more easily parse functional contributions from binding site and long-range SDs. By definition, making an amino acid substitu- tion at an SD will change function. We will use in vivo repression/response to effector and in vitro thermody- namic measurements of affinity/allosteric response to characterize the chimeras and potential SD variants. Specificity for alternative DNA ligands will be determined. Experiments are designed to answer the following questions:
Aim 1 : Can one linker facilitate allosteric communication with a variety of regulatory domains? [or do altered linker SD interactions abolish this function?] Aim 2: What are the functional contributions from specific positions in the linker? Aim 3: Can knowledge of SDs [in one linker] be used to transplant lacO1 DNA-binding to other linkers? Results will: (1) Identify the locations of SDs and determine if they make similar functional contributions to several homologues;(2) Yield a list of empirical rules for creating novel Lacl/GaIR proteins with biotechnological utility via domain recombination;and (3) Test the current prediction algorithms and generate a new sequence/function database for improving predictions. This work will facilitate expanded use of data generated by the Human Genome Project.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM079423-05
Application #
8122158
Study Section
Macromolecular Structure and Function B Study Section (MSFB)
Program Officer
Preusch, Peter C
Project Start
2007-08-01
Project End
2013-07-31
Budget Start
2011-08-01
Budget End
2013-07-31
Support Year
5
Fiscal Year
2011
Total Cost
$259,334
Indirect Cost

  Institution

Name
University of Kansas
Department
Biochemistry
Type
Schools of Medicine
DUNS #
016060860
City
Kansas City
State
KS
Country
United States
Zip Code
66160

  Publications

Sousa, Filipa L; Parente, Daniel J; Hessman, Jacob A et al. (2016) Data on publications, structural analyses, and queries used to build and utilize the AlloRep database. Data Brief 8:948-57
Sousa, Filipa L; Parente, Daniel J; Shis, David L et al. (2016) AlloRep: A Repository of Sequence, Structural and Mutagenesis Data for the LacI/GalR Transcription Regulators. J Mol Biol 428:671-678
Parente, Daniel J; Ray, J Christian J; Swint-Kruse, Liskin (2015) Amino acid positions subject to multiple coevolutionary constraints can be robustly identified by their eigenvector network centrality scores. Proteins 83:2293-306
Shis, David L; Hussain, Faiza; Meinhardt, Sarah et al. (2014) Modular, multi-input transcriptional logic gating with orthogonal LacI/GalR family chimeras. ACS Synth Biol 3:645-51
Parente, Daniel J; Swint-Kruse, Liskin (2013) Multiple co-evolutionary networks are supported by the common tertiary scaffold of the LacI/GalR proteins. PLoS One 8:e84398
Meinhardt, Sarah; Manley Jr, Michael W; Becker, Nicole A et al. (2012) Novel insights from hybrid LacI/GalR proteins: family-wide functional attributes and biologically significant variation in transcription repression. Nucleic Acids Res 40:11139-54
Tungtur, Sudheer; Skinner, Harlyn; Zhan, Hongli et al. (2011) In vivo tests of thermodynamic models of transcription repressor function. Biophys Chem 159:142-51
Tungtur, Sudheer; Parente, Daniel J; Swint-Kruse, Liskin (2011) Functionally important positions can comprise the majority of a protein's architecture. Proteins 79:1589-608
Tungtur, Sudheer; Meinhardt, Sarah; Swint-Kruse, Liskin (2010) Comparing the functional roles of nonconserved sequence positions in homologous transcription repressors: implications for sequence/function analyses. J Mol Biol 395:785-802
Swint-Kruse, Liskin; Matthews, Kathleen S (2009) Allostery in the LacI/GalR family: variations on a theme. Curr Opin Microbiol 12:129-37

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