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2. Targeted Mutagenesis of the Multicopy Myrosinase Gene Family in Allotetraploid Brassica juncea Reduces Pungency in Fresh Leaves across Environments

Author

Dale Karlson, Julius P. Mojica, Thomas J. Poorten, Shai J. Lawit, Sathya Jali, Raj Deepika Chauhan, Gina M. Pham, Pradeep Marri, Sharon L. Guffy, Justin M. Fear, Cherie A. Ochsenfeld, Tracey A. (Lincoln) Chapman, Bruno Casamali, Jorge P. Venegas, Hae Jin Kim, Ashley Call, William L. Sublett, Lolita G. Mathew, Aabid Shariff, Joseph M. Watts, Mike Mann, Aaron Hummel, and Ryan Rapp

Subjects
Ecology, Plant Science, CRISPR-CAS, Brassica juncea, leafy green, Cas12a, myrosinase, mustard bomb, glucosinolate, nutrition, targeted mutagenesis, biotechnology, Ecology, Evolution, Behavior and Systematics
Abstract

Recent breeding efforts in Brassica have focused on the development of new oilseed feedstock crop for biofuels (e.g., ethanol, biodiesel, bio-jet fuel), bio-industrial uses (e.g., bio-plastics, lubricants), specialty fatty acids (e.g., erucic acid), and producing low glucosinolates levels for oilseed and feed meal production for animal consumption. We identified a novel opportunity to enhance the availability of nutritious, fresh leafy greens for human consumption. Here, we demonstrated the efficacy of disarming the ‘mustard bomb’ reaction in reducing pungency upon the mastication of fresh tissue—a major source of unpleasant flavor and/or odor in leafy Brassica. Using gene-specific mutagenesis via CRISPR-Cas12a, we created knockouts of all functional copies of the type-I myrosinase multigene family in tetraploid Brassica juncea. Our greenhouse and field trials demonstrate, via sensory and biochemical analyses, a stable reduction in pungency in edited plants across multiple environments. Collectively, these efforts provide a compelling path toward boosting the human consumption of nutrient-dense, fresh, leafy green vegetables.

Published
2022
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3. Targeted Mutagenesis of the Multicopy

Author

Dale, Karlson, Julius P, Mojica, Thomas J, Poorten, Shai J, Lawit, Sathya, Jali, Raj Deepika, Chauhan, Gina M, Pham, Pradeep, Marri, Sharon L, Guffy, Justin M, Fear, Cherie A, Ochsenfeld, Tracey A, Lincoln Chapman, Bruno, Casamali, Jorge P, Venegas, Hae Jin, Kim, Ashley, Call, William L, Sublett, Lolita G, Mathew, Aabid, Shariff, Joseph M, Watts, Mike, Mann, Aaron, Hummel, and Ryan, Rapp

Abstract

Recent breeding efforts in

Published
2022

4. Macromolecular modeling and design in Rosetta: recent methods and frameworks

Author

Jack Maguire, Ragul Gowthaman, Marion F. Sauer, Georg Kuenze, Tanja Kortemme, Benjamin Basanta, Indigo Chris King, Jens Meiler, Rhiju Das, Ora Schueler-Furman, Nicholas A. Marze, Brandon Frenz, Christoffer Norn, Julia Koehler Leman, Jason W. Labonte, Kala Bharath Pilla, Lei Shi, Sergey Lyskov, Brian D. Weitzner, Nir London, Karen R. Khar, Jaume Bonet, Nawsad Alam, Andreas Scheck, Alexander M. Sevy, Lars Malmström, Thomas Huber, Christopher Bystroff, Lior Zimmerman, Lorna Dsilva, Bruno E. Correia, Roland L. Dunbrack, Sergey Ovchinnikov, Rocco Moretti, Scott Horowitz, Phil Bradley, Frank DiMaio, Noah Ollikainen, Brian Kuhlman, Jeffrey J. Gray, Melanie L. Aprahamian, Andrew Leaver-Fay, Santrupti Nerli, Brian Koepnick, Xingjie Pan, Manasi A. Pethe, Andrew M. Watkins, Summer B. Thyme, Enrique Marcos, Vikram Khipple Mulligan, Hahnbeom Park, Po-Ssu Huang, David K. Johnson, Daniel-Adriano Silva, Patrick Barth, Shannon Smith, Caleb Geniesse, Jason K. Lai, Patrick Conway, Amelie Stein, Jeliazko R. Jeliazkov, David Baker, Dominik Gront, Kalli Kappel, Firas Khatib, Robert Kleffner, Brian J. Bender, Richard Bonneau, Kyle A. Barlow, Joseph H. Lubin, Shourya S. Roy Burman, Nikolaos G. Sgourakis, Yuval Sedan, Ryan E. Pavlovicz, Kristin Blacklock, Seth Cooper, Barak Raveh, Alisa Khramushin, John Karanicolas, Justin B. Siegel, Sharon L. Guffy, Brian G. Pierce, Alex Ford, Darwin Y. Fu, Orly Marcu, Gideon Lapidoth, Brian Coventry, René M. de Jong, Shane O’Conchúir, Thomas W. Linsky, William R. Schief, Rebecca F. Alford, Scott E. Boyken, Sagar D. Khare, Maria Szegedy, Ray Yu-Ruei Wang, Steven M. Lewis, Hamed Khakzad, Timothy M. Jacobs, Frank D. Teets, Lukasz Goldschmidt, Daisuke Kuroda, Steffen Lindert, P. Douglas Renfrew, Yifan Song, Jared Adolf-Bryfogle, Michael S. Pacella, and Aliza B. Rubenstein

Subjects
atomic-accuracy, Models, Molecular, Computer science, Macromolecular Substances, Protein Conformation, Interoperability, computational design, Score, antibody structures, Biochemistry, Article, homing endonuclease specificity, 03 medical and health sciences, Software, Molecular Biology, 030304 developmental biology, 0303 health sciences, business.industry, Proteins, Usability, fold determination, Cell Biology, Molecular Docking Simulation, variable region, Docking (molecular), protein-structure prediction, small-molecule docking, Modeling and design, Peptidomimetics, User interface, Software engineering, business, de-novo design, sparse nmr data, Biotechnology
Abstract

The Rosetta software for macromolecular modeling, docking and design is extensively used in laboratories worldwide. During two decades of development by a community of laboratories at more than 60 institutions, Rosetta has been continuously refactored and extended. Its advantages are its performance and interoperability between broad modeling capabilities. Here we review tools developed in the last 5 years, including over 80 methods. We discuss improvements to the score function, user interfaces and usability. Rosetta is available at ., This Perspective reviews tools developed over the past five years in the macromolecular modeling, docking and design software Rosetta.

Published
2019

5. Evolution of a highly active and enantiospecific metalloenzyme from short peptides

Author

Brian Kuhlman, Douglas A. Hansen, Bryan S. Der, Zbigniew Pianowski, Sabine Studer, Donald Hilvert, Aaron Debon, Peer R. E. Mittl, Sharon L. Guffy, University of Zurich, and Hilvert, Donald

Subjects
Stereochemistry, 610 Medicine & health, Peptide, 010402 general chemistry, Cleavage (embryo), 01 natural sciences, Evolution, Molecular, Metalloproteins, 10019 Department of Biochemistry, Enzyme kinetics, Catalytic efficiency, Simultaneous optimization, chemistry.chemical_classification, 1000 Multidisciplinary, Multidisciplinary, 010405 organic chemistry, Hydrolysis, Esters, Enzymes, 0104 chemical sciences, Structure and function, Zinc, Enzyme, chemistry, Biocatalysis, 570 Life sciences, biology, Directed Molecular Evolution, Oligopeptides
Abstract

Evolution trains a from-scratch catalyst Metal-bound peptides can catalyze simple reactions such as ester hydrolysis and may have been the starting point for the evolution of modern enzymes. Studer et al. selected progressively more-proficient variants of a small protein derived from a computationally designed zinc-binding peptide. The resulting enzyme could perform the trained reaction at rates typical for naturally evolved enzymes and serendipitously developed a strong preference for a single enantiomer of the substrate. A structure of the final catalyst highlights how small, progressive changes can remodel both catalytic residues and protein architecture in unpredictable ways. Science , this issue p. 1285

Published
2018

6. Protocols for Requirement-Driven Protein Design in the Rosetta Modeling Program

Author

Minnie I. Langlois, Brian Kuhlman, Sharon L. Guffy, and Frank D. Teets

Subjects
0301 basic medicine, Models, Molecular, Computer science, Interface (Java), General Chemical Engineering, Protein design, Library and Information Sciences, 010402 general chemistry, computer.software_genre, Ligands, 01 natural sciences, Protein Structure, Secondary, Article, Set (abstract data type), 03 medical and health sciences, Software, Protein structure, Binding Sites, business.industry, Programming language, Novel protein, Sequence optimization, Process (computing), Proteins, General Chemistry, 0104 chemical sciences, Computer Science Applications, 030104 developmental biology, ComputingMethodologies_PATTERNRECOGNITION, Drug Design, business, computer
Abstract

We have developed a set of protocols in the molecular modeling program Rosetta for performing requirement-driven protein design. First, the user specifies a set of structural features that need to be present in the designed protein. These requirements can be general (e.g., "create a protein with five helices"), or they can be very specific and require the correct placement of a set of amino acids to bind a ligand. Next, a large set of protein models are generated that satisfy the design requirements. The models are built using a method that we recently introduced into Rosetta, called SEWING, that rapidly assembles novel protein backbones by combining pieces of naturally occurring proteins. In the last step of the process, rotamer-based sequence optimization and backbone refinement are performed with Rosetta, and a variety of quality metrics are used to pick sequences for experimental characterization. Here we describe the input files and user options needed to run SEWING and perform requirement-driven design and provide detailed instructions for two specific applications of the process: the design of new structural elements at a protein-protein interface and the design of ligand binding sites.

Published
2018

7. An excited state underlies gene regulation of a transcriptional riboswitch

Author

Qi Zhang, Bo Zhao, Benfeard Williams, and Sharon L. Guffy

Subjects
0301 basic medicine, Riboswitch, Models, Molecular, Magnetic Resonance Spectroscopy, Transcription, Genetic, Base pair, Protein Conformation, Aptamer, 010402 general chemistry, 01 natural sciences, Article, 03 medical and health sciences, Fluorides, Bacillus cereus, Transcription (biology), Molecular Biology, Regulation of gene expression, Chemistry, RNA, Cell Biology, Ligand (biochemistry), 0104 chemical sciences, 030104 developmental biology, Cobalamin riboswitch, Gene Expression Regulation, Biophysics
Abstract

The use of chemical exchange saturation transfer NMR reveals a previously hidden excited conformational state of the fluoride riboswitch, providing a model in which ligand binding allosterically suppresses a linchpin base pair to activate transcription. Riboswitches control gene expression through ligand-dependent structural rearrangements of the sensing aptamer domain. However, we found that the Bacillus cereus fluoride riboswitch aptamer adopts identical tertiary structures in solution with and without ligand. Using chemical-exchange saturation transfer (CEST) NMR spectroscopy, we revealed that the structured ligand-free aptamer transiently accesses a low-populated (∼1%) and short-lived (∼3 ms) excited conformational state that unravels a conserved 'linchpin' base pair to signal transcription termination. Upon fluoride binding, this highly localized, fleeting process is allosterically suppressed, which activates transcription. We demonstrated that this mechanism confers effective fluoride-dependent gene activation over a wide range of transcription rates, which is essential for robust toxicity responses across diverse cellular conditions. These results unveil a novel switching mechanism that employs ligand-dependent suppression of an aptamer excited state to coordinate regulatory conformational transitions rather than adopting distinct aptamer ground-state tertiary architectures, exemplifying a new mode of ligand-dependent RNA regulation.

Published
2017

8. Probing the minimal determinants of zinc binding with computational protein design

Author

Brian Kuhlman, Bryan S. Der, and Sharon L. Guffy

Subjects
0301 basic medicine, Models, Molecular, Molecular model, Protein Conformation, Protein design, chemistry.chemical_element, Bioengineering, Zinc, 010402 general chemistry, Crystallography, X-Ray, Protein Engineering, 01 natural sciences, Biochemistry, 03 medical and health sciences, Protein structure, Point Mutation, Binding site, Molecular Biology, Binding Sites, Chemistry, Hydrogen bond, Proteins, Hydrogen Bonding, Protein engineering, 0104 chemical sciences, 030104 developmental biology, Biophysics, Original Article, Biotechnology, Binding domain
Abstract

Structure-based protein design tests our understanding of the minimal determinants of protein structure and function. Previous studies have demonstrated that placing zinc binding amino acids (His, Glu, Asp or Cys) near each other in a folded protein in an arrangement predicted to be tetrahedral is often sufficient to achieve binding to zinc. However, few designs have been characterized with high-resolution structures. Here, we use X-ray crystallography, binding studies and mutation analysis to evaluate three alternative strategies for designing zinc binding sites with the molecular modeling program Rosetta. While several of the designs were observed to bind zinc, crystal structures of two designs reveal binding configurations that differ from the design model. In both cases, the modeling did not accurately capture the presence or absence of second-shell hydrogen bonds critical in determining binding-site structure. Efforts to more explicitly design second-shell hydrogen bonds were largely unsuccessful as evidenced by mutation analysis and low expression of proteins engineered with extensive primary and secondary networks. Our results suggest that improved methods for designing interaction networks will be needed for creating metal binding sites with high accuracy.

Published
2016

9. A novel intracellular fibulin-1D variant binds to the cytoplasmic domain of integrin beta 1 subunit

Author

William Scott Argraves, Waleed O. Twal, Sharon L. Guffy, and Samar M. Hammad

Subjects
Protein subunit, Placenta, Integrin, CD18, CHO Cells, CD49c, Article, Collagen receptor, Cricetulus, Pregnancy, Animals, Humans, Protein Isoforms, Molecular Biology, Cells, Cultured, biology, Integrin beta1, Calcium-Binding Proteins, Molecular biology, Cell biology, Alternative Splicing, Integrin alpha M, biology.protein, Integrin, beta 6, Female, ITGA6, Integrin alpha5beta1
Abstract

Fibulin-1 is a member of a growing family of proteins that includes eight members and is involved in cellular functions such as adhesion, migration and differentiation. Fibulin-1 has also been implicated in embryonic development of the heart and neural crest-derived structures. It is an integral part of the extracellular matrix (ECM) and has been shown to bind to a multitude of ECM proteins. However, fibulin-1 was first identified as a protein purified from placental extracts that binds to the cytoplasmic domain of integrin β1. Human fibulin-1 is alternatively spliced into four different isoforms namely A-D. These isoforms share a common N-terminus sequence that contains a secretion sequence but differ in their carboxy-terminal fibulin-1 module. In this report we identify a new splice variant of fibulin-1 that differs from all other fibulin-1 variants in the N-terminus sequence and has a similar carboxy-terminus sequence as fibulin-1D. This variant that we named fibulin-1D prime (fibulin-1D’) lacks a secretion sequence and the anaphlatoxin region of fibulin-1 variants. The protein has an apparent molecular weight of 70.5 kDa. Herein we show that fibulin-1D’ binds to the intracellular domain of integrin β1 as well as to integrin α5β1. The protein was localized intracellularly in CHO cells transfected with a pEF4 plasmid containing full-length coding sequence of fibulin-1D’. We also localized the protein in human placenta. We propose that the fibulin-1D’ variant might play a role in early embryo development as well as in modulating integrin β1 functions including adhesion and motility.

Published
2014

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