Analysis of solvent content and oligomeric states in protein crystals—does symmetry matter?

Chruszcz, M.; Potrzebowski, Wojciech; Zimmerman, Matthew D.; Grabowski, M.; Zheng, Heping; Lasota, Piotr; Minor, Władek

doi:10.1110/ps.073360508

Cited by 56 publications

(60 citation statements)

References 34 publications

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“…For the crystallographic structure and this model, the computed interaction energy per protein within the P321 structure was above that of the P6 structure, i.e., the calculation did not discern P321 as the preferred crystalline structure. The observed frequency of P321, however, is more than three times the frequency of P6 (21,40). In addition, P321 can accommodate deviations from the planar layering present in P6.…”

Section: Resultsmentioning

confidence: 85%

“…Glycine and small amino acids have been suggested to promote crystallization through the reduction of surface entropy (8,14,(52)(53)(54), and the presence of GX 3 G motifs at each protein-protein interface is consistent with a tightly packed crystal. Furthermore the volume per molecular weight (Matthew's coefficient) (55 (21). The solvent content (36%) is less than that observed for typical protein crystals (51%), hexagonal protein crystals (57%), and protein crystals with four polypeptide chains in the asymmetric unit (51%) (21,55,56).…”

Section: Resultsmentioning

confidence: 95%

“…Furthermore the volume per molecular weight (Matthew's coefficient) (55 (21). The solvent content (36%) is less than that observed for typical protein crystals (51%), hexagonal protein crystals (57%), and protein crystals with four polypeptide chains in the asymmetric unit (51%) (21,55,56).…”

Section: Resultsmentioning

confidence: 95%

“…1A) offers desirable features: (i) high symmetry, which can facilitate data collection and structure determination using X-ray crystallogra-phy, (ii) tubular solvent channels extending through the crystal, and (iii) polarity, i.e., large-scale parallel orientation of the proteins. Moreover, the P6 space group is one of the less common (2), occurring in only 0.1% of known protein crystal structures (21). Thus, achieving a designed crystal with P6 ordering is a stringent test of the approach.…”

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confidence: 99%

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Computational design of a protein crystal

Lanci

MacDermaid

Kang

et al. 2012

Proc. Natl. Acad. Sci. U.S.A.

157

162

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Protein crystals have catalytic and materials applications and are central to efforts in structural biology and therapeutic development. Designing predetermined crystal structures can be subtle given the complexity of proteins and the noncovalent interactions that govern crystallization. De novo protein design provides an approach to engineer highly complex nanoscale molecular structures, and often the positions of atoms can be programmed with sub-Å precision. Herein, a computational approach is presented for the design of proteins that self-assemble in three dimensions to yield macroscopic crystals. A three-helix coiled-coil protein is designed de novo to form a polar, layered, three-dimensional crystal having the P6 space group, which has a "honeycomb-like" structure and hexameric channels that span the crystal. The approach involves: (i) creating an ensemble of crystalline structures consistent with the targeted symmetry; (ii) characterizing this ensemble to identify "designable" structures from minima in the sequencestructure energy landscape and designing sequences for these structures; (iii) experimentally characterizing candidate proteins. A 2.1 Å resolution X-ray crystal structure of one such designed protein exhibits sub-Å agreement [backbone root mean square deviation (rmsd)] with the computational model of the crystal. This approach to crystal design has potential applications to the de novo design of nanostructured materials and to the modification of natural proteins to facilitate X-ray crystallographic analysis.M olecular design provides powerful tools for exploring how molecular properties dictate macroscopic structure and function. One of the most precise forms of self-organization, crystallization achieves orientation and symmetry across many length scales and can be leveraged to engineer materials with well-defined molecular order (1). In addition to their central role in structure determination, molecular crystals have many applications, including nanoparticle templating (2, 3), nonlinear optical devices (4), molecular scaffolding (5), and porous frameworks (6). A predictive understanding of how to achieve self-assembled macroscale structure and desired properties remains challenging, however, particularly when large, conformationally flexible molecules are employed.Small synthetic molecules have been designed that display complementary functional groups in a manner consistent with a chosen crystal structure. Intermolecular contacts are often patterned using strong, directional interactions (e.g., hydrogen bonding, metalcoordination, and electrostatic interactions) (7). The constituent molecules, however, are typically small and synthetic, thus limiting size, shape, and functionality. Hence, simultaneously achieving functional properties and the presentation of complementary intermolecular interactions that confer a targeted crystal structure can be difficult. Commonly, weak intermolecular forces stabilize crystalline ordering, and as a result, quantitative, predictive approaches to crystal de...

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Section: Resultsmentioning

confidence: 85%

Section: Resultsmentioning

confidence: 95%

Section: Resultsmentioning

confidence: 95%

mentioning

confidence: 99%

See 2 more Smart Citations

Computational design of a protein crystal

Lanci

MacDermaid

Kang

et al. 2012

Proc. Natl. Acad. Sci. U.S.A.

157

162

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show abstract

“…The lack of evolutionary pressure for proteins to crystallize indeed results in their crystals having most commonly the lowest-symmetry chiral (protein chains are chiral) point group compatible with that number of contacts, i.e., P2 1 2 1 2 1 [136]. Crystals of oligomeric proteins, for which evolution has shaped at least the oligomeric contacts, often assemble in complex asymmetric unit cells with more than ten distinct patches [137,138]. The competition between these interactions can favor the formation of small metastable crystallites, hindering the assembly of defectless crystals.…”

Section: A Simple Patchesmentioning

confidence: 99%

Soft matter perspective on protein crystal assembly

Fusco

Charbonneau

2016

Colloids and Surfaces B: Biointerfaces

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A structural and functional analysis of the glycosyltransferase BshA from Staphylococcus aureus: Insights into the reaction mechanism and regulation of bacillithiol production

Royer

Cook

2019

Protein Science

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Bacillithiol is a glucosamine‐derived antioxidant found in several pathogenic Gram‐positive bacteria. The compound is involved in maintaining the appropriate redox state within the cell as well as detoxifying foreign agents like the antibiotic fosfomycin. Bacillithiol is produced via the action of three enzymes, including BshA, a retaining GT‐B glycosyltransferase that utilizes UDP‐N‐acetylglucosamine and l‐malate to produce N‐acetylglucosaminyl‐malate. Recent studies suggest that retaining GT‐B glycosyltransferases like BshA utilize a substrate‐assisted mechanism that goes through an SNi‐like transition state. In a previous study, we relied on X‐ray crystallography as well as computational simulations to hypothesize the manner in which substrates would bind the enzyme, but several questions about substrate binding and the role of one of the amino acid residues persisted. Another study demonstrated that BshA might be subject to feedback inhibition by bacillithiol, but this phenomenon was not analyzed further to determine the exact mechanism of inhibition. Here we present X‐ray crystallographic structures and steady‐state kinetics results that help elucidate both of these issues. Our ligand‐bound crystal structures demonstrate that the active site provides an appropriate steric and geometric arrangement of ligands to facilitate the substrate‐assisted mechanism. Finally, we show that bacillithiol is competitive for UDP‐N‐acetylglucosamine with a Ki value near 120–130 μM and likely binds within the BshA active site, suggesting that bacillithiol modulates BshA activity via feedback inhibition. The work presented here furthers our understanding of bacillithiol metabolism and can aid in the development of inhibitors to counteract resistance to antibiotics such as fosfomycin.

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Analysis of solvent content and oligomeric states in protein crystals—does symmetry matter?

Cited by 56 publications

References 34 publications

Computational design of a protein crystal

Computational design of a protein crystal

Soft matter perspective on protein crystal assembly

A structural and functional analysis of the glycosyltransferase BshA from Staphylococcus aureus: Insights into the reaction mechanism and regulation of bacillithiol production

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