Your search keyword '"Miller, Mitchell D."' showing total 617 results

201. Using Electrostatics to Define the Active Site of Serratia Endonuclease.

Author

Walker, John M., Schein, Catherine H., Krause, Kurt L., and Miller, Mitchell D.

Abstract

The location of an enzyme's active site is usually known prior to the determination of its three-dimensional structure. Analysis of sequence homology may indicate residues that are near an enzyme's active site. Catalytic residues are often identified when site-directed mutagenesis experiments or chemical modification of residues lead to an alteration in enzyme activity. The enzyme's three-dimensional (3D) structure is then used to supplement and interpret preceding experimental data. Occasionally, a new protein structure is solved before the active site has been located through conventional methods. Using the extracellular endonuclease from Serratia marcescens as an example, we show here how the active site of an enzyme can sometimes be determined from electrostatic analysis of its 3D structure (1). [ABSTRACT FROM AUTHOR]

Published

2001

202. Deep learning-based prediction of electron density maps of proteins

Author

Pan, Tom, Jin, Shikai, Miller, Mitchell D., and Phillips, George N.

Published

2022

203. Crystal structures of three representatives of a new Pfam family PF14869 (DUF4488) suggest they function in sugar binding/uptake.

Author

Kumar, Abhinav, Punta, Marco, Axelrod, Herbert L., Das, Debanu, Farr, Carol L., Grant, Joanna C., Chiu, Hsiu‐Ju, Miller, Mitchell D., Coggill, Penelope C., Klock, Heath E., Elsliger, Marc‐André, Deacon, Ashley M., Godzik, Adam, Lesley, Scott A., and Wilson, Ian A.

Abstract

Crystal structures of three members (BACOVA_00364 from Bacteroides ovatus, BACUNI_03039 from Bacteroides uniformis and BACEGG_00036 from Bacteroides eggerthii) of the Pfam domain of unknown function (DUF4488) were determined to 1.95, 1.66, and 1.81 Å resolutions, respectively. The protein structures adopt an eight-stranded, calycin-like, β-barrel fold and bind an endogenous unknown ligand at one end of the β-barrel. The amino acids interacting with the ligand are not conserved in any other protein of known structure with this particular fold. The size and chemical environment of the bound ligand suggest binding or transport of a small polar molecule(s) as a potential function for these proteins. These are the first structural representatives of a newly defined PF14869 (DUF4488) Pfam family. [ABSTRACT FROM AUTHOR]

Published

2014

204. Structural analysis of arabinose-5-phosphate isomerase from Bacteroides fragilis and functional implications.

Author

Chiu, Hsiu-Ju, Grant, Joanna C., Farr, Carol L., Jaroszewski, Lukasz, Knuth, Mark W., Miller, Mitchell D., Elsliger, Marc-André, Deacon, Ashley M., Godzik, Adam, Lesley, Scott A., and Wilson, Ian A.

Subjects

STRUCTURAL analysis (Science), ARABINOSE, ISOMERASES, BACTEROIDES fragilis, CRYSTAL structure, ISOMERIZATION, BIOSYNTHESIS, MONOMERS

Abstract

The crystal structure of arabinose-5-phosphate isomerase (API) from Bacteroides fragilis (bfAPI) was determined at 1.7 Å resolution and was found to be a tetramer of a single-domain sugar isomerase (SIS) with an endogenous ligand, CMP-Kdo (cytidine 5′-monophosphate-3-deoxy-D-manno-oct-2-ulosonate), bound at the active site. API catalyzes the reversible isomerization of D-ribulose 5-phosphate to D-arabinose 5-phosphate in the first step of the Kdo biosynthetic pathway. Interestingly, the bound CMP-Kdo is neither the substrate nor the product of the reaction catalyzed by API, but corresponds to the end product in the Kdo biosynthetic pathway and presumably acts as a feedback inhibitor for bfAPI. The active site of each monomer is located in a surface cleft at the tetramer interface between three monomers and consists of His79 and His186 from two different adjacent monomers and a Ser/Thr-rich region, all of which are highly conserved across APIs. Structure and sequence analyses indicate that His79 and His186 may play important catalytic roles in the isomerization reaction. CMP-Kdo mimetics could therefore serve as potent and specific inhibitors of API and provide broad protection against many different bacterial infections. [ABSTRACT FROM AUTHOR]

Published

2014

205. Molecular characterization of novel pyridoxal-5′-phosphate-dependent enzymes from the human microbiome.

Author

Fleischman, Nicholas M., Das, Debanu, Kumar, Abhinav, Xu, Qingping, Chiu, Hsiu‐Ju, Jaroszewski, Lukasz, Knuth, Mark W., Klock, Heath E., Miller, Mitchell D., Elsliger, Marc‐André, Godzik, Adam, Lesley, Scott A., Deacon, Ashley M., Wilson, Ian A., and Toney, Michael D.

Abstract

Pyridoxal-5′-phosphate or PLP, the active form of vitamin B6, is a highly versatile cofactor that participates in a large number of mechanistically diverse enzymatic reactions in basic metabolism. PLP-dependent enzymes account for ∼1.5% of most prokaryotic genomes and are estimated to be involved in ∼4% of all catalytic reactions, making this an important class of enzymes. Here, we structurally and functionally characterize three novel PLP-dependent enzymes from bacteria in the human microbiome: two are from Eubacterium rectale, a dominant, nonpathogenic, fecal, Gram-positive bacteria, and the third is from Porphyromonas gingivalis, which plays a major role in human periodontal disease. All adopt the Type I PLP-dependent enzyme fold and structure-guided biochemical analysis enabled functional assignments as tryptophan, aromatic, and probable phosphoserine aminotransferases. [ABSTRACT FROM AUTHOR]

Published

2014

206. Crystal structure of a putative quorum sensing-regulated protein (PA3611) from the Pseudomonas-specific DUF4146 family.

Author

Das, Debanu, Chiu, Hsiu‐Ju, Farr, Carol L., Grant, Joanna C., Jaroszewski, Lukasz, Knuth, Mark W., Miller, Mitchell D., Tien, Henry J., Elsliger, Marc‐André, Deacon, Ashley M., Godzik, Adam, Lesley, Scott A., and Wilson, Ian A.

Abstract

ABSTRACT Pseudomonas aeruginosa is an opportunistic pathogen commonly found in humans and other organisms and is an important cause of infection especially in patients with compromised immune defense mechanisms. The PA3611 gene of P. aeruginosa PAO1 encodes a secreted protein of unknown function, which has been recently classified into a small Pseudomonas-specific protein family called DUF4146. As part of our effort to extend structural coverage of novel protein space and provide a structure-based functional insight into new protein families, we report the crystal structure of PA3611, the first structural representative of the DUF4146 protein family. Proteins 2014; 82:1086-1092. © 2013 Wiley Periodicals, Inc. [ABSTRACT FROM AUTHOR]

Published

2014

207. Crystal structure of a member of a novel family of dioxygenases (PF10014) reveals a conserved cupin fold and active site.

Author

Xu, Qingping, Grant, Joanna, Chiu, Hsiu‐Ju, Farr, Carol L., Jaroszewski, Lukasz, Knuth, Mark W., Miller, Mitchell D., Lesley, Scott A., Godzik, Adam, Elsliger, Marc‐André, Deacon, Ashley M., and Wilson, Ian A.

Abstract

ABSTRACT PF10014 is a novel family of 2-oxyglutarate-Fe2+-dependent dioxygenases that are involved in biosynthesis of antibiotics and regulation of biofilm formation, likely by catalyzing hydroxylation of free amino acids or other related ligands. The crystal structure of a PF10014 member from Methylibium petroleiphilum at 1.9 Å resolution shows strong structural similarity to cupin dioxygenases in overall fold and active site, despite very remote homology. However, one of the β-strands of the cupin catalytic core is replaced by a loop that displays conformational isomerism that likely regulates the active site. Proteins 2014; 82:164-170. © 2013 Wiley Periodicals, Inc. [ABSTRACT FROM AUTHOR]

Published

2014

208. The active site of Serratia endonuclease contains a conserved magnesium-water cluster

Author

Miller, Mitchell D., primary, Cai, Jiwen, additional, and Krause, Kurt L., additional

Published

1999

209. Stereochemical π-Facial Selectivity of the Diels−Alder Reaction of Benz[a]aceanthrylene and 1,4-Diphenylbenz[a]aceanthrylene

Author

Plummer, Benjamin F., primary, Faiz, Saadia, additional, Wiederhold, Ted, additional, Wooten, Marilyn, additional, Agyin, Joseph K., additional, Krause, Kurt L., additional, Miller, Mitchell D., additional, and Watson, William H., additional

Published

1997

210. Simulation of electrostatic and hydrodynamic properties ofSerratia endonuclease

Author

Antosiewicz, Jan, primary, Miller, Mitchell D., additional, Krause, Kurt L., additional, and McCammon, J. Andrew, additional

Published

1997

211. Structure of Bacterial Luciferase β2 Homodimer: Implications for Flavin Binding,

Author

Tanner, John J., primary, Miller, Mitchell D., additional, Wilson, Keith S., additional, Tu, Shiao-Chun, additional, and Krause, Kurt L., additional

Published

1997

212. Chemical Generation of C602- and Electron Transfer Mechanism for the Reactions with Alkyl Bromides

Author

Subramanian, Ramakrishnan, primary, Kadish, Karl M., additional, Vijayashree, Madakasira N., additional, Gao, Xiang, additional, Jones, M. Thomas, additional, Miller, Mitchell D., additional, Krause, Kurt L., additional, Suenobu, Tomoyoshi, additional, and Fukuzumi, Shunichi, additional

Published

1996

213. Identification of theSerratiaendonuclease dimer: Structural basis and implications for catalysis

Author

Miller, Mitchell D., primary and Krause, Kurt L., additional

Published

1996

214. 2.1 Å structure of Serratia endonuclease suggests a mechanism for binding to double-stranded DNA

Author

Miller, Mitchell D., primary, Tanner, Jack, additional, Alpaugh, Mary, additional, Benedik, Michael J., additional, and Krause, Kurt L., additional

Published

1994

215. Structure of an MmyB-Like Regulator from C. aurantiacus, Member of a New Transcription Factor Family Linked to Antibiotic Metabolism in Actinomycetes.

Author

Qingping Xu, van Wezel, Gilles P., Hsiu-Ju Chiu, Jaroszewski, Lukasz, Klock, Heath E., Knuth, Mark W., Miller, Mitchell D., Lesley, Scott A., Godzik, Adam, Elsliger, Marc-André, Deacon, Ashley M., and Wilson, Ian A.

Subjects

ACTINOMYCETALES, TRANSCRIPTION factors, ACTINOBACTERIA, HEREDITY, ANTI-infective agents

Abstract

Actinomycetes are important bacterial sources of antibiotics and other secondary metabolites. Many antibiotic gene clusters are controlled by pathway-specific activators that act in response to growth conditions. Here we present the crystal structure of an MmyB-like transcription regulator MltR (PDB code 3pxp) (Caur_2278) from Chloroflexus aurantiacus, in complex with a fatty acid (myristic acid). MltR is a distant homolog of the methylenomycin activator MmyB and consists of an Xre-type N-terminal DNA-binding domain and a C-terminal ligand-binding module that is related to the Per-Arnt-Sim (PAS) domain. This structure has enabled identification of a new family of bacterial transcription factors that are distributed predominantly in actinomycetes. Bioinformatics analysis of MltR and other characterized family members suggest that they are likely associated with antibiotic and fatty acid metabolism in actinomycetes. Streptomyces coelicolor SCO4944 is a candidate as an ancestral member of the family. Its ortholog in S. griseus, SGR_6891, is induced by A-factor, a γ-butyrolactone that controls antibiotic production and development, and is adjacent to the A-factor synthase gen, afsA. The location of mltR/mmyB homologs, in particular those adjacent to less well-studied antibiotic-related genes, makes them interesting genetic markers for identifying new antibiotic genes. A model for signal-triggered DNA-binding by MltR is proposed. [ABSTRACT FROM AUTHOR]

Published

2012

216. Structure of the pilus assembly protein TadZ from Eubacterium rectale: implications for polar localization.

Author

Xu, Qingping, Christen, Beat, Chiu, Hsiu-Ju, Jaroszewski, Lukasz, Klock, Heath E., Knuth, Mark W., Miller, Mitchell D., Elsliger, Marc-André, Deacon, Ashley M., Godzik, Adam, Lesley, Scott A., Figurski, David H., Shapiro, Lucy, and Wilson, Ian A.

Subjects

PILI (Microbiology), EUBACTERIALES, ADENOSINE triphosphatase, CAULOBACTER crescentus, MITOCHONDRIA formation

Abstract

Summary The tad (tight adherence) locus encodes a protein translocation system that produces a novel variant of type IV pili. The pilus assembly protein TadZ (called CpaE in Caulobacter crescentus) is ubiquitous in tad loci, but is absent in other type IV pilus biogenesis systems. The crystal structure of TadZ from Eubacterium rectale (ErTadZ), in complex with ATP and Mg2+, was determined to 2.1 Å resolution. ErTadZ contains an atypical ATPase domain with a variant of a deviant Walker-A motif that retains ATP binding capacity while displaying only low intrinsic ATPase activity. The bound ATP plays an important role in dimerization of ErTadZ. The N-terminal atypical receiver domain resembles the canonical receiver domain of response regulators, but has a degenerate, stripped-down 'active site'. Homology modelling of the N-terminal atypical receiver domain of CpaE indicates that it has a conserved protein-protein binding surface similar to that of the polar localization module of the social mobility protein FrzS, suggesting a similar function. Our structural results also suggest that TadZ localizes to the pole through the atypical receiver domain during an early stage of pili biogenesis, and functions as a hub for recruiting other pili components, thus providing insights into the Tad pilus assembly process. [ABSTRACT FROM AUTHOR]

Published

2012

217. Structural Analysis of Papain-Like NlpC/P60 Superfamily Enzymes with a Circularly Permuted Topology Reveals Potential Lipid Binding Sites.

Author

Qingping Xu, Rawlings, Neil D., Hsiu-Ju Chiu, Jaroszewski, Lukasz, Klock, Heath E., Knuth, Mark W., Miller, Mitchell D., Elsliger, Marc-Andre, Deacon, Ashley M., Godzik, Adam, Lesley, Scott A., and Wilson, Ian A.

Subjects

ENZYME analysis, PAPAIN, GENETICS, TOPOLOGY, CYSTEINE, PATHOGENIC bacteria, BACILLUS cereus, TYROSINE

Abstract

NlpC/P60 superfamily papain-like enzymes play important roles in all kingdoms of life. Two members of this superfamily, LRAT-like and YaeF/YiiX-like families, were predicted to contain a catalytic domain that is circularly permuted such that the catalytic cysteine is located near the C-terminus, instead of at the N-terminus. These permuted enzymes are widespread in virus, pathogenic bacteria, and eukaryotes. We determined the crystal structure of a member of the YaeF/YiiX-like family from Bacillus cereus in complex with lysine. The structure, which adopts a ligand-induced, ''closed'' conformation, confirms the circular permutation of catalytic residues. A comparative analysis of other related protein structures within the NlpC/P60 superfamily is presented. Permutated NlpC/P60 enzymes contain a similar conserved core and arrangement of catalytic residues, including a Cys/His-containing triad and an additional conserved tyrosine. More surprisingly, permuted enzymes have a hydrophobic S1 binding pocket that is distinct from previously characterized enzymes in the family, indicative of novel substrate specificity. Further analysis of a structural homolog, YiiX (PDB 2if6) identified a fatty acid in the conserved hydrophobic pocket, thus providing additional insights into possible function of these novel enzymes. [ABSTRACT FROM AUTHOR]

Published

2011

218. Structural and Sequence Analysis of Imelysin-Like Proteins Implicated in Bacterial Iron Uptake.

Author

Qingping Xu, Rawlings, Neil D., Farr, Carol L., Hsiu-Ju Chiu, Grant, Joanna C., Jaroszewski, Lukasz, Klock, Heath E., Knuth, Mark W., Miller, Mitchell D., Weekes, Dana, Elsliger, Marc-André, Deacon, Ashley M., Godzik, Adam, Lesley, Scott A., and Wilson, Ian A.

Subjects

PROTEIN structure, AMINO acid sequence, BACTERIAL proteins, IRON content of bacteria, PEPTIDASE, CRYSTAL structure, TOPOLOGY

Abstract

Imelysin-like proteins define a superfamily of bacterial proteins that are likely involved in iron uptake. Members of this superfamily were previously thought to be peptidases and were included in the MEROPS family M75. We determined the first crystal structures of two remotely related, imelysin-like proteins. The Psychrobacter arcticus structure was determined at 2.15 Å resolution and contains the canonical imelysin fold, while higher resolution structures from the gut bacteria Bacteroides ovatus, in two crystal forms (at 1.25 Å and 1.44 Å resolution), have a circularly permuted topology. Both structures are highly similar to each other despite low sequence similarity and circular permutation. The all-helical structure can be divided into two similar four-helix bundle domains. The overall structure and the GxHxxE motif region differ from known HxxE metallopeptidases, suggesting that imelysin-like proteins are not peptidases. A putative functional site is located at the domain interface. We have now organized the known homologous proteins into a superfamily, which can be separated into four families. These families share a similar functional site, but each has family-specific structural and sequence features. These results indicate that imelysin-like proteins have evolved from a common ancestor, and likely have a conserved function. [ABSTRACT FROM AUTHOR]

Published

2011

219. Structure and Function of the First Full-Length Murein Peptide Ligase (Mpl) Cell Wall Recycling Protein.

Author

Debanu Das, Hervé, Mireille, Feuerhelm, Julie, Farr, Carol L., Hsiu-Ju Chiu, Elsliger, Marc-André, Knuth, Mark W., Klock, Heath E., Miller, Mitchell D., Godzik, Adam, Lesley, Scott A., Deacon, Ashley M., Mengin-Lecreulx, Dominique, and Wilson, Ian A.

Subjects

PEPTIDOGLYCANS, LIGASES, BACTERIAL cell walls, X-ray crystallography, HYDROGEN-ion concentration, PHARMACEUTICAL research

Abstract

Bacterial cell walls contain peptidoglycan, an essential polymer made by enzymes in the Mur pathway. These proteins are specific to bacteria, which make them targets for drug discovery. MurC, MurD, MurE and MurF catalyze the synthesis of the peptidoglycan precursor UDP-N-acetylmuramoyl-L-alanyl-γ-D-glutamyl-meso-diaminopimelyl-D-alanyl-D-alanine by the sequential addition of amino acids onto UDP-N-acetylmuramic acid (UDP-MurNAc). MurC-F enzymes have been extensively studied by biochemistry and X-ray crystallography. In Gram-negative bacteria, ∼30-60% of the bacterial cell wall is recycled during each generation. Part of this recycling process involves the murein peptide ligase (Mpl), which attaches the breakdown product, the tripeptide L-alanyl-γ-D-glutamyl-meso-diaminopimelate, to UDP-MurNAc. We present the crystal structure at 1.65 Å resolution of a full-length Mpl from the permafrost bacterium Psychrobacter arcticus 273-4 (PaMpl). Although the Mpl structure has similarities to Mur enzymes, it has unique sequence and structure features that are likely related to its role in cell wall recycling, a function that differentiates it from the MurC-F enzymes. We have analyzed the sequence-structure relationships that are unique to Mpl proteins and compared them to MurC-F ligases. We have also characterized the biochemical properties of this enzyme (optimal temperature, pH and magnesium binding profiles and kinetic parameters). Although the structure does not contain any bound substrates, we have identified ∼30 residues that are likely to be important for recognition of the tripeptide and UDP-MurNAc substrates, as well as features that are unique to Psychrobacter Mpl proteins. These results provide the basis for future mutational studies for more extensive function characterization of the Mpl sequence-structure relationships. [ABSTRACT FROM AUTHOR]

Published

2011

220. Structure of the first representative of Pfam family PF04016 (DUF364) reveals enolase and Rossmann-like folds that combine to form a unique active site with a possible role in heavy-metal chelation.

Author

Miller, Mitchell D., Aravind, L., Bakolitsa, Constantina, Rife, Christopher L., Carlton, Dennis, Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Chiu, Hsiu-Ju, Clayton, Thomas, Deller, Marc C., Duan, Lian, Feuerhelm, Julie, Grant, Joanna C., Han, Gye Won, Jaroszewski, Lukasz, Jin, Kevin K., Klock, Heath E., Knuth, Mark W., and Kozbial, Piotr

Subjects

*CRYSTAL structure research, *ENOLASE, *STRUCTURAL genomics, *PROTEIN structure, *BIOINFORMATICS, *METHYLTRANSFERASES, *CHELATION

Abstract

The crystal structure of Dhaf4260 from Desulfitobacterium hafniense DCB-2 was determined by single-wavelength anomalous diffraction (SAD) to a resolution of 2.01 Å using the semi-automated high-throughput pipeline of the Joint Center for Structural Genomics (JCSG) as part of the NIGMS Protein Structure Initiative (PSI). This protein structure is the first representative of the PF04016 (DUF364) Pfam family and reveals a novel combination of two well known domains (an enolase N-terminal-like fold followed by a Rossmann-like domain). Structural and bioinformatic analyses reveal partial similarities to Rossmann-like methyltransferases, with residues from the enolase-like fold combining to form a unique active site that is likely to be involved in the condensation or hydrolysis of molecules implicated in the synthesis of flavins, pterins or other siderophores. The genome context of Dhaf4260 and homologs additionally supports a role in heavy-metal chelation. [ABSTRACT FROM AUTHOR]

Published

2010

221. The structure of Jann_2411 (DUF1470) from Jannaschia sp. at 1.45 Å resolution reveals a new fold (the ABATE domain) and suggests its possible role as a transcription regulator.

Author

Bakolitsa, Constantina, Bateman, Alex, Jin, Kevin K., McMullan, Daniel, Krishna, S. Sri, Miller, Mitchell D., Abdubek, Polat, Acosta, Claire, Astakhova, Tamara, Axelrod, Herbert L., Burra, Prasad, Carlton, Dennis, Chiu, Hsiu-Ju, Clayton, Thomas, Das, Debanu, Deller, Marc C., Duan, Lian, Elias, Ylva, Feuerhelm, Julie, and Grant, Joanna C.

Subjects

CRYSTAL structure research, PROTEIN research, STRUCTURAL analysis (Science), LIGANDS (Chemistry), ZINC-finger proteins, DNA-binding proteins

Abstract

The crystal structure of Jann_2411 from Jannaschia sp. strain CCS1, a member of the Pfam PF07336 family classified as a domain of unknown function (DUF1470), was solved to a resolution of 1.45 Å by multiple-wavelength anomalous dispersion (MAD). This protein is the first structural representative of the DUF1470 Pfam family. Structural analysis revealed a two-domain organization, with the N-terminal domain presenting a new fold called the ABATE domain that may bind an as yet unknown ligand. The C-terminal domain forms a treble-clef zinc finger that is likely to be involved in DNA binding. Analysis of the Jann_2411 protein and the broader ABATE-domain family suggests a role as stress-induced transcriptional regulators. [ABSTRACT FROM AUTHOR]

Published

2010

222. Conformational changes associated with the binding of zinc acetate at the putative active site of XcTcmJ, a cupin from Xanthomonas campestris pv. campestris.

Author

Axelrod, Herbert L., Kozbial, Piotr, McMullan, Daniel, Krishna, S. Sri, Miller, Mitchell D., Abdubek, Polat, Acosta, Claire, Astakhova, Tamara, Carlton, Dennis, Caruthers, Jonathan, Chiu, Hsiu-Ju, Clayton, Thomas, Deller, Marc C., Duan, Lian, Elias, Ylva, Feuerhelm, Julie, Grzechnik, Slawomir K., Grant, Joanna C., Han, Gye Won, and Jaroszewski, Lukasz

Subjects

ZINC acetate, XANTHOMONAS campestris, PROTEINS, CUPINS, METAL ions

Abstract

In the plant pathogen Xanthomonas campestris pv. campestris, the product of the tcmJ gene, XcTcmJ, encodes a protein belonging to the RmlC family of cupins. XcTcmJ was crystallized in a monoclinic space group ( C2) in the presence of zinc acetate and the structure was determined to 1.6 Å resolution. Previously, the apo structure has been reported in the absence of any bound metal ion [Chin et al. (2006), Proteins, 65, 1046-1050]. The most significant difference between the apo structure and the structure of XcTcmJ described here is a reorganization of the binding site for zinc acetate, which was most likely acquired from the crystallization solution. This site is located in the conserved metal ion-binding domain at the putative active site of XcTcmJ. In addition, an acetate was also bound within coordination distance of the zinc. In order to accommodate this binding, rearrangement of a conserved histidine ligand is required as well as several nearby residues within and around the putative active site. These observations indicate that binding of zinc serves a functional role in this cupin protein. [ABSTRACT FROM AUTHOR]

Published

2010

223. The structure of the first representative of Pfam family PF06475 reveals a new fold with possible involvement in glycolipid metabolism.

Author

Bakolitsa, Constantina, Kumar, Abhinav, McMullan, Daniel, Krishna, S. Sri, Miller, Mitchell D., Carlton, Dennis, Najmanovich, Rafael, Abdubek, Polat, Astakhova, Tamara, Chiu, Hsiu-Ju, Clayton, Thomas, Deller, Marc C., Duan, Lian, Elias, Ylva, Feuerhelm, Julie, Grant, Joanna C., Grzechnik, Slawomir K., Han, Gye Won, Jaroszewski, Lukasz, and Jin, Kevin K.

Subjects

CRYSTAL structure research, PSEUDOMONAS aeruginosa, METABOLISM, PROTEIN folding, LIPOPROTEINS, BACTERIAL cell walls

Abstract

The crystal structure of PA1994 from Pseudomonas aeruginosa, a member of the Pfam PF06475 family classified as a domain of unknown function (DUF1089), reveals a novel fold comprising a 15-stranded β-sheet wrapped around a single α-helix that assembles into a tight dimeric arrangement. The remote structural similarity to lipoprotein localization factors, in addition to the presence of an acidic pocket that is conserved in DUF1089 homologs, phospholipid-binding and sugar-binding proteins, indicate a role for PA1994 and the DUF1089 family in glycolipid metabolism. Genome-context analysis lends further support to the involvement of this family of proteins in glycolipid metabolism and indicates possible activation of DUF1089 homologs under conditions of bacterial cell-wall stress or host-pathogen interactions. [ABSTRACT FROM AUTHOR]

Published

2010

224. Structure of an essential bacterial protein YeaZ (TM0874) from Thermotoga maritima at 2.5 Å resolution.

Author

Xu, Qingping, McMullan, Daniel, Jaroszewski, Lukasz, Krishna, S. Sri, Elsliger, Marc-André, Yeh, Andrew P., Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Carlton, Dennis, Chiu, Hsiu-Ju, Clayton, Thomas, Duan, Lian, Feuerhelm, Julie, Grant, Joanna, Han, Gye Won, Jin, Kevin K., Klock, Heath E., Knuth, Mark W., and Miller, Mitchell D.

Subjects

CRYSTAL structure research, BACTERIAL proteins, THERMOTOGA maritima, PROTEINS, ACTIN

Abstract

YeaZ is involved in a protein network that is essential for bacteria. The crystal structure of YeaZ from Thermotoga maritima was determined to 2.5 Å resolution. Although this protein belongs to a family of ancient actin-like ATPases, it appears that it has lost the ability to bind ATP since it lacks some key structural features that are important for interaction with ATP. A conserved surface was identified, supporting its role in the formation of protein complexes. [ABSTRACT FROM AUTHOR]

Published

2010

225. Structure of LP2179, the first representative of Pfam family PF08866, suggests a new fold with a role in amino-acid metabolism.

Author

Bakolitsa, Constantina, Kumar, Abhinav, Carlton, Dennis, Miller, Mitchell D., Krishna, S. Sri, Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Chiu, Hsiu-Ju, Clayton, Thomas, Deller, Marc C., Duan, Lian, Elsliger, Marc-André, Feuerhelm, Julie, Grzechnik, Slawomir K., Grant, Joanna C., Han, Gye Won, Jaroszewski, Lukasz, Jin, Kevin K., and Klock, Heath E.

Subjects

CRYSTAL structure research, BACILLUS (Bacteria), PROTEIN folding, AMINO acid metabolism, PROTEINS, ADENOSYLMETHIONINE decarboxylase, GENOMICS

Abstract

The structure of LP2179, a member of the PF08866 (DUF1831) family, suggests a novel α+β fold comprising two β-sheets packed against a single helix. A remote structural similarity to two other uncharacterized protein families specific to the Bacillus genus (PF08868 and PF08968), as well as to prokaryotic S-adenosylmethionine decarboxylases, is consistent with a role in amino-acid metabolism. Genomic neighborhood analysis of LP2179 supports this functional assignment, which might also then be extended to PF08868 and PF08968. [ABSTRACT FROM AUTHOR]

Published

2010

226. Structure of the first representative of Pfam family PF09410 (DUF2006) reveals a structural signature of the calycin superfamily that suggests a role in lipid metabolism.

Author

Chiu, Hsiu-Ju, Bakolitsa, Constantina, Skerra, Arne, Lomize, Andrei, Carlton, Dennis, Miller, Mitchell D., Krishna, S. Sri, Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Clayton, Thomas, Deller, Marc C., Duan, Lian, Feuerhelm, Julie, Grant, Joanna C., Grzechnik, Slawomir K., Han, Gye Won, Jaroszewski, Lukasz, Jin, Kevin K., and Klock, Heath E.

Subjects

CRYSTAL structure research, PROTEIN research, LIPID metabolism, LIGANDS (Chemistry), LIPOCALINS

Abstract

The first structural representative of the domain of unknown function DUF2006 family, also known as Pfam family PF09410, comprises a lipocalin-like fold with domain duplication. The finding of the calycin signature in the N-terminal domain, combined with remote sequence similarity to two other protein families (PF07143 and PF08622) implicated in isoprenoid metabolism and the oxidative stress response, support an involvement in lipid metabolism. Clusters of conserved residues that interact with ligand mimetics suggest that the binding and regulation sites map to the N-terminal domain and to the interdomain interface, respectively. [ABSTRACT FROM AUTHOR]

Published

2010

227. Open and closed conformations of two SpoIIAA-like proteins (YP_749275.1 and YP_001095227.1) provide insights into membrane association and ligand binding.

Author

Kumar, Abhinav, Lomize, Andrei, Jin, Kevin K., Carlton, Dennis, Miller, Mitchell D., Jaroszewski, Lukasz, Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Chiu, Hsiu-Ju, Clayton, Thomas, Das, Debanu, Deller, Marc C., Duan, Lian, Feuerhelm, Julie, Grant, Joanna C., Grzechnik, Anna, Han, Gye Won, Klock, Heath E., and Knuth, Mark W.

Subjects

CRYSTAL structure research, SHEWANELLA, PROTEINS, BACTERIAL proteins, HYDROPHOBIC surfaces

Abstract

The crystal structures of the proteins encoded by the YP_749275.1 and YP_001095227.1 genes from Shewanella frigidimarina and S. loihica, respectively, have been determined at 1.8 and 2.25 Å resolution, respectively. These proteins are members of a novel family of bacterial proteins that adopt the α/β SpoIIAA-like fold found in STAS and CRAL-TRIO domains. Despite sharing 54% sequence identity, these two proteins adopt distinct conformations arising from different dispositions of their α2 and α3 helices. In the `open' conformation (YP_001095227.1), these helices are 15 Å apart, leading to the creation of a deep nonpolar cavity. In the `closed' structure (YP_749275.1), the helices partially unfold and rearrange, occluding the cavity and decreasing the solvent-exposed hydrophobic surface. These two complementary structures are reminiscent of the conformational switch in CRAL-TRIO carriers of hydrophobic compounds. It is suggested that both proteins may associate with the lipid bilayer in their `open' monomeric state by inserting their amphiphilic helices, α2 and α3, into the lipid bilayer. These bacterial proteins may function as carriers of nonpolar substances or as interfacially activated enzymes. [ABSTRACT FROM AUTHOR]

Published

2010

228. The structure of BVU2987 from Bacteroides vulgatus reveals a superfamily of bacterial periplasmic proteins with possible inhibitory function.

Author

Das, Debanu, Finn, Robert D., Carlton, Dennis, Miller, Mitchell D., Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Bakolitsa, Constantina, Chen, Connie, Chiu, Hsiu-Ju, Chiu, Michelle, Clayton, Thomas, Deller, Marc C., Duan, Lian, Ellrott, Kyle, Ernst, Dustin, Farr, Carol L., Feuerhelm, Julie, Grant, Joanna C., and Grzechnik, Anna

Subjects

CRYSTAL structure research, BACTEROIDES, PROTEINS, MICROORGANISMS, BETA-lactamase inhibitors

Abstract

Proteins that contain the DUF2874 domain constitute a new Pfam family PF11396. Members of this family have predominantly been identified in microbes found in the human gut and oral cavity. The crystal structure of one member of this family, BVU2987 from Bacteroides vulgatus, has been determined, revealing a β-lactamase inhibitor protein-like structure with a tandem repeat of domains. Sequence analysis and structural comparisons reveal that BVU2987 and other DUF2874 proteins are related to β-lactamase inhibitor protein, PepSY and SmpA_OmlA proteins and hence are likely to function as inhibitory proteins. [ABSTRACT FROM AUTHOR]

Published

2010

229. The structure of the first representative of Pfam family PF09836 reveals a two-domain organization and suggests involvement in transcriptional regulation.

Author

Das, Debanu, Grishin, Nick V., Kumar, Abhinav, Carlton, Dennis, Bakolitsa, Constantina, Miller, Mitchell D., Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Burra, Prasad, Chen, Connie, Chiu, Hsiu-Ju, Chiu, Michelle, Clayton, Thomas, Deller, Marc C., Duan, Lian, Ellrott, Kyle, Ernst, Dustin, Farr, Carol L., and Feuerhelm, Julie

Subjects

CRYSTAL structure research, PROTEIN research, NEISSERIA gonorrhoeae, DNA-binding proteins, GENOMICS

Abstract

Proteins with the DUF2063 domain constitute a new Pfam family, PF09836. The crystal structure of a member of this family, NGO1945 from Neisseria gonorrhoeae, has been determined and reveals that the N-terminal DUF2063 domain is likely to be a DNA-binding domain. In conjunction with the rest of the protein, NGO1945 is likely to be involved in transcriptional regulation, which is consistent with genomic neighborhood analysis. Of the 216 currently known proteins that contain a DUF2063 domain, the most significant sequence homologs of NGO1945 (∼40-99% sequence identity) are from various Neisseria and Haemophilus species. As these are important human pathogens, NGO1945 represents an interesting candidate for further exploration via biochemical studies and possible therapeutic intervention. [ABSTRACT FROM AUTHOR]

Published

2010

230. Structures of the first representatives of Pfam family PF06684 (DUF1185) reveal a novel variant of the Bacillus chorismate mutase fold and suggest a role in amino-acid metabolism.

Author

Bakolitsa, Constantina, Kumar, Abhinav, Jin, Kevin K., McMullan, Daniel, Krishna, S. Sri, Miller, Mitchell D., Abdubek, Polat, Acosta, Claire, Astakhova, Tamara, Axelrod, Herbert L., Burra, Prasad, Carlton, Dennis, Chen, Connie, Chiu, Hsiu-Ju, Clayton, Thomas, Das, Debanu, Deller, Marc C., Duan, Lian, Elias, Ylva, and Ellrott, Kyle

Subjects

CRYSTAL structure research, BACILLUS (Bacteria), MUTASES, AMINO acid metabolism, WAVELENGTHS, STRUCTURAL genomics, PROTEIN structure

Abstract

The crystal structures of BB2672 and SPO0826 were determined to resolutions of 1.7 and 2.1 Å by single-wavelength anomalous dispersion and multiple-wavelength anomalous dispersion, respectively, using the semi-automated high-throughput pipeline of the Joint Center for Structural Genomics (JCSG) as part of the NIGMS Protein Structure Initiative (PSI). These proteins are the first structural representatives of the PF06684 (DUF1185) Pfam family. Structural analysis revealed that both structures adopt a variant of the Bacillus chorismate mutase fold (BCM). The biological unit of both proteins is a hexamer and analysis of homologs indicates that the oligomer interface residues are highly conserved. The conformation of the critical regions for oligomerization appears to be dependent on pH or salt concentration, suggesting that this protein might be subject to environmental regulation. Structural similarities to BCM and genome-context analysis suggest a function in amino-acid synthesis. [ABSTRACT FROM AUTHOR]

Published

2010

231. Structures of the first representatives of Pfam family PF06938 (DUF1285) reveal a new fold with repeated structural motifs and possible involvement in signal transduction.

Author

Han, Gye Won, Bakolitsa, Constantina, Miller, Mitchell D., Kumar, Abhinav, Carlton, Dennis, Najmanovich, Rafael J., Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L., Chen, Connie, Chiu, Hsiu-Ju, Clayton, Thomas, Das, Debanu, Deller, Marc C., Duan, Lian, Ernst, Dustin, Feuerhelm, Julie, Grant, Joanna C., Grzechnik, Anna, and Jaroszewski, Lukasz

Subjects

CRYSTAL structure research, CELLULAR signal transduction, GENOMICS, PROTEIN structure, HOMOLOGY (Biology), NUCLEOTIDES

Abstract

The crystal structures of SPO0140 and Sbal_2486 were determined using the semiautomated high-throughput pipeline of the Joint Center for Structural Genomics (JCSG) as part of the NIGMS Protein Structure Initiative (PSI). The structures revealed a conserved core with domain duplication and a superficial similarity of the C-terminal domain to pleckstrin homology-like folds. The conservation of the domain interface indicates a potential binding site that is likely to involve a nucleotide-based ligand, with genome-context and gene-fusion analyses additionally supporting a role for this family in signal transduction, possibly during oxidative stress. [ABSTRACT FROM AUTHOR]

Published

2010

232. The structure of SSO2064, the first representative of Pfam family PF01796, reveals a novel two-domain zinc-ribbon OB-fold architecture with a potential acyl-CoA-binding role.

Author

Krishna, S. Sri, Aravind, L., Bakolitsa, Constantina, Caruthers, Jonathan, Carlton, Dennis, Miller, Mitchell D., Abdubek, Polat, Astakhova, Tamara, Axelrod, Herbert L, Chiu, Hsiu-Ju, Clayton, Thomas, Deller, Marc C., Duan, Lian, Feuerhelm, Julie, Grant, Joanna C., Han, Gye Won, Jaroszewski, Lukasz, Jin, Kevin K., Klock, Heath E., and Knuth, Mark W.

Subjects

CRYSTAL structure research, PROKARYOTIC genomes, STRUCTURAL genomics, PHYLOGENY, RUBREDOXINS, OLIGONUCLEOTIDES, N-terminal residues, PROTEIN-protein interactions

Abstract

SSO2064 is the first structural representative of PF01796 (DUF35), a large prokaryotic family with a wide phylogenetic distribution. The structure reveals a novel two-domain architecture comprising an N-terminal, rubredoxin-like, zinc ribbon and a C-terminal, oligonucleotide/oligosaccharide-binding (OB) fold domain. Additional N-terminal helical segments may be involved in protein-protein interactions. Domain architectures, genomic context analysis and functional evidence from certain bacterial representatives of this family suggest that these proteins form a novel fatty-acid-binding component that is involved in the biosynthesis of lipids and polyketide antibiotics and that they possibly function as acyl-CoA-binding proteins. This structure has led to a re-evaluation of the DUF35 family, which has now been split into two entries in the latest Pfam release (v.24.0). [ABSTRACT FROM AUTHOR]

Published

2010

233. Genomics, evolution, and crystal structure of a new family of bacterial spore kinases.

Author

Scheeff, Eric D., Axelrod, Herbert L., Miller, Mitchell D., Chiu, Hsiu-Ju, Deacon, Ashley M., Wilson, Ian A., and Manning, Gerard

Abstract

Bacterial spore formation is a complex process of fundamental relevance to biology and human disease. The spore coat structure is complex and poorly understood, and the roles of many of the protein components remain unclear. We describe a new family of spore coat proteins, the bacterial spore kinases (BSKs), and the first crystal structure of a BSK, YtaA (CotI) from Bacillus subtilis. BSKs are widely distributed in spore-forming Bacillus and Clostridium species, and have a dynamic evolutionary history. Sequence and structure analyses indicate that the BSKs are CAKs, a prevalent group of small molecule kinases in bacteria that is distantly related to the eukaryotic protein kinases. YtaA has substantial structural similarity to CAKs, but also displays distinctive features that broaden our understanding of the CAK group. Evolutionary constraint analysis of the protein surfaces indicates that members of the BSK family have distinct clade-conserved patterns in the substrate binding region, and probably bind and phosphorylate distinct targets. Several classes of BSKs have apparently independently lost catalytic activity to become pseudokinases, indicating that the family also has a major noncatalytic function. Proteins 2010. © 2009 Wiley-Liss, Inc. [ABSTRACT FROM AUTHOR]

Published

2010

234. Crystallization and preliminary crystallographic analysis of a novel nuclease from Serratia marcescens

Author

Miller, Mitchell D., primary, Benedik, Michael J., additional, Sullivan, Merry C., additional, Shipley, Nancy S., additional, and Krause, Kurt L., additional

Published

1991

235. Crystal structure of a novel Sm-like protein of putative cyanophage origin at 2.60 Å resolution.

Author

Das, Debanu, Kozbial, Piotr, Axelrod, Herbert L., Miller, Mitchell D., McMullan, Daniel, Krishna, S. Sri, Abdubek, Polat, Acosta, Claire, Astakhova, Tamara, Burra, Prasad, Carlton, Dennis, Chen, Connie, Chiu, Hsiu-Ju, Clayton, Thomas, Deller, Marc C., Duan, Lian, Elias, Ylva, Elsliger, Marc-André, Ernst, Dustin, and Farr, Carol

Abstract

ECX21941 represents a very large family (over 600 members) of novel, ocean metagenome-specific proteins identified by clustering of the dataset from the Global Ocean Sampling expedition. The crystal structure of ECX21941 reveals unexpected similarity to Sm/LSm proteins, which are important RNA-binding proteins, despite no detectable sequence similarity. The ECX21941 protein assembles as a homopentamer in solution and in the crystal structure when expressed in Escherichia coli and represents the first pentameric structure for this Sm/LSm family of proteins, although the actual oligomeric form in vivo is currently not known. The genomic neighborhood analysis of ECX21941 and its homologs combined with sequence similarity searches suggest a cyanophage origin for this protein. The specific functions of members of this family are unknown, but our structure analysis of ECX21941 indicates nucleic acid-binding capabilities and suggests a role in RNA and/or DNA processing. Proteins 2009. © 2008 Wiley-Liss, Inc. [ABSTRACT FROM AUTHOR]

Published

2009

236. Crystal structure of the Fic (Filamentation induced by cAMP) family protein SO4266 (gi|24375750) from Shewanella oneidensis MR-1 at 1.6 Å resolution.

Author

Das, Debanu, Krishna, S. Sri, McMullan, Daniel, Miller, Mitchell D., Xu, Qingping, Abdubek, Polat, Acosta, Claire, Astakhova, Tamara, Axelrod, Herbert L., Burra, Prasad, Carlton, Dennis, Chiu, Hsiu-Ju, Clayton, Thomas, Deller, Marc C., Duan, Lian, Elias, Ylva, Elsliger, Marc-André, Ernst, Dustin, Feuerhelm, Julie, and Grzechnik, Anna

Published

2009

237. Crystal structure of a novel archaeal AAA+ ATPase SSO1545 from Sulfolobus solfataricus.

Author

Xu, Qingping, Rife, Christopher L., Carlton, Dennis, Miller, Mitchell D., Krishna, S. Sri, Elsliger, Marc-André, Abdubek, Polat, Astakhova, Tamara, Chiu, Hsiu-Ju, Clayton, Thomas, Duan, Lian, Feuerhelm, Julie, Grzechnik, Slawomir K., Hale, Joanna, Han, Gye Won, Jaroszewski, Lukasz, Jin, Kevin K., Klock, Heath E., Knuth, Mark W., and Kumar, Abhinav

Published

2009

238. Crystal structure of AICAR transformylase IMP cyclohydrolase (TM1249) from Thermotoga maritima at 1.88 Å resolution.

Author

Axelrod, Herbert L., McMullan, Daniel, Krishna, S. Sri, Miller, Mitchell D., Elsliger, Marc-Andre, Abdubek, Polat, Ambing, Eileen, Astakhova, Tamara, Carlton, Dennis, Chiu, Hsiu-Ju, Clayton, Thomas, Duan, Lian, Feuerhelm, Julie, Grzechnik, Slawomir K., Hale, Joanna, Han, Gye Won, Haugen, Justin, Jaroszewski, Lukasz, Jin, Kevin K., and Klock, Heath E.

Published

2008

239. Crystal structure of 2-keto-3-deoxygluconate kinase (TM0067) from Thermotoga maritima at 2.05 Å resolution.

Author

Mathews, Irimpan I., McMullan, Daniel, Miller, Mitchell D., Canaves, Jaume M., Elsliger, Marc-André, Floyd, Ross, Grzechnik, Slawomir K., Jaroszewski, Lukasz, Klock, Heath E., Koesema, Eric, Kovarik, John S., Kreusch, Andreas, Kuhn, Peter, McPhillips, Timothy M., Morse, Andrew T., Quijano, Kevin, Rife, Christopher L., Schwarzenbacher, Robert, Spraggon, Glen, and Stevens, Raymond C.

Published

2008

240. Crystal structure of 2-phosphosulfolactate phosphatase (ComB) from Clostridium acetobutylicum at 2.6 Å resolution reveals a new fold with a novel active site.

Author

DiDonato, Michael, Krishna, S. Sri, Schwarzenbacher, Robert, McMullan, Daniel, Agarwalla, Sanjay, Brittain, Scott M., Miller, Mitchell D., Abdubek, Polat, Ambing, Eileen, Axelrod, Herbert L., Canaves, Jaume M., Chiu, Hsiu-Ju, Deacon, Ashley M., Duan, Lian, Elsliger, Marc-André, Godzik, Adam, Grzechnik, Slawomir K., Hale, Joanna, Hampton, Eric, and Haugen, Justin

Published

2006

241. Crystal structure of an ORFan protein (TM1622) from Thermotoga maritima at 1.75 Å resolution reveals a fold similar to the Ran-binding protein Mog1p.

Author

Xu, Qingping, Krishna, S. Sri, McMullan, Daniel, Schwarzenbacher, Robert, Miller, Mitchell D., Abdubek, Polat, Agarwalla, Sanjay, Ambing, Eileen, Astakhova, Tamara, Axelrod, Herbert L., Canaves, Jaume M., Carlton, Dennis, Chiu, Hsiu-Ju, Clayton, Thomas, DiDonato, Michael, Duan, Lian, Elsliger, Marc-André, Feuerhelm, Julie, Grzechnik, Slawomir K., and Hale, Joanna

Published

2006

242. Structure of bacterial luciferase beta2 homodimer: Implications for flavin binding.

Author

Tanner, John J. and Miller, Mitchell D.

Subjects

*VIBRIO, *FLAVINS, *REACTIVITY (Chemistry)

Abstract

Discusses the impact of the structure of the beta2 homodimer of Vibrio harveyi luciferase on flavin binding. Background on luciferases; Comparison of dimer interfaces of homodimer and heterodimer; Quality of the structure; Binding and dissociation rate constants.

Published

1997

243. Stereochemical...facial selectivity of the Diels-Alder reaction of benz[a] aceanthrylene and 1,4-...

Author

Plummer, Benjamin F., Faiz, Saadia, Wiederhold, Ted, Wooten, Marilyn, Agyin, Joseph K., Krause, Kurt L., Miller, Mitchell D., and Watson, William H.

Published

1997

244. Simulation of electrostatic and hydrodynamic properties of Serratia endonuclease.

Author

Antosiewicz, Jan, Miller, Mitchell D., Krause, Kurt L., and McCammon, J. Andrew

Published

1997

245. Crystal structure of a zinc‐containing glycerol dehydrogenase (TM0423) from Thermotoga maritimaat 1.5 Å resolution

Author

Brinen, Linda S., Canaves, Jaume M., Dai, Xiaoping, Deacon, Ashley M., Elsliger, Marc A., Eshaghi, Said, Floyd, Ross, Godzik, Adam, Grittini, Carina, Grzechnik, Slawomir K., Guda, Chittibabu, Jaroszewski, Lukasz, Karlak, Cathy, Klock, Heath E., Koesema, Eric, Kovarik, John S., Kreusch, Andreas, Kuhn, Peter, Lesley, Scott A., McMullan, Daniel, McPhillips, Timothy M., Miller, Mark A., Miller, Mitchell D., Morse, Andrew, Moy, Kin, Ouyang, Jie, Robb, Alyssa, Rodrigues, Kevin, Selby, Thomas L., Spraggon, Glen, Stevens, Raymond C., Bedem, Henry van den, Velasquez, Jeff, Vincent, Juli, Wang, Xianhong, West, Bill, Wolf, Guenter, Taylor, Susan S., Hodgson, Keith O., Wooley, John, and Wilson, Ian A.

Published

2003

246. An X-ray microsource based system for crystal screening and beamline development during synchrotron shutdown periods

Author

Miller, Mitchell D. and Deacon, Ashley M.

Subjects

*INVESTMENTS, *CRYSTALLOGRAPHY, *CRYSTALS, *SOLIDS

Abstract

Abstract: Crystallographic end-stations require a significant investment in state-of-the-art equipment, as well as a significant effort in software development. The equipment often sits idle during annual maintenance shutdowns. In order to utilize the existing hardware and software during these shutdowns, we installed a sealed-tube microsource X-ray generator in the beamline 9-2 hutch at Stanford Synchrotron Radiation Laboratory (SSRL). A multi-layer optic provides good flux and spectral purity. The small physical size of the source, the long optic to focus distance (635mm) and the short source to optic distance (65mm) allowed the use of existing beamline components, without any significant modification. The system replaces a short section of beam pipe upstream of the beam conditioning slits and shutter. The system can be installed and removed from the beamline in less than 1 day. The Joint Center for Structural Genomics (JCSG) and SSRL Structural Molecular Biology group developed the Stanford Automated Mounting (SAM) system and installed it on beamlines at SSRL. The JCSG relies on this system to test crystals for diffraction. The installation of the X-ray microsource in beamline 9-2 allowed crystal screening to continue during SSRL shutdowns. Using a standard screening protocol of two 10min exposures, separated by a 90° phi rotation, the system was capable of screening up to 400 crystals per week and was left to run unattended for up to 4 days. Over 8200 crystals were screened during the last four SSRL shutdown periods. An X-ray generator can also be useful for ongoing beamline development. Shutdown periods provide easier access to the experimental hardware; however, some tests require beam. The X-ray microsource offers the ability to conduct these tests during periods when users are not scheduled. [Copyright &y& Elsevier]

Published

2007

247. Simulation of electrostatic and hydrodynamic properties of <TOGGLE>Serratia</TOGGLE> endonuclease

Author

Antosiewicz, Jan, Miller, Mitchell D., Krause, Kurt L., and McCammon, J. Andrew

Abstract

We analyze the electrostatic and hydrodynamic properties of a nuclease from the pathogenic gram-negative bacterium Serratia marcescens using finite-difference Poisson-Boltzmann methods for electrostatic calculations and a bead-model approach for diffusion coefficient calculations. Electrostatic properties are analyzed for the enzyme in monomeric and dimeric forms and also in the context of DNA binding by the nuclease. Our preliminary results show that binding of a double-stranded DNA dodecamer by nuclease causes an overall shift in the charge of the protein by approximately three units of elementary charge per monomer, resulting in a positively charged protein at physiologic pH. In these calculations, the free enzyme was found to have a negative (−1 e) charge per monomer at pH 7. The most dramatic shift in pKa involves His 89 whose pKa increases by three pH units upon DNA binding. This shift leads to a protonated residue at pH 7, in contrast to the unprotonated form in the free enzyme. DNA binding also leads to a decrease in the energetic distances between the most stable protonation states of the enzyme. Dimerization has no significant effect on the electrostatic properties of each of the monomers for both free enzyme and that bound to DNA. Results of hydrodynamic calculations are consistent with the dimeric form of the enzyme in solution. The computed translational diffusion coefficient for the dimer model of the enzyme is in very good agreement with measurements from light scattering experiments. Preliminary electrooptical calculations indicate that the dimer should possess a large dipole moment (approximately 600 Debye units) as well as substantial optical anisotropy (limiting reduced linear electric dichroism of about 0.3). Therefore, this system may serve as a good model for investigation of electric and hydrodynamic properties by relaxation electrooptical experiments. © 1997 John Wiley & Sons, Inc.

Published

1997

248. Crystal structure of the photosensory module from a PAS-less cyanobacterial phytochrome as Pr shows a mix of dark-adapted and photoactivated features.

Author

Burgie, E. Sethe, Mickles, Alayna J., Fang Luo, Miller, Mitchell D., and Vierstra, Richard D.

Abstract

Phytochromes (Phys) are a diverse collection of photoreceptors that regulate numerous physiological and developmental processes in microorganisms and plants through photointerconversion between red-light-absorbing Pr and farred light-absorbing Pfr states. Light is detected by an N-terminal photo-sensing module (PSM) sequentially comprised of Period/ARNT/Sim (PAS), cGMP-phosphodiesterase/adenylyl cyclase/FhlA (GAF), and Phy-specific (PHY) domains, with the bilin chromophore covalently-bound within the GAF domain. Phys sense light via the Pr/Pfr ratio measured by the light-induced rotation of the bilin D-pyrrole ring that triggers conformational changes within the PSM, which for microbial Phys reaches into an output region. A key step is a β-stranded to a-helical reconfiguration of a hairpin loop extending from the PHY domain to contact the GAF domain. Besides canonical Phys, cyanobacteria express several variants, including a PASless subfamily that harbors just the GAF and PHY domains for light detection. Prior 2D-NMR studies of a model PAS-less Phy from Synechococcus_sp._JA-2-3B'a(2-13) (Syβ-Cph1) proposed a unique photoconversion mechanism involving an A-pyrrole ring rotation while magic-angle-spinning NMR probing the chromophore proposed the prototypic D-ring flip. To help solve this conundrum, we determined the crystallographic structure of the GAF-PHY region from Syβ-Cph1 as Pr. Surprisingly, this structure differs from canonical Phys by having a Pr ZZZsyn, syn, anti bilin configuration but shifted to the activated position in the binding pocket with consequent folding of the hairpin loop to a-helical, an architecture common for Pfr. Collectively, the PSM of Syβ-Cph1 as Pr displayed a mix of dark-adapted and photoactivated features whose coplanar A-C pyrrole rings support a D-ring flip mechanism. [ABSTRACT FROM AUTHOR]

Published

2024

249. Structure and Function of a Dual Reductase–Dehydratase Enzyme System Involved in p-Terphenyl Biosynthesis

Author

Clinger, Jonathan A., Zhang, Yinan, Liu, Yang, Miller, Mitchell D., Hall, Ronnie E., Van Lanen, Steven G., Phillips Jr., George N., Thorson, Jon S., and Elshahawi, Sherif I.

Abstract

We report the identification of the tergene cluster responsible for the formation of the p-terphenyl derivatives terfestatins B and C and echoside B from the Appalachian Streptomycesstrain RM-5-8. We characterize the function of TerB/C, catalysts that work together as a dual enzyme system in the biosynthesis of natural terphenyls. TerB acts as a reductase and TerC as a dehydratase to enable the conversion of polyporic acid to a terphenyl triol intermediate. X-ray crystallography of the apo and substrate-bound forms for both enzymes provides additional mechanistic insights. Validation of the TerC structural model via mutagenesis highlights a critical role of arginine 143 and aspartate 173 in catalysis. Cumulatively, this work highlights a set of enzymes acting in harmony to control and direct reactive intermediates and advances fundamental understanding of the previously unresolved early steps in terphenyl biosynthesis.

Published

2021

250. Observation of substrate diffusion and ligand binding in enzyme crystals using high-repetition-rate mix-and-inject serial crystallography

Author

Pandey, Suraj, Calvey, George, Katz, Andrea M., Malla, Tek Narsingh, Koua, Faisal H. M., Martin-Garcia, Jose M., Poudyal, Ishwor, Yang, Jay-How, Vakili, Mohammad, Yefanov, Oleksandr, Zielinski, Kara A., Bajt, Sasa, Awel, Salah, Doerner, Katarina, Frank, Matthias, Gelisio, Luca, Jernigan, Rebecca, Kirkwood, Henry, Kloos, Marco, Koliyadu, Jayanath, Mariani, Valerio, Miller, Mitchell D., Mills, Grant, Nelson, Garrett, Olmos, Jose L., Sadri, Alireza, Sato, Tokushi, Tolstikova, Alexandra, Xu, Weijun, Ourmazd, Abbas, Spence, John C. H., Schwander, Peter, Barty, Anton, Chapman, Henry N., Fromme, Petra, Mancuso, Adrian P., Phillips, George N., Bean, Richard, Pollack, Lois, and Schmidt, Marius

Subjects

3. Good health

Abstract

IUCrJ 8(6), 878 - 895 (2021). doi:10.1107/S2052252521008125, Here, we illustrate what happens inside the catalytic cleft of an enzyme when substrate or ligand binds on single-millisecond timescales. The initial phase of the enzymatic cycle is observed with near-atomic resolution using the most advanced X-ray source currently available: the European XFEL (EuXFEL). The high repetition rate of the EuXFEL combined with our mix-and-inject technology enables the initial phase of ceftriaxone binding to the Mycobacterium tuberculosis ��-lactamase to be followed using time-resolved crystallography in real time. It is shown how a diffusion coefficient in enzyme crystals can be derived directly from the X-ray data, enabling the determination of ligand and enzyme���ligand concentrations at any position in the crystal volume as a function of time. In addition, the structure of the irreversible inhibitor sulbactam bound to the enzyme at a 66 ms time delay after mixing is described. This demonstrates that the EuXFEL can be used as an important tool for biomedically relevant research., Published by Chester