Your search keyword '"Tracy Palmer"' showing total 5 results

1. Organophosphate Hydrolase Is a Lipoprotein and Interacts with Pi-specific Transport System to Facilitate Growth of Brevundimonas diminuta Using OP Insecticide as Source of Phosphate

Author

Dayananda Siddavattam, Aparna Nandavaram, Hari Parapatla, Tracy Palmer, and Sunil Parthasarathy

Subjects

0301 basic medicine, Signal peptide, Insecticides, Signal peptidase, Arginine transport, Stereochemistry, Lipoproteins, Cell Membrane, Caulobacteraceae, Cell Biology, Periplasmic space, Biology, Signal peptidase II, Microbiology, Biochemistry, Phosphoric Monoester Hydrolases, Serine, 03 medical and health sciences, 030104 developmental biology, Bacterial Proteins, Phosphate Transport Proteins, Brevundimonas diminuta, Bacterial outer membrane, Molecular Biology

Abstract

Organophosphate hydrolase (OPH), encoded by the organophosphate degradation (opd) island, hydrolyzes the triester bond found in a variety of organophosphate insecticides and nerve agents. OPH is targeted to the inner membrane of Brevundimonas diminuta in a pre-folded conformation by the twin arginine transport (Tat) pathway. The OPH signal peptide contains an invariant cysteine residue at the junction of the signal peptidase (Spase) cleavage site along with a well conserved lipobox motif. Treatment of cells producing native OPH with the signal peptidase II inhibitor globomycin resulted in accumulation of most of the pre-OPH in the cytoplasm with negligible processed OPH detected in the membrane. Substitution of the conserved lipobox cysteine to serine resulted in release of OPH into the periplasm, confirming that OPH is a lipoprotein. Analysis of purified OPH revealed that it was modified with the fatty acids palmitate and stearate. Membrane-bound OPH was shown to interact with the outer membrane efflux protein TolC and with PstS, the periplasmic component of the ABC transporter complex (PstSACB) involved in phosphate transport. Interaction of OPH with PstS appears to facilitate transport of Pi generated from organophosphates due to the combined action of OPH and periplasmically located phosphatases. Consistent with this model, opd null mutants of B. diminuta failed to grow using the organophosphate insecticide methyl parathion as sole source of phosphate.

Published

2016

2. Cysteine Scanning Mutagenesis and Disulfide Mapping Studies of the TatA Component of the Bacterial Twin Arginine Translocase

Author

Grant Buchanan, Matthew G. Hicks, Ben C. Berks, Tracy Palmer, Ida Porcelli, Nicholas P. Greene, and Sonya M. Schermann

Subjects

biology, Escherichia coli Proteins, Membrane Transport Proteins, Biological Transport, Cell Biology, Biochemistry, Transmembrane protein, Twin-arginine translocation pathway, Transmembrane domain, Protein structure, Mutagenesis, Helix, biology.protein, Translocase, Cysteine, Disulfides, Protein Structure, Quaternary, Molecular Biology, Integral membrane protein

Abstract

The Tat (twin arginine translocation) system transports folded proteins across the bacterial cytoplasmic membrane and the thylakoid membrane of plant chloroplasts. The integral membrane proteins TatA, TatB, and TatC are essential components of the Tat pathway. TatA forms high order oligomers and is thought to constitute the protein-translocating unit of the Tat system. Cysteine scanning mutagenesis was used to systematically investigate the functional importance of residues in the essential N-terminal transmembrane and amphipathic helices of Escherichia coli TatA. Cysteine substitutions of most residues in the amphipathic helix, including all the residues on the hydrophobic face of the helix, severely compromise Tat function. Glutamine 8 was identified as the only residue in the transmembrane helix that is critical for TatA function. The cysteine variants in the transmembrane helix were used in disulfide mapping experiments to probe the oligomeric arrangement of TatA protomers within the larger TatA complex. Residues in the center of the transmembrane helix (including residues 10-16) show a distinct pattern of cross-linking indicating that this region of the protein forms well defined interactions with other protomers. At least two interacting faces were detected. The results of our TatA studies are compared with analogous data for the homologous, but functionally distinct, TatB protein. This comparison reveals that it is only in TatA that the amphipathic helix is sensitive to amino acid substitutions. The TatA amphipathic helix may play a role in forming and controlling the path of substrate movement across the membrane.

Published

2007

3. TatD Is a Cytoplasmic Protein with DNase Activity

Author

Margaret Wexler, Rachael L. Jack, Ben C. Berks, Erik G. Bogsch, Nicola R. Stanley, Frank Sargent, Tracy Palmer, and Colin Robinson

Subjects

chemistry.chemical_classification, Signal peptide, Operon, Cell Biology, Biology, medicine.disease_cause, Biochemistry, Twin-arginine translocation pathway, Gene product, Enzyme, chemistry, medicine, Overproduction, Molecular Biology, Gene, Escherichia coli

Abstract

The Escherichia coli Tat system mediates Sec-independent export of protein precursors bearing twin arginine signal peptides. Genes known to be involved in this process include tatA, tatB, and tatC that form an operon with a fourth gene, tatD. ThetatD gene product has two homologues in E. colicoded by the unlinked ycfH and yjjV genes. AnE. coli strain with in-frame chromosomal deletions in all three of tatD, ycfH, and yjjVexhibits no significant defect in the cellular location of five cofactor-containing enzymes that are synthesized with twin arginine signal peptides. Neither these mutations nor overproduction of the TatD protein cause any discernible effect on the export kinetics of an additional E. coli Tat pathway substrate. It is concluded that proteins of the TatD family have no obligate involvement in protein export by the Tat system. TatD is shown to be a cytoplasmic protein. TatD binds to immobilized Ni2+ or Zn2+affinity columns and exhibits magnesium-dependent DNase activity. Features of the tatA operon that may control TatD expression are discussed.

Published

2000

4. The Twin Arginine Consensus Motif of Tat Signal Peptides Is Involved in Sec-independent Protein Targeting in Escherichia coli

Author

Nicola R. Stanley, Tracy Palmer, and Ben C. Berks

Subjects

Signal peptide, Arginine, medicine.disease_cause, Biochemistry, Twin-arginine translocation pathway, Bacterial Proteins, Consensus Sequence, Protein targeting, Escherichia coli, Serine, medicine, Consensus sequence, Molecular Biology, chemistry.chemical_classification, biology, Membrane transport protein, Escherichia coli Proteins, Lysine, Membrane Transport Proteins, Cell Biology, Amino acid, Amino Acid Substitution, chemistry, Mutagenesis, Site-Directed, biology.protein, Leucine, Carrier Proteins

Abstract

In Escherichia coli a subset of periplasmic proteins is exported through the Tat pathway to which substrates are directed by an NH(2)-terminal signal peptide containing a consensus SRRXFLK "twin arginine" motif. The importance of the individual amino acids of the consensus motif for in vivo Tat transport has been assessed by site-directed mutagenesis of the signal peptide of the Tat substrate pre-SufI. Although the invariant arginine residues are crucial for efficient export, we find that slow transport of SufI is still possible if a single arginine is conservatively substituted by a lysine residue. Thus, in at least one signal peptide context there is no absolute dependence of Tat transport on the arginine pair. The consensus phenylalanine residue was found to be a critical determinant for efficient export but could be functionally substituted by leucine, another amino acid with a highly hydrophobic side chain. Unexpectedly, the consensus lysine residue was found to retard Tat transport. These observations and others suggest that the sequence conservation of the Tat consensus motif is a reflection of the functional importance of the consensus residues. Tat signal peptides characteristically have positively charged carboxyl-terminal regions. However, changing the sign of this charge does not affect export of SufI.

Published

2000

5. Sec-independent Protein Translocation in Escherichia coli

Author

Ben C. Berks, Tracy Palmer, Frank Sargent, and Nicola R. Stanley

Subjects

Mutant, Cell Biology, Biology, medicine.disease_cause, Biochemistry, Transmembrane protein, Twin-arginine translocation pathway, Complementation, chemistry.chemical_compound, chemistry, TATB, medicine, Molecular Biology, Integral membrane protein, Gene, Escherichia coli

Abstract

In Escherichia coli, transmembrane translocation of proteins can proceed by a number of routes. A subset of periplasmic proteins are exported via the Tat pathway to which proteins are directed by N-terminal “transfer peptides” bearing the consensus (S/T)RRXFLK “twin-arginine” motif. The Tat system involves the integral membrane proteins TatA, TatB, TatC, and TatE. Of these, TatA, TatB, and TatE are homologues of the Hcf106 component of the ΔpH-dependent protein import system of plant thylakoids. Deletion of the tatB gene alone is sufficient to block the export of seven endogenous Tat substrates, including hydrogenase-2. Complementation analysis indicates that while TatA and TatE are functionally interchangeable, the TatB protein is functionally distinct. This conclusion is supported by the observation that Helicobacter pylori tatA will complement an E. coli tatA mutant, but not a tatB mutant. Analysis of Tat component stability in various tat deletion backgrounds shows that TatC is rapidly degraded in the absence of TatB suggesting that TatC complexes, and is stabilized by, TatB.

Published

1999