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Pilus biogenesis and epithelial cell adherence of Neisseria gonorrhoeae pilC double knock-out mutants (1995)

Rudel, Thomas ; Boxberger, Hans-Jürgen ; Meyer, Thomas F.

Osney Mead, Oxford OX2 0EL, UK : Blackwell Scientific Publications

Molecular microbiology 17 (1995), S. 0

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ISSN: 1365-2958

Source: Blackwell Publishing Journal Backfiles 1879-2005

Topics: Biology , Medicine

Notes: The phase-variable PilC proteins of pathogenic Neisseria species have recently been implicated in both assembly and cellular adherence functions of the type 4 pili of these pathogens. We describe here the cloning of full-length pilC1 and pilC2 genes and the complete sequencing of the pilC2 gene of Neisseria gonorrhoeae MS11. Sequential inactivation of both genes by gene replacement in piliated (P+) variants of N. gonorrhoeae MS11 led initially to a non-piliated (P−) phenotype; however, spontaneous P+ variants could be derived from some pilC1,2 double mutants which produced morphologically intact pili. Purified pili from pilC1,2 mutants revealed no detectable PilC protein. Instead, a novel protein about 70 kDa in size appeared in the pili preparations of P+ mutants; this protein exhibited no immunological cross-reactivity with PilC1 or PilC2. We propose that this novel factor replaces the function of PilC in pilus biogenesis. Using isogenic N. gonorrhoeae strains which produce identical PilE (pilin) proteins we demonstrate that pili associated with the 70 kDa protein do not confer gonococcal adherence to human epithelial cells, in contrast to pili assembled in the presence of PilC1 or PilC2.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1111/j.1365-2958.1995.mmi_17061057.x

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Uptake and nuclear transport of Neisseria IgA1 protease-associated α-proteins in human cells (1995)

Pohlner, Johannes ; Langenberg, Uwe ; Wölk, Uwe ; [et al.]

Osney Mead, Oxford OX2 0EL, UK : Blackwell Scientific Publications

Molecular microbiology 17 (1995), S. 0

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ISSN: 1365-2958

Source: Blackwell Publishing Journal Backfiles 1879-2005

Topics: Biology , Medicine

Notes: Pathogenic Neisseria species, the causative agents of gonorrhoea and bacterial meningitis, encode a family of polymorphic exo-proteins which are autoproteolytically processed into several distinct extracellular components, including an IgA1 protease and an α-protein. IgA1 protease, a putative virulence determinant, is a sequence-specific endopeptidase known to cleave human IgA1, but additional target proteins have been postulated. The physical linkage of IgA1 protease and a-protein suggests a functional relationship of both precursor components. Previous work has shown that α-protein is essential neither for extracellular transport nor for the proteolytic activity of IgA1 protease. Intriguingly, α-proteins carry amino acid sequences reminiscent of nuclear location signals of viral and eukaryotic proteins. Here we demonstrate the functionality of these nuclear location signal sequences in transfected eukaryotic cells. Chimeric α-proteins show nuclear transport and selectively associate with nucleolar structures. More importantly, native purified α-proteins are capable of entering certain human primary cells from the exterior via an endocytotic route and accumulate in the nuclei. The neisserial α-proteins share several features with eukaryotic transcription factors, such as the formation of dimers via a heptad repeat sequence. We propose a role for a-proteins in the regulation of host-cell functions. As the α-proteins are covalently connected with IgA1 protease they may also serve as carriers for the IgA1 protease into human cells where additional proteolytic targets may exist. Neisseria meningitidis, which locally colonizes the nasopharyngeal mucosa of many human individuals without apparently causing symptoms, secretes this nucleus-targeted factor in large quantities.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1111/j.1365-2958.1995.mmi_17061073.x

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3

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A rapid luciferase transfection assay for transcription activation effects and stability control of estrogenic drugs in cell cultures (1994)

Meyer, Thomas ; Koop, Ronald ; Angerer, Erwin ; [et al.]

Springer

Journal of cancer research and clinical oncology 120 (1994), S. 359-364

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ISSN: 1432-1335

Keywords: Estrogen receptor ; Estrogenic plantinum(II) complex ; Luciferase ; Transfection ; Drug stability

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract A rapid assay system for measuring the potential of estrogenic drugs is introduced. Luciferase induction could be measured in estrogen-receptor-positive human MCF-7 breast cancer cells, which had been transfected with a novel luciferase reporter plasmid ERE luc. The minimal requirement was 1 h exposure to the inducing drug and 3.5 h of incubation after removal of the drug. The assay system was used to measure the stability of the drug diaqua-[1,2-bis (2,6-dichloro-4-hydroxyphenyl) ethylenediamine] platinum(II) sulfate, containing an estrogenic ligand and reactive platinum. Luciferase activity was observed only when the drug was in the culture medium and cells for short times, whereas the estrogenic ligand alone remained active. It is assumed that binding of the platinum moiety to macromolecular constituents of the culture or cells renders the drug inaccessible for binding to the estrogen receptor.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01247461

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4

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Structure-based design of potent CDK1 inhibitors derived from olomoucine (2000)

Furet, Pascal ; Zimmermann, Juerg ; Capraro, Hans-Georg ; [et al.]

Springer

Journal of computer aided molecular design 14 (2000), S. 403-409

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ISSN: 1573-4951

Keywords: cyclin-dependent kinase ; CDK1 ; inhibitor ; olomoucine ; structure-based design

Source: Springer Online Journal Archives 1860-2000

Topics: Chemistry and Pharmacology

Notes: Abstract Cyclin-dependent kinase 1 (CDK1), an enzyme participating in the regulation of the cell cycle, constitutes a possible target in the search for new antitumor agents. Starting from the purine derivative olomoucine and following a structure-based approach, potent inhibitors of this enzyme were rapidly identified. The molecular modeling aspects of this work are described.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1023/A:1008115004986

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5

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Cloning and characterization of the Neisseria gonorrhoeae MS11 folC gene (1996)

Fussenegger, Martin ; Meyer, Thomas F.

Springer

Molecular genetics and genomics 250 (1996), S. 277-285

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ISSN: 1617-4623

Keywords: Key words Gonococcus ; Folic acid ; Dihydrofolate synthetase ; Folylpolyglutamate synthetase ; One-carbon metabolism

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Abstract The gene coding for folylpoly-(γ)-glutamate synthetase (FPGS)-dihydrofolate synthetase (DHFS) of Neisseria gonorrhoeae (Ngo) has been cloned by functional complementation of an Escherichia coli folC mutant (SF4). The sequence encodes a 224-residue protein of 46.4 kDa. It shows 46% identity to the E. coli FPGS-DHFS and 29% identity to the FPGS of Lactobacillus casei. Sequence comparisons between the three genes reveal regions of high homology, including ATP binding sites required for bifunctionality, all of which may be important for FPGS activity. In contrast to L. casei FPGS, the E. coli and Ngo enzymes share some additional regions which may be essential for DHFS activity. The products of Ngo folC and flanking genes were monitored by T7 promoter expression. Interestingly, deletion of the upstream folI gene, which encodes a 16.5 kDa protein, abolishes the capacity of folC to complement E. coli SF4 to the wild-type phenotype. The ability to complement can be restored by folI provided in trans. Unlike folC mutants, gonococcal folI mutants are viable and display no apparent phenotype. Thus, in contrast to E. coli, Ngo folC is expressed at a sufficiently high level from its own promoter, in the absence of FolI. This study provides the first insights into the genetic complexity of one-carbon metabolism in Ngo.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02174385

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6

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Construction of hermes shuttle vectors: a versatile system useful for genetic complementation of transformable and non-transformableNeisseria mutants (1996)

Kupsch, Eva-Marià ; Aubel, Dominique ; Gibbs, Carol P. ; [et al.]

Springer

Molecular genetics and genomics 250 (1996), S. 558-569

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ISSN: 1617-4623

Keywords: Plasmid vector ; Conjugation ; Generalized mutagenesis ; Homologous recombination ; Natural transformation competence

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Abstract A versatile shuttle system has been developed for genetic complementation with cloned genes of transformable and non-transformableNeisseria mutants. By random insertion of a selectable marker into the conjugativeNeisseria plasmidptetM25.2, a site within this plasmid was identified that is compatible with plasmid replication and with conjugative transfer of plasmid. Regions flanking the permissive insertion site of ptetM25.2 were cloned inEscherichia coli and served as a basis for the construction of the Hermes vectors. Hermes vectors are composed of anE. coli replicon that does not support autonomous replication inNeisseria, e.g. ColE1, p15A, orori fd, fused with a shuttle consisting of a selectable marker and a multiple cloning site flanked by the integration region of ptetM25.2. Complementation of a non-transformableNeisseria strain involves a three-step process: (i) insertion of the desired gene into a Hermes vector; (ii) transformation of Hermes into aNeisseria strain containing ptetM25.2 to create a hybrid ptetM25.2 via gene replacement by the Hermes shuttle cassette; and (iii) conjugative transfer of the hybrid ptetM25.2 into the finalNeisseria recipient. Several applications for the genetic manipulation of pathogenicNeisseriae are described.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02174444

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7

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Nucleotide sequence of ompV, the gene for a major Vibrio cholerae outer membrane protein (1986)

Pohlner, Johannes ; Meyer, Thomas F. ; Jalajakumari, M. B. ; [et al.]

Springer

Molecular genetics and genomics 205 (1986), S. 494-500

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ISSN: 1617-4623

Keywords: Signal sequence ; Gene regulation ; Export ; Codon usage

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Summary The nucleotide sequence of the ompV gene of Vibrio cholerae was determined. The product of the gene is a 28,000 dalton protein which, after the removal of a 19 amino acid signal sequence, produces a mature outer membrane protein of 26,000 daltons. The cleavage site was determined by amino-terminal amino acid sequencing of the purified mature protein. The DNA upstream of the gene shows the presence of a typical promoter region as judged from the Escherichia coli consensus information; however, the Shine-Dalgarno sequence is associated with a region capable of forming a secondary structure in the mRNA. The formation of this structure would inhibit binding of the mRNA to the ribosome and reduce translation. It is proposed that this structure is recognized by a positive activator in V. cholerae and because of its absence in E. coli ompV is poorly expressed. The distribution of rare codons within ompV suggests that they may serve to slow down the translation of particular domains such that the nascent polypeptide has an opportunity to take up its conformation without interference from the later formed regions. Such a mechanism could aid localization of the protein if export were by a cotranslational secretion system.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00338088

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8

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Recognition of two initiation codons for the synthesis of phage fd gene 2 protein (1980)

Meyer, Thomas F. ; Beyreuther, Konrad ; Geider, Klaus

Springer

Molecular genetics and genomics 180 (1980), S. 489-494

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ISSN: 1617-4623

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Summary Bacteriophage fd gene 2 protein was specifically labeled with radioactive amino acids and was isolated from membranous cell structures as an apparently homogenous protein. Amino acid sequence analysis revealed that the protein was initiated at two distinct AUG codons close to the ribosome binding site. The two resulting translation products were found to begin with a deformylated methionine residue. Initiation at the first signal was used for 90% of the chains and at the second signal for 10% of the sequenced molecules. The use of one or the other chain start may influence functions of gene 2 protein.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00268051

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9

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Serological properties and processing in Escherichia coli K12 of OmpV fusion proteins of Vibrio cholerae (1986)

Pohlner, Johannes ; Meyer, Thomas F. ; Manning, Paul A.

Springer

Molecular genetics and genomics 205 (1986), S. 501-506

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ISSN: 1617-4623

Keywords: Signal sequence ; Antigenic epitopes ; Outer membrane protein ; Immunogenicity

Source: Springer Online Journal Archives 1860-2000

Topics: Biology

Notes: Summary Fusion proteins comprising the amino-terminal 99 amino acids of the bacteriophage MS2 replicase and various portions of OmpV a major outer membrane protein of Vibrio cholerae were expressed in Escherichia coli K12. These fusions were expressed under the control of the PL promoter of bacteriophage λ, and expression was controlled using a cIts repressor. Fusions occurring within the secretory signal sequence of OmpV gave rise to the production of mature OmpV. The efficiency, however, decreased with progressive deletion of the signal sequence within the fusions. The reactivity of various OmpV fusions with antisera raised against purified OmpV and whole bacteria demonstrated the existence of two antigenic domains: one present in the denatured form and another in the membrane-associated form of OmpV. These domains correspond to markedly hydrophilic regions of the protein as would be predicted for surface-exposed epitopes.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00338089

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10

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Tyrosine Phosphorylation of Moesin in Arachidonic Acid–Stimulated Human Platelets (1998)

Meyer, Thomas ; Uher, Thomas ; Schwartz, Peter ; [et al.]

Springer

Journal of thrombosis and thrombolysis 6 (1998), S. 117-124

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ISSN: 1573-742X

Keywords: moesin ; ezrin ; tyrosine phosphorylation ; arachidonic acid ; platelets

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract Moesin, a member of the ezrin/radixin/moesin (ERM) family of cytoskeletal proteins, has been implicated in dynamic membrane-based processes such as the formation and stabilization of filopodia. Ezrin is known to be a substrate of tyrosine kinases in activated T cells and epithelial growth factor–stimulated A431 cells. For the closely related 77-kD protein moesin, which shares 72% identity with ezrin on the basis of their amino acid sequences, a reversible phosphorylation on tyrosine residues has not yet been described. Because our scanning electron microscopy studies revealed the appearance of multiple, up to 3 μm long filopodia on the surface of activated human platelets, we investigated the participation of moesin in dynamic shape changes on platelet stimulation with arachidonic acid. Antimoesin immunoprecipitates obtained under denaturing conditions from lysates of resting platelets contained only low amounts of tyrosine-phosphorylated moesin. In lysates of arachidonic acid–stimulated platelets, the level of tyrosine phosphorylation was significantly increased. This activation-dependent phosphorylation of moesin was verified by probing antiphosphotyrosine immunoprecipitates from unstimulated and stimulated platelets with antimoesin antibodies. Tyrosine-phosphorylated moesin was detectable only in the presence of the tyrosine phosphatase inhibitor vanadate, suggesting that a coordinated balance between kinase and phosphatase activities controls the steady-state level of moesin phosphorylation.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1023/A:1008845421381

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