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1

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V. Functions of S-layers

Beveridge, Terrance J. ; Pouwels, Peter H. ; Sára, Margit ; [et al.]

Oxford University Press (OUP) ; 1997

In: FEMS Microbiology Reviews Vol. 20, No. 1-2 ( 1997-06), p. 99-149

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In: FEMS Microbiology Reviews, Oxford University Press (OUP), Vol. 20, No. 1-2 ( 1997-06), p. 99-149

Type of Medium: Online Resource

ISSN: 1574-6976

URL: Article

DOI: 10.1111/j.1574-6976.1997.tb00305.x

Language: English

Publisher: Oxford University Press (OUP)

Publication Date: 1997

detail.hit.zdb_id: 1500468-5

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2

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Evaluation of a New System for Developing Particulate Enzymes Based on the Surface (S)-Layer Protein (RsaA) of 〈I〉Caulobacter crescentus〈/I〉: Fusion With the b〈I〉-1,4-Glycanase (Cex) From the Cellulolytic Bacterium 〈/I〉Cellulomonas fimi〈I〉 Yields a Robust, Catalytically Active Product

Duncan, Gillian ; Tarling, Chris A. ; Bingle, Wade H. ; [et al.]

Springer Science and Business Media LLC ; 2005

In: Applied Biochemistry and Biotechnology Vol. 127, No. 2 ( 2005), p. 095-110

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In: Applied Biochemistry and Biotechnology, Springer Science and Business Media LLC, Vol. 127, No. 2 ( 2005), p. 095-110

Type of Medium: Online Resource

ISSN: 0273-2289

URL: Issue

URL: Article

DOI: 10.1385/ABAB:127:2

DOI: 10.1385/ABAB:127:2:095

Language: English

Publisher: Springer Science and Business Media LLC

Publication Date: 2005

detail.hit.zdb_id: 2072711-2

SSG: 12

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3

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Expression and testing of Pseudomonas aeruginosa vaccine candidate proteins prepared with the Caulobacter crescentus S-layer protein expression system

Umelo-Njaka, Elizabeth ; Nomellini, John F. ; Bingle, Wade H. ; [et al.]

Elsevier BV ; 2001

In: Vaccine Vol. 19, No. 11-12 ( 2001-12), p. 1406-1415

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In: Vaccine, Elsevier BV, Vol. 19, No. 11-12 ( 2001-12), p. 1406-1415

Type of Medium: Online Resource

ISSN: 0264-410X

URL: Article

DOI: 10.1016/S0264-410X(00)00362-5

Language: English

Publisher: Elsevier BV

Publication Date: 2001

detail.hit.zdb_id: 1468474-3

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4

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Characterization of the surface layer protein from Azotobacter vinelandii

Bingle, Wade H. ; Doran, James L. ; Page, William J.

Canadian Science Publishing ; 1986

In: Canadian Journal of Microbiology Vol. 32, No. 2 ( 1986-02-01), p. 112-120

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In: Canadian Journal of Microbiology, Canadian Science Publishing, Vol. 32, No. 2 ( 1986-02-01), p. 112-120

Abstract: The regular surface array protein (S protein) of Azotobacter vinelandii was extracted from outer membrane fragments with distilled water and further purified by gel filtration chromatography. The protein was shown to behave anomalously on sodium dodecyl sulfate polyacrylamide gels producing a number of conformational isomers. The amino acid composition of S protein was similar to that of other surface array proteins, particularly in its lack of cysteine. The theoretical monomelic molecular weight of S protein was calculated to be 60 218 based on the total amino acid composition and the apparent molecular weight determined by sodium dodecyl sulfate – polyacrylamide gel electrophoresis. Circular dichroism spectra indicated that S protein was composed of approximately 35% β sheet structure, negligible α helix, with the remainder of the polypeptide backbone aperiodic in nature. The effect of the divalent cations Ca 2+ and Mg 2+ on the conformation of S protein was examined by circular dichroism spectroscopy; however, no conformational change was detected in response to the presence of these species nor did S-protein monomer aggregate into multimers in the presence of these cations. Purified S-protein monomer was inactive in divalent cation mediated reassembly of the S layer onto the surface of distilled water washed cells. A larger multimeric form present only in fresh preparations appeared to be the active species involved in in vitro reassembly of the A. vinelandii surface array.

Type of Medium: Online Resource

ISSN: 0008-4166 , 1480-3275

URL: Article

DOI: 10.1139/m86-023

RVK:

WA 15000

Language: English

Publisher: Canadian Science Publishing

Publication Date: 1986

detail.hit.zdb_id: 280534-0

detail.hit.zdb_id: 1481972-7

SSG: 12

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5

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A method for separating fungal hyphae from soil

Bingle, Wade H. ; Paul, Eldor A.

Canadian Science Publishing ; 1986

In: Canadian Journal of Microbiology Vol. 32, No. 1 ( 1986-01-01), p. 62-66

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In: Canadian Journal of Microbiology, Canadian Science Publishing, Vol. 32, No. 1 ( 1986-01-01), p. 62-66

Abstract: When fungal hyphae were separated from two mineral soils by wet sieving and density gradient centrifugation, a preparation consisting of 50% of the total soil fungal hyphae and 3% of the soil dry weight was obtained. Residual soil particles were removed by an additional sieving step which resulted in a final recovery of 20% of the fungal hyphae from soil. Scanning electron microscopy revealed that some soil particles still contaminated the hyphae but the exact amount of soil could not be determined by dry weight measurements. These data indicated that reasonable separation of fungal hyphae from soil for use in biomass (i.e., nutrient analysis) studies is feasible.

Type of Medium: Online Resource

ISSN: 0008-4166 , 1480-3275

URL: Article

DOI: 10.1139/m86-012

RVK:

WA 15000

Language: English

Publisher: Canadian Science Publishing

Publication Date: 1986

detail.hit.zdb_id: 280534-0

detail.hit.zdb_id: 1481972-7

SSG: 12

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6

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An ''all-purpose" cellulase reporter for gene fusion studies and application to the paracrystalline surface (S)-layer protein of Caulobacter crescentus

Bingle, Wade H. ; Kurtz Jr., Harry D. ; Smit, John

Canadian Science Publishing ; 1993

In: Canadian Journal of Microbiology Vol. 39, No. 1 ( 1993-01-01), p. 70-80

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In: Canadian Journal of Microbiology, Canadian Science Publishing, Vol. 39, No. 1 ( 1993-01-01), p. 70-80

Abstract: The secreted endoglucanase (CenA) from the Gram-positive bacterium Cellulomonas fimi and a deletion derivative (ΔCenA) lacking the N-terminal leader peptide of native CenA were used to explore the potential of ΔCenA as a reporter molecule in Caulobacter crescentus. Expression of cenA in C. crescentus yielded extracellular endoglucanase activity, suggesting that the N-terminal leader peptide of CenA could direct the enzyme to the periplasm where it subsequently leaked into the medium. In contrast, expression of ΔcenA yielded only cell-associated endoglucanase activity; this suggested that the enzyme retained activity in the C. crescentus cytoplasm. Using the putative cytoplasmic and periplasmic forms of ΔCenA as markers, a simple assay for periplasmic ΔCenA hybrids was developed. This assay indicated that ΔCenA activity was largely independent of cellular location. To facilitate the use of ΔCenA as a reporter, a broad host range translational fusion vector (pEC215) incorporating ΔcenA was constructed. This vector was used to investigate factors important to the expression of the gene (rsaA) encoding the paracrystalline surface protein (S-layer) of the bacterium. It was found that altering the 5′ untranslated region of the rsaA mRNA reduced gene expression by 70%. One rsaA:ΔcenA gene fusion resulting from these experiments that incorporated only rsaA translation initiation information was further modified to serve as a general reporter for creating transcriptional gene fusions with other promoters. Gene fusions between alkaline phosphatase (phoA) and either cenA or lacZ were used to supplement information about RsaA secretion derived from rsaA:phoA gene fusions. It was found that linkage of the N-terminal leader peptide of CenA to PhoA yielded 50–100 times more cell-associated PhoA activity in C. crescentus than linkage of the RsaA N terminus. Taken together, these experiments indicated that ΔCenA was useful for tagging proteins localized to the cytoplasm, exported to the periplasm, or secreted from the cell, as well as for monitoring events in the cytoplasm such as examining factors important to the level of gene expression. Further, because ΔCenA was active in all cell compartments, it could be used to estimate the efficiency of hybrid protein export-secretion from enzyme activity measurements alone. In short, ΔCenA possessed many of the attributes of an "all-purpose" reporter.Key words: gene fusions, protein secretion, cellulase, alkaline phosphatase, Caulobacter crescentus.

Type of Medium: Online Resource

ISSN: 0008-4166 , 1480-3275

URL: Article

DOI: 10.1139/m93-010

RVK:

WA 15000

Language: English

Publisher: Canadian Science Publishing

Publication Date: 1993

detail.hit.zdb_id: 280534-0

detail.hit.zdb_id: 1481972-7

SSG: 12

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7

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Cell‐surface display of a Pseudomonas aeruginosa strain K pilin peptide within the paracrystalline S‐layer of Caulobacter crescentus

Bingle, Wade H. ; Nomellini, John F. ; Smit, John

Wiley ; 1997

In: Molecular Microbiology Vol. 26, No. 2 ( 1997-10), p. 277-288

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In: Molecular Microbiology, Wiley, Vol. 26, No. 2 ( 1997-10), p. 277-288

Abstract: The paracrystalline surface (S)‐layer of Caulobacter crescentus is composed of a single secreted protein (RsaA) that interlocks in a hexagonal pattern to completely envelop the bacterium. Using a genetic approach, we inserted a 12 amino acid peptide from Pseudomonas aeruginosa strain K pilin at numerous semirandom positions in RsaA. We then used an immunological screen to identify those sites that presented the inserted pilin peptide on the C . crescentus cell surface as a part of the S‐layer. Eleven such sites (widely separated in the primary sequence) were identified, demonstrating for the first time that S‐layers can be readily exploited as carrier proteins to display ‘epitope‐size’ heterologous peptides on bacterial cell surfaces. Whereas intact RsaA molecules carrying a pilin peptide could always be found on the surface of C . crescentus regardless of the particular insertion site, introduction of the pilin peptide at 9 of the 11 sites resulted in some proteolytic cleavage of RsaA. Two types of proteolytic phenomena were observed. The first was characterized by a single cleavage within the pilin peptide insert with both fragments of the S‐layer protein remaining anchored to the outer membrane. The other proteolytic phenomenon was characterized by cleavage of the S‐layer protein at a point distant from the site of the pilin peptide insertion. This cleavage always occurred at the same location in RsaA regardless of the particular insertion site, yielding a surface‐anchored 26 kDa proteolytic fragment bearing the RsaA N‐terminus; the C‐terminal cleavage product carrying the pilin peptide was released into the growth medium. When the results of this work were combined with the results of a previous study, the RsaA primary sequence could be divided into three regions with respect to the location of a peptide insertion and its effect on S‐layer biogenesis: (i) insertions in the extreme N‐terminus of RsaA either produce no apparent effect on S‐layer biogenesis or disrupt surface‐anchoring of the protein; (ii) insertions in the extreme C‐terminus either produce no apparent effect on S‐layer biogenesis or disrupt protein secretion; and (iii) insertions more centrally located in the protein either have no apparent effect on S‐layer biogenesis or result in proteolytic cleavage of RsaA. These data are discussed in relation to our previous assignment of the RsaA N‐ and C‐terminus as regions that are important for surface anchoring and secretion respectively.

Type of Medium: Online Resource

ISSN: 0950-382X , 1365-2958

URL: Article

DOI: 10.1046/j.1365-2958.1997.5711932.x

Language: English

Publisher: Wiley

Publication Date: 1997

detail.hit.zdb_id: 1501537-3

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8

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The extreme N-terminus of the Caulobacter crescentus surface-layer protein directs export of passenger proteins from the cytoplasm but is not required for secretion of the native protein

Bingle, Wade H. ; Le, Khai D. ; Smit, John

Canadian Science Publishing ; 1996

In: Canadian Journal of Microbiology Vol. 42, No. 7 ( 1996-07-01), p. 672-684

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In: Canadian Journal of Microbiology, Canadian Science Publishing, Vol. 42, No. 7 ( 1996-07-01), p. 672-684

Abstract: The paracrystalline surface layer (S-layer) of Caulobacter crescentus is composed of a single protein (RsaA, 1026 amino acids) that associates noncovalently with the lipopolysaccharide of the outer membrane. Like many other extracellular proteins of Gram-negative bacteria, the S-layer protein is not processed during transport to the cell surface. To study the secretion of RsaA, several N-terminal deletions of the protein were made by modifying the 5′-region of the rsaA gene. This analysis showed that portions of the N-terminus totalling the first 775 N-terminal amino acids (75% of the protein) could be removed from RsaA without abolishing secretion of the remainder of the protein. Although the RsaA N-terminus was not required for secretion, an N-terminal domain consisting of either 34 or 52 RsaA-derived amino acids promoted export of the alkaline phosphatase reporter (PhoA) and a cellulase reporter (ΔCenA) from the cytoplasm; using the cellulase reporter, the efficiency of hybrid protein export was estimated at 9%. No enzyme activity was detected in the cell-free culture fluids as the result of expressing any gene fusion, indicating that no hybrid protein was completely secreted from the cell. RsaA:PhoA hybrid proteins were also exported from the E. coli cytoplasm, a bacterium not expected to contain the necessary machinery for the secretion of RsaA. Taken together, these data indicate that the secretion pathway of RsaA relies on a C-terminal secretion signal and that once separated from the context of the native protein, the extreme N-terminus of RsaA can act as an inefficient cryptic export signal that is not used during native RsaA secretion.Key words: Caulobacter, S-layer, protein secretion.

Type of Medium: Online Resource

ISSN: 0008-4166 , 1480-3275

URL: Article

DOI: 10.1139/m96-092

RVK:

WA 15000

Language: English

Publisher: Canadian Science Publishing

Publication Date: 1996

detail.hit.zdb_id: 280534-0

detail.hit.zdb_id: 1481972-7

SSG: 12

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9

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Caulobacter crescentus Synthesizes an S-Layer-Editing Metalloprotease Possessing a Domain Sharing Sequence Similarity with Its Paracrystalline S-Layer Protein

Umelo-Njaka, Elizabeth ; Bingle, Wade H. ; Borchani, Faten ; [et al.]

American Society for Microbiology ; 2002

In: Journal of Bacteriology Vol. 184, No. 10 ( 2002-05-15), p. 2709-2718

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In: Journal of Bacteriology, American Society for Microbiology, Vol. 184, No. 10 ( 2002-05-15), p. 2709-2718

Abstract: Strains of Caulobacter crescentus elaborate an S-layer, a two-dimensional protein latticework which covers the cell surface. The S-layer protein (RsaA) is secreted by a type I mechanism (relying on a C-terminal signal) and is unusual among type I secreted proteins because high levels of protein are produced continuously. In efforts to adapt the S-layer for display of foreign peptides and proteins, we noted a proteolytic activity that affected S-layer monomers with foreign inserts. The cleavage was precise, resulting in fragments with an unambiguous N-terminal sequence. We developed an assay to screen for loss of this activity (i.e., presentation of foreign peptides without degradation), using transposon and traditional mutagenesis. A metalloprotease gene designated sap (S-layer-associated protease) was identified which could complement the protease-negative mutants. The N-terminal half of Sap possessed significant similarity to other type I secreted proteases (e.g., alkaline protease of Pseudomonas aeruginosa ), including the characteristic RTX repeat sequences, but the C-terminal half which normally includes the type I secretion signal exhibited no such similarity. Instead, there was a region of significant similarity to the N-terminal region of RsaA. We hypothesize that Sap evolved by combining the catalytic portion of a type I secreted protease with an S-layer-like protein, perhaps to associate with nascent S-layer monomers to “scan” for modifications.

Type of Medium: Online Resource

ISSN: 0021-9193 , 1098-5530

URL: Article

DOI: 10.1128/JB.184.10.2709-2718.2002

Language: English

Publisher: American Society for Microbiology

Publication Date: 2002

detail.hit.zdb_id: 1481988-0

SSG: 12

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10

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Transformation of Azotobacter vinelandii OP with a broad host range plasmid containing a cloned chromosomal nif-DNA marker

Bingle, Wade H.

Elsevier BV ; 1988

In: Plasmid Vol. 19, No. 3 ( 1988-5), p. 242-250

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In: Plasmid, Elsevier BV, Vol. 19, No. 3 ( 1988-5), p. 242-250

Type of Medium: Online Resource

ISSN: 0147-619X

URL: Article

DOI: 10.1016/0147-619X(88)90042-X

RVK:

WA 15000

Language: English

Publisher: Elsevier BV

Publication Date: 1988

detail.hit.zdb_id: 1471554-5

SSG: 12

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