The Surface Layer (S-layer) Glycoprotein of Geobacillus stearothermophilus NRS 2004/3a

Schäffer, Christina; Wugeditsch, Thomas; Kählig, Hanspeter; Scheberl, Andrea; Zayni, Sonja; Messner, Paul

doi:10.1074/jbc.m108873200

Cited by 70 publications

(108 citation statements)

References 49 publications

(35 reference statements)

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“…We found two anomeric protons at 5.32 ppm (H-1, α-anomer; d, J 1,2 =1.6 Hz) and 4.92 ppm (H-1, β-anomer; broad singlet), H-C-OH protons at 3.39-3.87 ppm, one O-methyl group at 3.51 ppm, and two methyl groups at 1.31 ppm (J 5,6 = 5.3 Hz) and 1.33 ppm (J 5,6 = 6.7 Hz) for the α and β anomers respectively. We found good agreement between our spectral data and 2-Omethylrhamnose as the terminal sugar in a glycan polymer (Schäffer et al, 2002).…”

Section: Fraction F 3 B: Separation Of F 3 B On Four Ag Columns Resulsupporting

confidence: 70%

“…In the HSQC spectrum we observed a correlation between βH-3 (3.37 ppm) and a carbon at 82.4 ppm, which we assigned as βC-3, further establishing the site of methylation. There is a cross peak between H-4 (3.45 ppm) and a carbon at 71.4 ppm, which we assigned as βC-4, in good agreement with the values assigned by Popper and Fry (2003) We used the same reasoning to identify F 3 B2 as a α/ß mixture of 2-Omethylrhamnose (XVI) (Zdorovenko et al 2001;Schäffer et al 2002). Fractions F 3 B1…”

Section: Fraction F 3 B: Separation Of F 3 B On Four Ag Columns Resulsupporting

confidence: 51%

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Characterization of methyl sugars, 3-deoxysugars and methyl deoxysugars in marine high molecular weight dissolved organic matter

Panagiotopoulos

Repeta

Johnson

2007

Organic Geochemistry

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Section: Fraction F 3 B: Separation Of F 3 B On Four Ag Columns Resulsupporting

confidence: 70%

Section: Fraction F 3 B: Separation Of F 3 B On Four Ag Columns Resulsupporting

confidence: 51%

Characterization of methyl sugars, 3-deoxysugars and methyl deoxysugars in marine high molecular weight dissolved organic matter

Panagiotopoulos

Repeta

Johnson

2007

Organic Geochemistry

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“…For the introduction of a distinctive protein N-glycosylation consensus sequence from the C. jejuni AcrA N-glycoprotein replacing the naturally O-glycosylation sites of the S-layer protein, [19,20] a modified sgsE gene containing an artificial KpnI site at position nt 1830 (corresponding to amino acid position 611), coding for a protein with a PelB signal peptide and lacking the amino acid sequence between L 610 and E 804 was constructed. N-and Cterminal parts of sgsE were amplified separately by PCR using the primer pairs A_sgsE_for(NcoI)/sgsEteil_rev(KpnI) and sgsE-teil_for(KpnI)/sgsE_rev(XhoI), respectively.…”

Section: Engineering Of N-glycosylation Sites On Sgsementioning

confidence: 99%

“…SgsE is a 903-amino acid protein, which includes a 30-amino acid signal peptide aligned by an entropy-driven process into a 2D crystalline array [8] with oblique (p2) symmetry exhibiting nanometer-scaled periodicity (lattice parameters: a = 11.6 nm, b = 9.4 nm, γ ≈ 78°). [18,19] SgsE was chosen for proof of concept because it is naturally O-glycosylated with long-chain poly-L-rhamnans linked via a β-D-galactose residue to the amino acids threonine 590 , threonine 620 , and serine 794 of the S-layer protein. [19,20] The protein-inherent glycosylation sites are predicted to form a loop structure that is spatially accessible to the glycosylation machinery of the bacterium.…”

Section: Introductionmentioning

confidence: 99%

“…[18,19] SgsE was chosen for proof of concept because it is naturally O-glycosylated with long-chain poly-L-rhamnans linked via a β-D-galactose residue to the amino acids threonine 590 , threonine 620 , and serine 794 of the S-layer protein. [19,20] The protein-inherent glycosylation sites are predicted to form a loop structure that is spatially accessible to the glycosylation machinery of the bacterium. Thus, these sites offer ideal targets for engineering of specific glycosylation sequences that would be recognized by heterologous oligosaccharyl:protein transferases, as required for S-layer neoglycoprotein design.…”

Section: Introductionmentioning

confidence: 99%

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Recombinant Glycans on an S‐Layer Self‐Assembly Protein: A New Dimension for Nanopatterned Biomaterials

Steiner

Hanreich

Kainz

et al. 2008

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Crucial biological phenomena are mediated through carbohydrates that are displayed in a defined manner and interact with molecular scale precision. We lay the groundwork for the integration of recombinant carbohydrates into a "biomolecular construction kit" for the design of new biomaterials, by utilizing the self-assembly system of the crystalline cell surface (S)-layer protein SgsE of Geobacillus stearothermophilus NRS 2004/3a. SgsE is a naturally O-glycosylated protein, with intrinsic properties that allow it to function as a nanopatterned matrix for the periodic display of glycans. By using a combined carbohydrate/protein engineering approach, two types of S-layer neoglycoproteins are produced in Escherichia coli. Based on the identification of a suitable periplasmic targeting system for the SgsE self-assembly protein as a cellular prerequisite for Europe PMC Funders Author ManuscriptsEurope PMC Funders Author Manuscripts protein glycosylation, and on engineering of one of the natural protein O-glycosylation sites into a target for N-glycosylation, the heptasaccharide from the AcrA protein of Campylobacter jejuni and the O7 polysaccharide of E. coli are co-or post-translationally transferred to the S-layer protein by the action of the oligosaccharyltransferase PglB. The degree of glycosylation of the Slayer neoglycoproteins after purification from the periplasmic fraction reaches completeness. Electron microscopy reveals that recombinant glycosylation is fully compatible with the S-layer protein self-assembly system. Tailor-made ("functional") nanopatterned, self-assembling neoglycoproteins may open up new strategies for influencing and controlling complex biological systems with potential applications in the areas of biomimetics, drug targeting, vaccine design, or diagnostics.

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Self‐assembling Protein Systems: Microbial S‐layers

Sleytr¹,

Sára²,

Pum³

et al. 2002

Biopolymers Online

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Introduction Historical Outline Occurrence and Ultrastructure Isolation and Chemical Characterization Molecular Biology, Genetics and Biosynthesis Assembly and Morphogenesis Self‐assembly in vivo Self‐assembly in vitro Functional Aspects Biodegradation Production of S‐layer Proteins Application of S‐layer Proteins S‐layer Ultrafiltration Membranes S‐layers as Matrix for the Immobilization of Functional Macromolecules S‐layer‐based Dipsticks Supramolecular Structures Generated by Oriented Recrystallization of S‐layer Fusion Proteins on Supports Precoated with SCWP S‐layers as Templates for the Formation of Regularly Arranged Nanoparticles S‐layers as Supporting Structures for Functional Lipid Membranes (Planar Membranes and Liposomes) S‐layers for Vaccine Development Outlook and Perspectives Patents

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The Surface Layer (S-layer) Glycoprotein of Geobacillus stearothermophilus NRS 2004/3a

Cited by 70 publications

References 49 publications

Characterization of methyl sugars, 3-deoxysugars and methyl deoxysugars in marine high molecular weight dissolved organic matter

Characterization of methyl sugars, 3-deoxysugars and methyl deoxysugars in marine high molecular weight dissolved organic matter

Recombinant Glycans on an S‐Layer Self‐Assembly Protein: A New Dimension for Nanopatterned Biomaterials

Self‐assembling Protein Systems: Microbial S‐layers

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