Small‐Angle Scattering of S‐Layer Metallization

Aichmayer, Barbara; Mertig, Michael; Kirchner, Alexander; Paris, Oskar; Fratzl, Peter

doi:10.1002/adma.200501646

Cited by 25 publications

(29 citation statements)

References 28 publications

(35 reference statements)

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“…A 2-layer sandwich architecture has been observed for the N-terminal domain of the C. difficile SLP [96], three triple-helix bundles for the N-terminal domain of the SbsC SLP from G. stearothermophilus [97], and a β-propeller fold for a putative SLP of the archaeal Methanosarcina acetivorans [98] and the Gram-negative bacteria Bacteroides uniformis [99]. This technique has also been used to analyze the formation of Pd nanoparticles on crystalline bacterial S-layers, showing the response of the S-layer lattice to the loading with Pd complexes and metallic Pd particles as well as the effects of two different reducing agents (H 2 and dimethylaminoborane) on the nanoparticle arrays [100].…”

Section: X-ray Crystallography and Small Angle X-ray Scatteringmentioning

confidence: 99%

Biophysical Methods for the Elucidation of the S-Layer Proteins/Metal Interaction

Mobili

2013

IJBCRR

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Surface-layers (S-layers) are macromolecular paracrystalline arrays of proteins or glycoproteins that can self-assemble into 2-dimensional semi-permeable meshworks to overlay the cell surface of many bacteria and archaea. They usually assemble into lattices with oblique, square or hexagonal symmetry and serve as an interface between the bacterial cell and the environment. Isolated S-layers can recrystallize into two-dimensional regular arrays in suspension or on various surfaces, thus being an appropriate material for several bionanotechnological purposes. Promising applications of S-layers include their use as biotemplates for the capture of metal ions or the synthesis of metal nanoclusters. Research ArticleInternational Journal of Biochemistry Research & Review, 3(1): 39-62, 2013 40 Considering the use of S-layers as biotemplates for the organization of metal ions or metallic nanoclusters, research on potential of surface layer proteins (SLP) and metals can be understood as an interdisciplinary field, in which different biophysical techniques supply complementary information. In this review, we discuss the SLP as native or engineered "bottom-up" building blocks for metal immobilization structures. We also describe the biophysical techniques used to analyze metal binding properties as well as the information obtained from the investigation of these structures.

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Section: X-ray Crystallography and Small Angle X-ray Scatteringmentioning

confidence: 99%

Biophysical Methods for the Elucidation of the S-Layer Proteins/Metal Interaction

Mobili

2013

IJBCRR

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“…The possibility to reconstitute isolated S-layer monomers in vitro into two-dimensional (2D) arrays with perfect uniformity [5,6] makes them an almost ideal biological template for supra-molecular engineering. Taking advantage of their spatially well-defined physical and chemical surface properties, S layers have extensively been used for the template-directed chemical synthesis of regular 2D semiconducting [7,8] and metallic [9][10][11][12][13][14] nanoparticle arrays. The specific property that their regular 2D structure is preserved under dry conditions [14] has recently allowed using S layers as templates for the organization of gasphase deposited FePt nanoparticles into 2D arrays [15][16][17].…”

Section: Introductionmentioning

confidence: 99%

“…Taking advantage of their spatially well-defined physical and chemical surface properties, S layers have extensively been used for the template-directed chemical synthesis of regular 2D semiconducting [7,8] and metallic [9][10][11][12][13][14] nanoparticle arrays. The specific property that their regular 2D structure is preserved under dry conditions [14] has recently allowed using S layers as templates for the organization of gasphase deposited FePt nanoparticles into 2D arrays [15][16][17]. In addition, the electronic structure of S layers has been investigated by photoemission and NEXAFS spectroscopy [18][19][20][21][22].…”

Section: Introductionmentioning

confidence: 99%

Catalytic Carbon Monoxide Oxidation Using Bio-Templated Platinum Clusters

et al. 2009

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The catalytic properties of highly dispersed, bacterial surface layer supported nanoscale platinum clusters immobilized at alumina particles are studied with respect to carbon monoxide oxidation. Compared to samples prepared from platinum impregnated alumina, the templated metal clusters are catalytically active at lower temperatures. The catalytic behaviour of the samples is discussed with respect to their cluster morphology studied by TEM.

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“…In the case of interaction of the proteins, such as in lattices of noncovalently linked S-layer proteins, the structure factor value differs from 1, which considerably complicates procedures to gain information on the system. With regard to S-layers, SAXS has been used to describe the wet chemical metallization of S-layers under different chemical conditions (21). There, an approach was chosen to model the scattering intensity at low values of the scattering vector q by a mixture of mono-and bilayers and the scattering intensity at high q values by a square lattice as concluded from reconstruction of TEM images (21).…”

mentioning

confidence: 99%

“…With regard to S-layers, SAXS has been used to describe the wet chemical metallization of S-layers under different chemical conditions (21). There, an approach was chosen to model the scattering intensity at low values of the scattering vector q by a mixture of mono-and bilayers and the scattering intensity at high q values by a square lattice as concluded from reconstruction of TEM images (21). Furthermore, protein-protein interaction within the S-layer was taken into account by combining molecular dynamics simulations and refining the model with experimental SAXS data (22), where the subunit also was modeled on the amino acid level (23).…”

mentioning

confidence: 99%

Small-Angle X-Ray Scattering for Imaging of Surface Layers on Intact Bacteria in the Native Environment

et al. 2013

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Crystalline cell surface layers (S-layers) represent a natural two-dimensional (2D) protein self-assembly system with nanometerscale periodicity that decorate many prokaryotic cells. Here, we analyze the S-layer on intact bacterial cells of the Gram-positive organism Geobacillus stearothermophilus ATCC 12980 and the Gram-negative organism Aquaspirillum serpens MW5 by smallangle X-ray scattering (SAXS) and relate it to the structure obtained by transmission electron microscopy (TEM) after platinum/ carbon shadowing. By measuring the scattering pattern of X rays obtained from a suspension of bacterial cells, integral information on structural elements such as the thickness and lattice parameters of the S-layers on intact, hydrated cells can be obtained nondestructively. In contrast, TEM of whole mounts is used to analyze the S-layer lattice type and parameters as well as the physical structure in a nonaqueous environment and local information on the structure is delivered. Application of SAXS to S-layer research on intact bacteria is a challenging task, as the scattering volume of the generally thin (3-to 30-nm) bacterial S-layers is low in comparison to the scattering volume of the bacterium itself. For enhancement of the scattering contrast of the S-layer in SAXS measurement, either silicification (treatment with tetraethyl orthosilicate) is used, or the difference between SAXS signals from an S-layer-deficient mutant and the corresponding S-layer-carrying bacterium is used for determination of the scattering signal. The good agreement of the SAXS and TEM data shows that S-layers on the bacterial cell surface are remarkably stable. Surface layers (S-layers) are a distinct cell surface decoration comprised of regularly arrayed, two-dimensional (2D) protein or glycoprotein crystals present on many prokaryotic organisms from almost all known phylogenetic branches (1-4). S-layers form upon self-assembly and exhibit nanometer-scale periodicity with oblique (p1, p2), square (p4), or hexagonal (p3, p6) lattice symmetry and species-specific lattice constant values in the range of 10 to 25 nm. The S-layer self-assembly system holds great promise as a bottom-up approach for organizing matter at the nanometer scale as required in the field of nanobiotechnology (5).Because of their cell surface location, ultrastructural studies of S-layer lattices have been frequently performed by high-resolution transmission electron microscopic (TEM) methods such as ultrathin sectioning or heavy-metal shadow casting of freezeetched or freeze-dried whole cells (6) as well as image analysis (7) or cryo-sectioning of frozen-hydrated cells (8). These electron microscopic approaches, except the latter, suffer from the drawback of the requirement for water-free specimens, implying a requirement for specific sample treatment prior to analysis. The standard procedures of chemical fixation, dehydration, and staining of cells for TEM analysis may affect cell morphology and ultrastructure and, thus, prevent the accurate determination of distinct S-l...

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Small‐Angle Scattering of S‐Layer Metallization

Cited by 25 publications

References 28 publications

Biophysical Methods for the Elucidation of the S-Layer Proteins/Metal Interaction

Biophysical Methods for the Elucidation of the S-Layer Proteins/Metal Interaction

Catalytic Carbon Monoxide Oxidation Using Bio-Templated Platinum Clusters

Small-Angle X-Ray Scattering for Imaging of Surface Layers on Intact Bacteria in the Native Environment

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