Jussi-Petteri Suuronen

Analysis of short fibres orientation in steel fibre-reinforced concrete (SFRC) by X-ray tomography

The mechanical properties of fibre composite materials are largely determined by the orientation of fibres within the matrix. Which orientation distribution short fibres follow in different parts of a structural element is still a subject for research and discussions in the scientific community. In this article, we present a modern and advanced method for measuring the orientation of short fibres in steel fibre-reinforced concrete (SFRC) by X-ray microtomography. With this method, a voxel image of the fibres is obtained directly in 3D, and the orientation of each individual fibre is calculated based on a skeletonized representation of this image. Scans of 12 SFRC samples, taken from the central height region of real-size floor slabs, reveal the fibres to be mostly horizontally oriented near the centre of a floor slab and more vertically oriented near the edge; here the alignment with the formwork dominates. The fibre orientation distributions are characterized by several orientation parameters as quantitative measures for the alignment. On the practical side, this method has the potential to be incorporated into the development and production process of SFRC structures to verify how the fibres contribute to capacity.

X-ray scattering and microtomography study on the structural changes of never-dried silver birch, European aspen and hybrid aspen during drying

Abstract The impact of drying on the structure of the never-dried hardwood cell wall was studied at nanometer level by means of wide- and small-angle X-ray scattering (WAXS, SAXS), and at micrometer level by X-ray microtomography (μCT). Never-dried silver birch, European aspen and hybrid aspen samples were measured by WAXS in situ during drying in air. The samples included juvenile and mature wood, as well as normal and tension wood to allow comparison of the effects of different matrix compositions and microfibril angles. The deformations of cellulose crystallites and amorphous components of the cell wall were detected as changes in the cellulose reflections 200 and 004 and amorphous halo in the WAXS patterns. Especially, the width of the reflection 004, corresponding to the cellulose chain direction, increased due to drying in all the samples, indicating an increase of strain and disorder of the chains. Also, the cellulose unit cell shrank 0.2–0.3% during drying in this direction in all the samples except in hybrid aspen tension wood. According to the SAXS results of silver birch, the distance between micro-fibrils decreased during drying. It was detected by μCT that the mean cross-sectional maximum width of the parenchymatous rays decreased from that of never-dried to air-dried birch by roughly 16%.

Effects of pressurized hot water extraction on the nanoscale structure of birch sawdust

Pressurized hot water extraction with a flow-through system was used to extract hemicelluloses and lignin from birch sawdust. The structure of the extraction residue was studied on various levels. Molecular mass distributions were determined with gel permeation chromatography and the crystal structure of cellulose was characterized using wide-angle X-ray scattering (WAXS). Information on the short-range order of cellulose microfibrils and on the nanoscale pore structure was obtained with small-angle X-ray scattering (SAXS), and the micrometre scale cellular morphology was imaged with X-ray microtomography. The pressurized hot water treatment was observed to increase the lateral width of cellulose crystallites, determined with WAXS, whereas a possible small decrease in the crystallinity of cellulose compared to native wood was detected. The molecular mass of cellulose remained at a relatively high level. According to the SAXS results, a tighter lateral association of cellulose microfibrils was observed in the extracted samples, which possibly led to opening of pores between bundles of microfibrils, as indicated by an increased specific surface area. A reduction in the thickness of the fibre cell walls was evidenced by X-ray microtomography.

Enzymatic oxidation as a potential new route to produce polysaccharide aerogels

Specific enzymatic oxidation of terminal galactosyl-containing polysaccharides (guar galactomannan (GM), and tamarind seed galactoxyloglucan (XG)) was used to prepare hydrogels. The hydrogels were lyophilized to form novel types of polysaccharide aerogels: biobased and biodegradable, lightweight, and stiff materials. The compressive moduli of the aerogels were greatly dependent on the oxidation, polysaccharide type, freezing method, and ambient moisture. Ice crystal templated, oriented aerogels from oxidized XG (XG-OX) showed the highest compressive modulus, 359 kPa, when determined parallel to the freezing and drying direction (i.e., the vertical direction). The water vapor sorption of freeze-dried GM and XG was not significantly affected by oxidation, even though the oxidized GM (GM-OX) and XG-OX aerogels were no longer water-soluble. GM-OX and XG-OX aerogels absorbed liquid water 40 and 20 times their initial weight, respectively. Focused ion beam scanning electron microscopy showed that the inner structure of oriented aerogels from GM-OX consisted of a honeycomb architecture with a pore diameter of some tens of micrometers. On the other hand, corresponding aerogels from XG-OX seemed to contain longer capillaries oriented in the freezing direction. This observation was supported by imaging the XG-OX aerogels using high-resolution synchrotron X-ray microtomography. The enzymatic hydro- and aerogel preparation method is considered a green way to obtain novel, functional products from polysaccharides.

Determining collagen distribution in articular cartilage using contrast-enhanced micro-computed tomography

Summary Objective Collagen distribution within articular cartilage (AC) is typically evaluated from histological sections, e.g., using collagen staining and light microscopy (LM). Unfortunately, all techniques based on histological sections are time-consuming, destructive, and without extraordinary effort, limited to two dimensions. This study investigates whether phosphotungstic acid (PTA) and phosphomolybdic acid (PMA), two collagen-specific markers and X-ray absorbers, could (1) produce contrast for AC X-ray imaging or (2) be used to detect collagen distribution within AC. Method We labeled equine AC samples with PTA or PMA and imaged them with micro-computed tomography (micro-CT) at pre-defined time points 0, 18, 36, 54, 72, 90, 180, 270 h during staining. The micro-CT image intensity was compared with collagen distributions obtained with a reference technique, i.e., Fourier-transform infrared imaging (FTIRI). The labeling time and contrast agent producing highest association (Pearson correlation, Bland–Altman analysis) between FTIRI collagen distribution and micro-CT -determined PTA distribution was selected for human AC. Results Both, PTA and PMA labeling permitted visualization of AC features using micro-CT in non-calcified cartilage. After labeling the samples for 36 h in PTA, the spatial distribution of X-ray attenuation correlated highly with the collagen distribution determined by FTIRI in both equine (mean ± S.D. of the Pearson correlation coefficients, r = 0.96 ± 0.03, n = 12) and human AC (r = 0.82 ± 0.15, n = 4). Conclusions PTA-induced X-ray attenuation is a potential marker for non-destructive detection of AC collagen distributions in 3D. This approach opens new possibilities in development of non-destructive 3D histopathological techniques for characterization of OA.

Seasonal variation in formation, structure, and chemical properties of phloem in Picea abies as studied by novel microtechniques

AbstractMain conclusionPhloem production and structural development were interlinked with seasonal variation in the primary and secondary metabolites of phloem. Novel microtechniques provided new perspectives on understanding phloem structure and chemistry. To gain new insights into phloem formation in Norway spruce (Picea abies), we monitored phloem cell production and seasonal variation in the primary and secondary metabolites of inner bark (non-structural carbohydrates and phenolic stilbene glucosides) during the 2012 growing season in southern and northern Finland. The structure of developing phloem was visualised in 3D by synchrotron X-ray microtomography. The chemical features of developing phloem tissues isolated by laser microdissection were analysed by chemical microanalysis. Within-year phloem formation was associated with seasonal changes in non-structural carbohydrates and phenolic extractive contents of inner bark. The onset of phloem cell production occurred in early and mid-May in southern and northern Finland, respectively. The maximal rate of phloem production and formation of a tangential band of axial phloem parenchyma occurred in mid-June, when total non-structural carbohydrates peaked (due to the high amount of starch). In contrast, soluble sugar content dropped during the most active growth period and increased in late summer and winter. The 3D visualisation showed that the new axial parenchyma clearly enlarged from June to August. Sub-cellular changes appeared to be associated with accumulation of stilbene glucosides and soluble sugars in the newest phloem. Stilbene glucosides also increased in inner bark during late summer and winter. Our findings may indicate that stilbene biosynthesis in older phloem predominantly occurs after the formation of the new band(s) of axial parenchyma. The complementary use of novel microtechniques provides new perspectives on the formation, structure, and chemistry of phloem.

Visualizing water-filled versus embolized status of xylem conduits by desktop x-ray microtomography

BackgroundThe hydraulic conductivity of the stem is a major factor limiting the capability of trees to transport water from the soil to transpiring leaves. During drought conditions, the conducting capacity of xylem can be reduced by some conduits being filled with gas, i.e. embolized. In order to understand the dynamics of embolism formation and repair, considerable attention has been given to developing reliable and accurate methods for quantifying the phenomenon. In the past decade, non-destructive imaging of embolism formation in living plants has become possible. Magnetic resonance imaging has been used to visualize the distribution of water within the stem, but in most cases it is not possible to resolve individual cells. Recently, high-resolution synchrotron x-ray microtomography has been introduced as a tool to visualize the water contents of individual cells in vivo, providing unprecedented insight into the dynamics of embolism repair. We have investigated the potential of an x-ray tube -based microtomography setup to visualize and quantify xylem embolism and embolism repair in water-stressed young saplings and shoot tips of Silver and Curly birch (Betula pendula and B. pendula var. carelica).ResultsFrom the microtomography images, the water-filled versus gas-filled status of individual xylem conduits can be seen, and the proportion of stem cross-section that consists of embolized tissue can be calculated. Measuring the number of embolized vessels in the imaged area is a simple counting experiment. In the samples investigated, wood fibers were cavitated in a large proportion of the xylem cross-section shortly after watering of the plant was stopped, but the number of embolized vessels remained low several days into a drought period. Under conditions of low evaporative demand, also refilling of previously embolized conduits was observed.ConclusionsDesktop x-ray microtomography is shown to be an effective method for evaluating the water-filled versus embolized status of the stem xylem in a small living sapling. Due to its non-destructive nature, the risk of inducing embolisms during sampling is greatly reduced. Compared with synchrotron imaging beamlines, desktop microtomography offers easier accessibility, while maintaining sufficient resolution to visualize the water contents of individual cells.

High-resolution X-ray computed microtomography: A holistic approach to metamorphic fabric analyses

An intrinsic limitation of studying microstructures in thin section is that their spatial (three-dimensional, 3-D) distribution, shape, and orientation have to be inferred by combining 2-D data from different sections. This procedure always involves some degree of interpretation that in some cases can be ambiguous. Recent advances in high-resolution X-ray computed microtomography have made possible the direct imaging in 3-D of volumes of rock to centimeter scale. This rapidly evolving technology is nondestructive and provides a holistic approach of microstructural analysis that eliminates interpretative procedures associated with 2-D methods. Spatial images can be generated through any part of the rock sample and used as virtual petrographic sections. Our application of this technique to an oriented drill core sample from the classic Orijarvi metamorphic region of southern Finland reveals a number of in situ 3-D aspects, including: (1) the spatial distribution and shape of andalusite porphyroblasts, (2) the geometry of a matrix foliation anastomosing around the porphyroblasts, (3) a millimeter-scale compositional layering that controlled the oscillation of porphyroblasts and sulfide mineralization, and (4) distinct inclusion trail patterns characterizing porphyroblast core versus rim zones. The combined data indicate that the steeply dipping bedding-subparallel foliation that characterizes the Orijarvi area formed by bulk north-south crustal shortening and associated vertical stretching.

Methods for fibre orientation analysis of X-ray tomography images of steel fibre reinforced concrete (SFRC)

One of the most important factors to determine the mechanical properties of a fibre composite material is the orientation of the fibres in the matrix. This paper presents Hessian matrix-based algorithms to retrieve the orientation of individual fibres out of steel fibre reinforced cementitious composites samples scanned with an X-ray computed tomography scanner. The software implemented with the algorithms includes a massive data filtering component to remove noise from the data-sets and prepare them correctly for the analysis. Due to its short computational times and limited need for user intervention, the software is able to process and analyse large batches of data in short periods and provide results in a variety of visual and numerical formats. The application and comparison of these algorithms lead to further insight into the material behaviour. In contrast to the usual assumption that the fibres act only along their main axis, it is shown that the contribution of hooked-end fibres in other directions may be noticeable. This means that fibres, depending on their shape, should act as orthotropic inclusions. The methods can be used by research laboratories and companies on an everyday basis to obtain fibre orientations from samples, which in turn can be used in research, to study stress–strain behaviour, as input to constitutive models or for quality assurance.

Delivering Agents Locally into Articular Cartilage by Intense MHz Ultrasound

There is no cure for osteoarthritis. Current drug delivery relies on systemic delivery or injections into the joint. Because articular cartilage (AC) degeneration can be local and drug exposure outside the lesion can cause adverse effects, localized drug delivery could permit new drug treatment strategies. We investigated whether intense megahertz ultrasound (frequency: 1.138 MHz, peak positive pressure: 2.7 MPa, Ispta: 5 W/cm2, beam width: 5.7 mm at −6 dB, duty cycle: 5%, pulse repetition frequency: 285 Hz, mechanical index: 1.1) can deliver agents into AC without damaging it. Using ultrasound, we delivered a drug surrogate down to a depth corresponding to 53% depth of the AC thickness without causing histologically detectable damage to the AC. This may be important because early osteoarthritis typically exhibits histopathologic changes in the superficial AC. In conclusion, we identify intense megahertz ultrasound as a technique that potentially enables localized non-destructive delivery of osteoarthritis drugs or drug carriers into articular cartilage.