Quantitative evaluation of bone resorption activity of osteoclast‐like cells by measuring calcium phosphate resorbing area using incubator‐facilitated and video‐enhanced microscopy

Quantitative evaluation of the ability of bone resorption activity in live osteoclast‐like cells (OCLs) has not yet been reported on. In this study, we observed the sequential morphological change of OCLs and measured the resorbing calcium phosphate (CP) area made by OCLs alone and with the addition of elcatonin utilizing incubator facilitated video‐enhanced microscopy. OCLs, which were obtained from a coculture of ddy‐mouse osteoblastic cells and bone marrow cells, were cultured on CP‐coated quartz cover slips. The CP‐free area increased constantly in the OCLs alone, whereas it did not increase after the addition of elcatonin. This study showed that analysis of the resorbed areas under the OCL body using this method enables the sequential quantitative evaluation of the bone resorption activity and the effect of several therapeutic agents on bone resorption in vitro. Microsc. Res. Tech, 2009. © 2008 Wiley‐Liss, Inc.     

Intramammary challenge of lipopolysaccharide stimulates secretion of lingual antimicrobial peptide into milk of dairy cows

Lingual antimicrobial peptide (LAP) belongs to the β-defensin family in cattle and is found in bovine milk. However, it is unclear whether LAP is involved in the early immune response to mammary infection. The aim of the study was to investigate the changes of LAP concentration in milk after intramammary challenge with lipopolysaccharide (LPS), the gram-negative bacteria cell membrane component, in dairy cows. Milk was collected before and after LPS or phosphate-buffered saline (control) challenge every hour for 12 h on d 0 and twice daily from d 1 to 7. Somatic cell count (SCC), LAP concentration, and lactoperoxidase (LPO) activity in the milk were measured. Somatic cell count started to increase at 2 h postchallenge and remained high until d 5 (694 ± 187 × 10³ to >1,000 ± 0 × 10³ cells/mL at d 0; >1,000 ± 0 × 10³ cells/mL at d 1 to 3; 684 ± 194 × 10³ to 829 ± 108 × 10³ cells/mL at d 4; 527 ± 197 × 10³ to 656 ± 145 × 10³ cells/mL at d 5). Somatic cell count increased in the control cows, although the levels were lower compared with those in the LPS challenge group. The LAP concentration in milk increased significantly at 2 h post-LPS-challenge and was maintained at high levels until d 2 (8.6 ± 0.6 to 17.5 ± 2.3 nM). In the control cow infused with phosphate-buffered saline, there was no increase of LAP concentration in milk (5.1 ± 0.6 to 7.2 ± 0.8 nM). Increase of LPO activity in the milk was observed at 6 h after LPS challenge and continued until d 3 (4.7 ± 0.3 to 9.4 ± 1.1 U). No increase of LPO activity was observed in the milk of control cows. The increase and subsequent decrease in LAP concentration after LPS challenge occurred earlier than those of LPO activity. In multiparous cows with LPS infusion, there was a significantly negative relationship between the days leading to the basal levels in LAP concentration and LPO activity (r = −0.75). These results suggest that LPS induces secretion of LAP into milk within hours and that LPO may have a synergistic antimicrobial function with LAP in mammary glands of dairy cows.     

Effects of Window Size on Accuracy and Spatial Resolution in Windowed Phase‐Shifting Digital Holographic Interferometry1

Abstract: Phase‐shifting digital holographic interferometry is a new method to measure displacement distribution on the surface of an object. Usually holography has speckle noise, which leads to a large error in the analysis of displacement and strain distributions. We previously proposed windowed phase‐shifting digital holographic interferometry (windowed PSDHI). The use of this method leads to accurate displacement analysis, decreasing the effect of speckle patterns. However, noise reduction involves a defect, which renders the spatial resolution low. In this paper, by comparing the conventional noise reduction method using spatial averaging with the windowed PSDHI on spatial resolution, the effectiveness of noise reduction is discussed.     

Identification of Specimen Position and Orientation Using Standard Deviation of Intensity in Phase‐Shifting Digital Holography1

Abstract: Phase‐shifting digital holography is a useful method to measure the displacement distribution and the strain distribution of an object surface. The complex amplitude distribution of an object surface is obtained as the complex amplitude distribution at a reconstruction distance. It is, however, difficult to measure the reconstruction distance by actual measurement. We discovered that the standard deviation of the intensity on the reconstructed image becomes the maximum value when the reconstruction distance is the same as the actual optical path length. The displacement distributions are obtained for the x‐, y‐ and z‐directions. When the normal direction of an object surface inclines from the z‐direction, the displacements defined on the xyz‐coordinate system should be transformed into the object coordinate system. It is, therefore, required to develop a measurement method of the orientation of the object to obtain the parameters for transforming from the xyz‐coordinate system into the object coordinate system. In this paper, the method to identify the position and the orientation of a specimen using the standard deviation of the intensity distribution is proposed.     

Some properties of boronized layers on steels with direct diode laser

Boronized layer on steel is known to be formed by thermal diffusion of boron into the surface of steel improving corrosion-erosion resistant properties. Boronizing is carried out at temperatures ranging from 800 °C to 1050 °C and takes from one to several hours. There is one problem in this process, however, that the structure and properties of the base material are influenced considerably by the high temperature and long time of treatment. In order to avoid the aforementioned drawbacks of pack boronizing and laser-assisted boronizing, a better way is to activate the pack boronizing media and the workpiece with a high density power. The laser boronizing processes do not change the properties of the base material. In this study, the effect of laser characteristics was examined on the laser boronizing of carbon steel. After laser boronizing, the microstructure of the boride layer was analysed with an optical microscope and X-ray diffractometer (XRD). The mechanical properties of borided layer are evaluated using Vickers hardness tester and sand erosion tester. Results showed that the boride layer was composed of FeB and Fe₂B with thickness ranging 200-300 μm. The laser boronizing process did not change the properties of the base material.     

Application of microbial genes to recalcitrant biomass utilization and environmental conservation

Recent papers concerning the application of microbial genes to recalcitrant biomass utilization and environmental conservation are reviewed. Microbial genes have been integrated and expressed in plants and microorganisms. When cellulose-degrading enzyme genes are expressed in rice plants, the transgenic plants exhibit swollen cell walls which increases the digestibility of rice straw in the rumen. When genes encoding aromatic compound-degrading enzymes are expressed in plants, it is expected that aromatic compounds contaminating soil would be degraded during the growth of the transgenic plants. The former transgenic plants are utilized as feed and the latter for phytoremediation. Dockerin and cohesin interactions occurring in the cellulase complex, cellulosome, are applied to the construction of artificial enzyme complexes and protein purification by expressing the genes in transformed bacteria and/or silkworms, respectively. In the case of the forced expression of bacterial genes encoding chitinase and/or hydrogenase in the wild-type bacteria, chitin degradation and hydrogen gas production in the transformed bacteria occur at much higher rates than in the wild type.     

Reconsideration of the quantitative characterization of the reaction intermediate on electrocatalysts by a rotating ring-disk electrode: The intrinsic yield of H2O2 on Pt/C

To solve the problem of the catalyst-loading-effect on quantifying the reaction intermediates on the surface of electrocatalysts with a rotating ring-disk electrode, we studied the formation of hydrogen peroxide in the oxygen reduction reaction on Pt/C with various sample loadings and then proposed an extrapolation model for measuring the intrinsic yield of H₂O₂, which can quantitatively reflect the characteristics of the surface of a given catalyst. In the extrapolation model, the catalyst loading effect can be compensated by taking the catalyst loading-dependent probability of the re-adsorption + further reaction of the desorbed H₂O₂ into consideration. The core concept in this extrapolation model is that the probability of the re-adsorption + reaction of the desorbed H₂O₂ becomes zero if there is no other active site available (i.e., at the extrapolated hypothetical point of zero catalyst loading) for re-adsorption of the desorbed H₂O₂. The intrinsic yield of H₂O₂ by extrapolation was much higher than that measured by the conventional model, in which the re-adsorption + reaction of the desorbed H₂O₂ is not considered, and thus the catalyst loading-dependent apparent yield of H₂O₂ does not properly reflect the intrinsic characteristics of the surface of a given catalyst.     

Flexizymes: their evolutionary history and the origin of catalytic function

Transfer RNA (tRNA) is an essential component of the cell's translation apparatus. These RNA strands contain the anticodon for a given amino acid, and when "charged" with that amino acid are termed aminoacyl-tRNA. Aminoacylation, which occurs exclusively at one of the 3'-terminal hydroxyl groups of tRNA, is catalyzed by a family of enzymes called aminoacyl-tRNA synthetases (ARSs). In a primitive translation system, before the advent of sophisticated protein-based enzymes, this chemical event could conceivably have been catalyzed solely by RNA enzymes. Given the evolutionary implications, our group attempted in vitro selection of artificial ARS-like ribozymes, successfully uncovering a functional ribozyme (r24) from an RNA pool of random sequences attached to the 5'-leader region of tRNA. This ribozyme preferentially charges aromatic amino acids (such as phenylalanine) activated with cyanomethyl ester (CME) onto specific kinds of tRNA. During the course of our studies, we became interested in developing a versatile, rather than a specific, aminoacylation catalyst. Such a ribozyme could facilitate the preparation of intentionally misacylated tRNAs and thus serve a convenient tool for manipulating the genetic code. On the basis of biochemical studies of r24, we constructed a truncated version of r24 (r24mini) that was 57 nucleotides long. This r24mini was then further shortened to 45 nucleotides. This ribozyme could charge various tRNAs through very simple three-base-pair interactions between the ribozyme's 3'-end and the tRNA's 3'-end. We termed this ribozyme a "flexizyme" (Fx3 for this particular construct) owing to its flexibility in addressing tRNAs. To devise an even more flexible tool for tRNA acylation, we attempted to eliminate the amino acid specificity from Fx3. This attempt yielded an Fx3 variant, termed dFx, which accepts amino acid substrates having 3,5-dinitrobenzyl ester instead of CME as a leaving group. Similar selection attempts with the original phenylalanine-CME and a substrate activated by (2-aminoethyl)amidocarboxybenzyl thioester yielded the variants eFx and aFx (e and a denote enhanced and amino, respectively). In this Account, we describe the history and development of these flexizymes and their appropriate substrates, which provide a versatile and easy-to-use tRNA acylation system. Their use permits the synthesis of a wide array of acyl-tRNAs charged with artificial amino and hydroxy acids. In parallel to these efforts, we initiated a crystallization study of Fx3 covalently conjugated to a microhelix RNA, which is an analogue of tRNA. The X-ray crystal structure, solved as a co-complex with phenylalanine ethyl ester and U1A-binding protein, revealed the structural basis of this enzyme. Most importantly, many biochemical observations were consistent with the crystal structure. Along with the predicted three regular-helix regions, however, the flexizyme has a unique irregular helix that was unexpected. This irregular helix constitutes a recognition pocket for the aromatic ring of the amino acid side chain and precisely brings the carbonyl group to the 3'-hydroxyl group of the tRNA 3'-end. This study has clearly defined the molecular interactions between Fx3, tRNA, and the amino acid substrate, revealing the fundamental basis of this unique catalytic system.     

Ex Vivo Expanded and Activated Natural Killer Cells Prolong the Overall Survival of Mice with Glioblastoma-like Cell-Derived Tumors

Glioblastoma (GBM) is the leading malignant intracranial tumor and is associated with a poor prognosis. Highly purified, activated natural killer (NK) cells, designated as genuine induced NK cells (GiNKs), represent a promising immunotherapy for GBM. We evaluated the anti-tumor effect of GiNKs in association with the programmed death 1(PD-1)/PD-ligand 1 (PD-L1) immune checkpoint pathway. We determined the level of PD-1 expression, a receptor known to down-regulate the immune response against malignancy, on GiNKs. PD-L1 expression on glioma cell lines (GBM-like cell line U87MG, and GBM cell line T98G) was also determined. To evaluate the anti-tumor activity of GiNKs in vivo, we used a xenograft model of subcutaneously implanted U87MG cells in immunocompromised NOG mice. The GiNKs expressed very low levels of PD-1. Although PD-L1 was expressed on U87MG and T98G cells, the expression levels were highly variable. Our xenograft model revealed that the retro-orbital administration of GiNKs and interleukin-2 (IL-2) prolonged the survival of NOG mice bearing subcutaneous U87MG-derived tumors. PD-1 blocking antibodies did not have an additive effect with GiNKs for prolonging survival. GiNKs may represent a promising cell-based immunotherapy for patients with GBM and are minimally affected by the PD-1/PD-L1 immune evasion axis in GBM.