Electron Microscope Observation of Microspore Division of Wheat in Vitro

First mitosis of wheat microspores in anther culture was studied by electron microscope. The division types of the most pollen grains were unequal (A pathway) and that of others were equal (B pathway). The characteristics of unequal division of microspores in vitro in contrast with in Vivo were as follows: (1) Phragmoplast and “phragmoplast-pla- smalemma complex” were of occurrence after nucleus division but new cell wall could not form between two daughter nuclei. (2) Generative cells were various in size, shape and amount of cytoplasmic organelles. (3) Generative cell could attach to intine at all times and underwent sporophyte division there. "Phragmoplast-plasmalemma complex" surrounding generative cell did not disappear even after generative cell detached from the intine, so that there was always an obvious demarcation line between derivative nuclei of generative and vegetative nucleus.     

The P680 Difference Spectrum Induced by Continuous Light in Malaxis monophyllos Chloroplasts

In chloroplasts from M. monophyllos (L.) Sw., the difference spectrum of light-induced P680 which was measured under physiological temperature and neutral pH and in the presence of potassium ferricyanide was obtained by steady-state method. In contrast under the same conditions, the P680 signal was not observed in spinach chloroplasts. Either preilumination with white light or long duration treatment with potassium ferricyanide caused marked similar changes in the difference spectrum of M. monophyllos chloroplasts, i.e. besides the bleaching bands at wavelength near 680 mm and 440 nm were the same as the control, the remarkable bleaching bands at about 660 nm and 422 nm appeared. These results were discussed briefly.     

On the nomenclature of Chinese drug “Cangzhu”

This paper is the documentation of specimens and literature reffered to Atractylodes lancea (Thunb.) DC. etc. As a result, it is found that, in taxonomy of the genus Atractylodes, what represcents by four long-established names, i. e. Atractylodes lancea (Thunb.) DC., A. ovata (Thunb.) DC., A. chinensis (Bunge) Koidz. and A. lyrata Sieb. et Zucc., in fact, is the one and same species. According to the law of priority in nomenclature, the first name should be given to Chinese drug “Cangzhu”, while theother three names have to be treated as its synonyms.     

Crystallization and preliminary X-ray diffraction analysis of a recombinant bacterial heme oxygenase (Hmu O) from Corynebacterium diphtheriae.

Hmu O is a 24-kDa soluble bacterial heme degradation enzyme found in the pathogen Corynebacterium diphtheriae, the causative agent of diphtheria. Similar to the mammalian heme oxygenase, it binds hemin stoichiometrically and catalyzes the oxygen-dependent conversion of hemin to biliverdin, carbon monoxide, and free iron. Iron is an essential nutrient for bacteria and especially important for pathogenesis. Here we report the first crystallization and preliminary crystallographic study of the heme-Hmu O complex formed from hemin and a recombinant Hmu O, which was expressed in Escherichia coli from a synthetic gene based on the putative hmu O gene sequence. Crystals of the heme-Hmu O complex were obtained by the sitting drop vapor diffusion method using a precipitant solution containing 18% (w/v) PEG 8000 and 0.2 M calcium acetate in 0.1 M sodium cacodylate (pH 6.5). Using synchrotron radiation, the heme-Hmu O crystal diffracted to 2.8 A resolution. It belongs to the monoclinic space group C2, with unit cell parameters a = 123.18 A, b = 44.51 A, c = 92.10 A, and beta = 123.3 degrees. Assuming one molecule of the heme-Hmu O complex per asymmetric unit, the calculated value of Vm is 2.89 A3/Da.     

Reconstitution of the glycosylphosphatidylinositol-anchored protein Thy-1: interaction with membrane phospholipids and galactosylceramide.

Glycosylphosphatidylinositol (GPI)-anchored membrane proteins are proposed to interact preferentially with glycosphingolipids and cholesterol to form microdomains, which may play an important role in apical targeting and signal transduction. The objective of the present study was to investigate the interaction of the GPI-anchored protein Thy-1 with phospholipids and a glycosphingolipid. Purified Thy-1 was reconstituted into lipid bilayer vesicles of dimyristoyl-phosphatidylcholine (DMPC) alone or in combination with galactosylceramide (GC). The ability of Thy-1 to perturb the gel to a liquid-crystalline phase transition of DMPC was examined by differential scanning calorimetry. As the mole fraction of Thy-1 increased, the phase transition enthalpy, deltaH, declined. Analysis indicated that each molecule of Thy-1 perturbed over 50 phospholipids, suggesting that, in addition to the anchor insertion into the bilayer, the protein itself may interact with the membrane surface. Inclusion of 5% w/w GC in the bilayer resulted in a striking change in the interaction of Thy-1 with phospholipids. At low Thy-1 content, there was a reduction in the phase transition temperature and an increase in phospholipid cooperativity, suggesting the formation of Thy-1/GC-enriched domains. DeltaH initially decreased with increasing Thy-1 content of the bilayer; however, at higher Thy-1 mole ratios, deltaH rose again. These results are interpreted in terms of a model whereby, at low protein:lipid mole ratios, Thy-1 preferentially sequesters GC to form enriched microdomains. At high protein:lipid mole ratios, Thy-1 may alter its conformation in response to steric crowding within these domains such that its interaction with the bilayer surface is reduced.     

Integrating the actin and vimentin cytoskeletons. adhesion-dependent formation of fimbrin-vimentin complexes in macrophages.

Cells adhere to the substratum through specialized structures that are linked to the actin cytoskeleton. Recent studies report that adhesion also involves the intermediate filament (IF) and microtubule cytoskeletons, although their mechanisms of interaction are unknown. Here we report evidence for a novel adhesion-dependent interaction between components of the actin and IF cytoskeletons. In biochemical fractionation experiments, fimbrin and vimentin coprecipitate from detergent extracts of macrophages using vimentin- or fimbrin-specific antisera. Fluorescence microscopy confirms the biochemical association. Both proteins colocalized to podosomes in the earliest stages of cell adhesion and spreading. The complex is also found in filopodia and retraction fibers. After detergent extraction, fimbrin and vimentin staining of podosomes, filopodia, and retraction fibers are lost, confirming that the complex is localized to these structures. A 1:4 stoichiometry of fimbrin binding to vimentin and a low percentage (1%) of the extracted vimentin suggest that fimbrin interacts with a vimentin subunit. A fimbrin-binding site was identified in the NH(2)-terminal domain of vimentin and the vimentin binding site at residues 143-188 in the CH1 domain of fimbrin. Based on these observations, we propose that a fimbrin-vimentin complex may be involved in directing the assembly of the vimentin cytoskeleton at cell adhesion sites.     

Extended Rank Analysis of Covariance as a More Efficient Matched Analysis Considering Trend Information

Classical matched analysis, regarded as analysis of covariance (ANOCOVA) in a broad sense, makes no attempt in modeling and may therefore be inefficient. In this paper, we discuss the relative efficiencies of the ERMP (extended rank and matched‐pair) test (Chen and Quade , 2000) to standard matched methods, and extend it to the case of multivariate covariables X . Taking advantage of trend information between the response Y and the covariables X by ranking after matching, ERMP test achieves better efficiency than a proposed class of weighted matched statistics. When Y is dichotomous, the optimal weighted matched statistic is equivalent to the Mantel‐Haenszel statistic. Example and simulation results also suggest the conclusion.     

HuR-positive stress granules: Potential targets for age-related osteoporosis

Aging impairs osteoblast function and bone turnover, resulting in age-related bone degeneration. Stress granules (SGs) are membrane-less organelles that assemble in response to stress via the recruitment of RNA-binding proteins (RBPs), and have emerged as a novel mechanism in age-related diseases. Here, we identified HuR as a bone-related RBP that aggregated into SGs and facilitated osteogenesis during aging. HuR-positive SG formation increased during osteoblast differentiation, and HuR overexpression mitigated the reduction in SG formation observed in senescent osteoblasts. Moreover, HuR positively regulated the mRNA stability and expression of its target β-catenin by binding and recruiting β-catenin into SGs. As a potential therapeutic target, HuR activator apigenin (API) enhanced its expression and thus aided osteoblasts differentiation. API treatment increased HuR nuclear export, enhanced the recruitment of β-catenin into HuR-positive SGs, facilitated β-catenin nuclear translocation, and contributed osteogenesis. Our findings highlight the roles of HuR and its SGs in promoting osteogenesis during skeletal aging and lay the groundwork for novel therapeutic strategies against age-related skeletal disorders.     

Fluorescent carbon dots synthesized by waste wind turbine blade for photocatalytic degradation

Developing novel waste recycling strategies has become a feasible solution to overcome environmental pollution. In this work, a method of using waste wind turbine blade (WTB) as a carbon source to synthesize blue fluorescent carbon dots (B-CDs) by hydrothermal treatment is proposed. B-CDs are spherical and have an average particle size of 5.2 nm. The surface is rich in C–O, C=O, −CH₃, and N–H bond functional groups, containing five elements: C, O, N, Si, and Ca. The optimal emission wavelength of B-CDs is 463 nm, corresponding to an excitation wavelength of 380 nm. Notably, a relatively high quantum yield of 29.9% and a utilization rate of 40% were obtained. In addition, B-CDs can serve as a photocatalyst to degrade methylene blue dye, with a degradation efficiency of 64% under 40-min irradiation conditions. The presence of holes has a significant influence on the degradation process.