Synthesis and magnetic properties of CoPt nanoparticles

High magnetocrystalline anisotropy CoPt particles with an average size of 8 nm were synthesized by the superhydride reduction of CoCl2CoCl2 and Pt(acac)2Pt(acac)2 at a high temperature. As-made particles showed a disordered face-centered cubic lattice and were superparamagnetic. Upon heat treatment at temperatures above 600 °C, the particles transformed to the L10L10 phase, as indicated by the appearance of the superlattice peaks in the x-ray diffraction and high magnetocrystalline anisotropy. The temperature dependence of the coercivity of nanoparticles annealed at 650 °C was measured from 10 to 300 K and analyzed using a Sharrock formula. After annealing at 650 °C, the anisotropy of the nanoparticles was K∼1.7×107 erg/cm3.K∼1.7×107 erg/cm3. © 2004 American Institute of Physics.Peer Reviewedhttp://deepblue.lib.umich.edu/bitstream/2027.42/69714/2/JAPIAU-95-11-6747-1.pd

Self-assembly of magnetic biofunctional nanoparticles

Spherical, ferromagnetic FePt nanoparticles with a particle size of 3 nm were prepared by the simultaneous polyol reduction of Fe(acac)3Fe(acac)3 and Pt(acac)2Pt(acac)2 in phenyl ether in the presence of oleic acid and oleylamine. The oleic acid ligands can be replaced with 11-mercaptoundecanoic acid, giving particles that can be dispersed in water. Both x-ray diffraction and transmission electron microscopy indicated that FePt particles were not affected by ligands replacement. Dispersions of the FePt particles with 11-mercaptoundecanoic acid ligands and ammonium counter ions gave self-assembled films consisting of highly ordered hexagonal arrays of particles.Peer Reviewedhttp://deepblue.lib.umich.edu/bitstream/2027.42/87511/2/10Q901_1.pd

Dendritic Cell-Mediated-Immunization with Xenogenic PrP and Adenoviral Vectors Breaks Tolerance and Prolongs Mice Survival against Experimental Scrapie

In prion diseases, PrPc, a widely expressed protein, is transformed into a pathogenic form called PrPSc, which is in itself infectious. Antibodies directed against PrPc have been shown to inhibit PrPc to PrPSc conversion in vitro and protect in vivo from disease. Other effectors with potential to eliminate PrPSc-producing cells are cytotoxic T cells directed against PrP-derived peptides but their ability to protect or to induce deleterious autoimmune reactions is not known. The natural tolerance to PrPc makes difficult to raise efficient adaptive responses. To break tolerance, adenovirus (Ad) encoding human PrP (hPrP) or control Ad were administered to wild-type mice by direct injection or by transfer of Ad-transduced dendritic cells (DCs). Control Ad-transduced DCs from Tg650 mice overexpressing hPrP were also used for immunization. DC-mediated but not direct administration of AdhPrP elicited antibodies that bound to murine native PrPc. Frequencies of PrP-specific IFNγ-secreting T cells were low and in vivo lytic activity only targeted cells strongly expressing hPrP. Immunohistochemical analysis revealed that CD3+ T cell infiltration was similar in the brain of vaccinated and unvaccinated 139A-infected mice suggesting the absence of autoimmune reactions. Early splenic PrPSc replication was strongly inhibited ten weeks post infection and mean survival time prolonged from 209 days in untreated 139A-infected mice to 246 days in mice vaccinated with DCs expressing the hPrP. The efficacy appeared to be associated with antibody but not with cytotoxic cell-mediated PrP-specific responses

The IDENTIFY study: the investigation and detection of urological neoplasia in patients referred with suspected urinary tract cancer - a multicentre observational study

Objective To evaluate the contemporary prevalence of urinary tract cancer (bladder cancer, upper tract urothelial cancer [UTUC] and renal cancer) in patients referred to secondary care with haematuria, adjusted for established patient risk markers and geographical variation. Patients and Methods This was an international multicentre prospective observational study. We included patients aged ≥16 years, referred to secondary care with suspected urinary tract cancer. Patients with a known or previous urological malignancy were excluded. We estimated the prevalence of bladder cancer, UTUC, renal cancer and prostate cancer; stratified by age, type of haematuria, sex, and smoking. We used a multivariable mixed-effects logistic regression to adjust cancer prevalence for age, type of haematuria, sex, smoking, hospitals, and countries. Results Of the 11 059 patients assessed for eligibility, 10 896 were included from 110 hospitals across 26 countries. The overall adjusted cancer prevalence (n = 2257) was 28.2% (95% confidence interval [CI] 22.3–34.1), bladder cancer (n = 1951) 24.7% (95% CI 19.1–30.2), UTUC (n = 128) 1.14% (95% CI 0.77–1.52), renal cancer (n = 107) 1.05% (95% CI 0.80–1.29), and prostate cancer (n = 124) 1.75% (95% CI 1.32–2.18). The odds ratios for patient risk markers in the model for all cancers were: age 1.04 (95% CI 1.03–1.05; P < 0.001), visible haematuria 3.47 (95% CI 2.90–4.15; P < 0.001), male sex 1.30 (95% CI 1.14–1.50; P < 0.001), and smoking 2.70 (95% CI 2.30–3.18; P < 0.001). Conclusions A better understanding of cancer prevalence across an international population is required to inform clinical guidelines. We are the first to report urinary tract cancer prevalence across an international population in patients referred to secondary care, adjusted for patient risk markers and geographical variation. Bladder cancer was the most prevalent disease. Visible haematuria was the strongest predictor for urinary tract cancer

In vitro propagation of Araucaria cunninghamii and other species of the araucariaceae via axillary meristems

Stem segments with 3-5 leaf axils, excised from the upper portion of the mainstem of 2-year-old hoop pine (Araucaria cunninghamii Aiton ex D. Don) seedlings, produced orthotropic buds from the concealed axillary meristems when cultured on a basal medium (BM) of half-strength Murashige and Skoog (MS) inorganic salts, the medium level of growth factors and amino acids of de Fossard, 20 g L sucrose and 6.5 g/L agar. This procedure was also successful with A. balansae, A. bidwillii, A. colurnnaris, A. hunsteinri, A. luxurians, A. montana, A. rulei, A. scopulorum and Agathis robusta and with stem segments from orthotropic coppice shoots of juvenile morphology collected from the stumps of 20-year old hoop pines felled near ground level. The hoop pine explants were highly sensitive to cytokinin; 1 µM and 10 µM 6-benzylaminopurine caused the formation of distorted buds and total inhibition of bud development respectively. Lofier concentrations (0.001-0.1 µM) did not noticeably influence bud formation or development. A low rate of multiplication was induced by reculturing the stem segments after the excision of the initial shoots. New buds developed in the leaf axils of that part of the initial shoot which remained attached to the primary stem explant. Shoots derived from seedling and coppice cultures of hoop pine and seedling cultures of Agathis robusta rooted in vitro on BM + 0.1-10.0 µM indole-3-butyric acid (IBA), but with only 5-20% success. Up to 80% rooting was obtained if both hoop pine shoot types (i. e. from seedling and coppice cultures) were cultured on modified BM (quarter strength MS salts, 10 µM IBA plus no agar) for 2 weeks, before being transferred to a mixture of non-sterile peat and perlite or vermiculite and perlite, maintained under a high humidity (90-95%). Plantlets were subsequently transferred to normal glasshouse conditions and then to the field with less than 5% mortality. Thus hoop pine can be added to the relatively small number of conifers for which the capacity to micropropagate juvenile and mature plants and successfully establish their clones in the field has been demonstrated