Braiding Interactions in Anyonic Quantum Walks

The anyonic quantum walk is a dynamical model describing a single anyon propagating along a chain of stationary anyons and interacting via mutual braiding statistics. We review the recent results on the effects of braiding statistics in anyonic quantum walks in quasi-one dimensional ladder geometries. For anyons which correspond to spin-1/2 irreps of the quantum groups $SU(2)_k$, the non-Abelian species $(1<k<\infty)$ gives rise to entanglement between the walker and topological degrees of freedom which is quantified by quantum link invariants over the trajectories of the walk. The decoherence is strong enough to reduce the walk on the infinite ladder to classical like behaviour. We also present numerical results on mixing times of $SU(2)_2$ or Ising model anyon walks on cyclic graphs. Finally, the possible experimental simulation of the anyonic quantum walk in Fractional Quantum Hall systems is discussed.Comment: 13 pages, submitted to Proceedings of the 2nd International Conference on Theoretical Physics (ICTP 2012

Transport properties of anyons in random topological environments

The quasi one-dimensional transport of Abelian and non-Abelian anyons is studied in the presence of a random topological background. In particular, we consider the quantum walk of an anyon that braids around islands of randomly filled static anyons of the same type. Two distinct behaviours are identified. We analytically demonstrate that all types of Abelian anyons localise purely due to the statistical phases induced by their random anyonic environment. In contrast, we numerically show that non-Abelian Ising anyons do not localise. This is due to their entanglement with the anyonic environment that effectively induces dephasing. Our study demonstrates that localisation properties strongly depend on non-local topological interactions and it provides a clear distinction in the transport properties of Abelian and non-Abelian statistics.Comment: 9 pages, 5 figure

Statistical dynamics of a non-Abelian anyonic quantum walk

We study the single particle dynamics of a mobile non-Abelian anyon hopping around many pinned anyons on a surface. The dynamics is modelled by a discrete time quantum walk and the spatial degree of freedom of the mobile anyon becomes entangled with the fusion degrees of freedom of the collective system. Each quantum trajectory makes a closed braid on the world lines of the particles establishing a direct connection between statistical dynamics and quantum link invariants. We find that asymptotically a mobile Ising anyon becomes so entangled with its environment that its statistical dynamics reduces to a classical random walk with linear dispersion in contrast to particles with Abelian statistics which have quadratic dispersion.Comment: 7 pages, 5 figure

Gene transfer into hepatocytes using asialoglycoprotein receptor mediated endocytosis of DNA complexed with an artificial tetra-antennary galactose ligand

We have constructed an artificial ligand for the hepatocyte-specific asialoglycoprotein receptor for the purpose of generating a synthetic delivery system for DNA. This ligand has a tetra-antennary structure, containing four terminal galactose residues on a branched carrier peptide. The carbohydrate residues of this glycopeptide were introduced by reductive coupling of lactose to the alpha- and epsilon-amino groups of the two N-terminal lysines on the carrier peptide. The C-terminus of the peptide, containing a cysteine separated from the branched N-terminus by a 10 amino acid spacer sequence, was used for conjugation to 3-(2-pyridyldithio)propionate-modified polylysine via disulfide bond formation. Complexes containing plasmid DNA bound to these galactose-polylysine conjugates have been used for asialoglycoprotein receptor-mediated transfer of a luciferase gene into human (HepG2) and murine (BNL CL.2) hepatocyte cell lines. Gene transfer was strongly promoted when amphipathic peptides with pH-controlled membrane-disruption activity, derived from the N-terminal sequence of influenza virus hemagglutinin HA-2, were also present in these DNA complexes. Thus, we have essentially borrowed the small functional domains of two large proteins, asialoglycoprotein and hemagglutinin, and assembled them into a supramolecular complex to generate an efficient gene-transfer system

Influence of molecular weight, temperature, and extensional rheology on melt blowing process stability for linear isotactic polypropylene

In this work, three linear isotactic polypropylenes with different weight-average molecular weights, M-w, and comparable polydispersities were used to produce nonwovens by melt blowing technology at two different temperatures, T. The air/polymer flow rate was changed to maintain the same average fiber diameter, resulting in a different broadness of fiber diameter distribution, which was quantified by the coefficient of variation, CV. The elasticity of the material was evaluated by the reptation-mode relaxation time, lambda(1), and the Rouse-mode reorientation time, lambda(2), determined from the deformation rate dependent shear viscosity data. Extensional rheology was evaluated using uniaxial extensional viscosity measured over a very wide range of strain rates (2 x 10(4) s(-1)-2 x 10(6) s(-1)) using entrance pressure drop and Gibson methods. An obtained plateau value of uniaxial extensional viscosity at the highest extensional strain rates, eta(E,infinity) (normalized by the three times zero-shear rate viscosity, eta(0)), and the minimum uniaxial extensional viscosity, eta(E,min), were related to M-w and T using simple equations. It has been found that the stability of fiber production captured by CV depends exclusively on the extensional properties of the polypropylene melts, namely, eta(E,U,)infinity/3 eta(0) and eta(E,U,min). These findings are important especially with regard to the stable production of polymeric nanofibers by melt blowing technology

Coupling of adenovirus to transferrin-polylysine/DNA complexes greatly enhances receptor-mediated gene delivery and expression of transfected genes.

We are developing efficient methods for gene transfer into tissue culture cells. We have previously shown that coupling of a chimeric adenovirus with polylysine allowed the construction of an adenovirus-polylysine-reporter-gene complex that transferred the transporter gene with great efficiency into HeLa cells. We have now explored simpler, biochemical means for coupling adenovirus to DNA/polylysine complexes and show that such complexes yield virtually 100% transfection in tissue culture cell lines. In these methods adenovirus is coupled to polylysine, either enzymatically through the action of transglutaminase or biochemically by biotinylating adenovirus and streptavidinylating the polylysine moiety. Combination complexes containing DNA, adenovirus-polylysine, and transferrin-polylysine have the capacity to transfer the reporter gene into adenovirus-receptor- and/or transferrin-receptor-rich cells

Spectral Energy Distributions of Type 1 AGN in the COSMOS Survey I - The XMM-COSMOS Sample

The "Cosmic Evolution Survey" (COSMOS) enables the study of the Spectral Energy Distributions (SEDs) of Active Galactic Nuclei (AGN) because of the deep coverage and rich sampling of frequencies from X-ray to radio. Here we present a SED catalog of 413 X-ray (\xmm) selected type 1 (emission line FWHM$>2000$ km s$^{-1}$) AGN with Magellan, SDSS or VLT spectrum. The SEDs are corrected for the Galactic extinction, for broad emission line contributions, constrained variability, and for host galaxy contribution. We present the mean SED and the dispersion SEDs after the above corrections in the rest frame 1.4 GHz to 40 keV, and show examples of the variety of SEDs encountered. In the near-infrared to optical (rest frame $\sim 8\mu m$-- 4000\AA), the photometry is complete for the whole sample and the mean SED is derived from detections only. Reddening and host galaxy contamination could account for a large fraction of the observed SED variety. The SEDs are all available on-line.Comment: 22 pages, 22 figures, ApJ accepted, scheduled to be published October 20th, 2012, v75

Histological assessment of paxgene tissue fixation and stabilization reagents

Within SPIDIA, an EC FP7 project aimed to improve pre analytic procedures, the PAXgene Tissue System (PAXgene), was designed to improve tissue quality for parallel molecular and morphological analysis. Within the SPIDIA project promising results were found in both genomic and proteomic experiments with PAXgene-fixed and paraffin embedded tissue derived biomolecules. But, for this technology to be accepted for use in both clinical and basic research, it is essential that its adequacy for preserving morphology and antigenicity is validated relative to formalin fixation. It is our aim to assess the suitability of PAXgene tissue fixation for (immuno)histological methods. Normal human tissue specimens (n = 70) were collected and divided into equal parts for fixation either with formalin or PAXgene. Sections of the obtained paraffin-embedded tissue were cut and stained. Morphological aspects of PAXgene-fixed tissue were described and also scored relative to formalin-fixed tissue. Performance of PAXgene-fixed tissue in immunohistochemical and in situ hybridization assays was also assessed relative to the corresponding formalin-fixed tissues. Morphology of PAXgene-fixed paraffin embedded tissue was well preserved and deemed adequate for diagnostics in most cases. Some antigens in PAXgene-fixed and paraffin embedded sections were detectable without the need for antigen retrieval, while others were detected using standard, formalin fixation based, immunohistochemistry protocols. Comparable results were obtained with in situ hybridization and histochemical stains. Basically all assessed histological techniques were found to be applicable to PAXgene-fixed and paraffin embedded tissue. In general results obtained with PAXgene-fixed tissue are comparable to those of formalin-fixed tissue. Compromises made in morphology can be called minor compared to the advantages in the molecular pathology possibilities

High-Level Expression of Various Apolipoprotein (a) Isoforms by "Transferrinfection". The Role of Kringle IV Sequences in the Extracellular Association with Low-Density Lipoprotein

Characterization of the assembly of lipoprotein(a) [Lp(a)] is of fundamental importance to understanding the biosynthesis and metabolism of this atherogenic lipoprotein. Since no established cell lines exist that express Lp(a) or apolipoprotein(a) [apo(a)], a "transferrinfection" system for apo(a) was developed utilizing adenovirus receptor- and transferrin receptor-mediated DNA uptake into cells. Using this method, different apo(a) cDNA constructions of variable length, due to the presence of 3, 5, 7, 9, 15, or 18 internal kringle IV sequences, were expressed in cos-7 cells or CHO cells. All constructions contained kringle IV-36, which includes the only unpaired cysteine residue (Cys-4057) in apo(a). r-Apo(a) was synthesized as a precursor and secreted as mature apolipoprotein into the medium. When medium containing r-apo(a) with 9, 15, or 18 kringle IV repeats was mixed with normal human plasma LDL, stable complexes formed that had a bouyant density typical of Lp(a). Association was substantially decreased if Cys-4057 on r-apo(a) was replaced by Arg by site-directed mutagenesis or if Cys-4057 was chemically modified. Lack of association was also observed with r-apo(a) containing only 3, 5, or 7 kringle IV repeats without "unique kringle IV sequences", although Cys-4057 was present in all of these constructions. Synthesis and secretion of r-apo(a) was not dependent on its sialic acid content. r-Apo(a) was expressed even more efficiently in sialylation-defective CHO cells than in wild-type CHO cells. In transfected CHO cells defective in the addition of N-acetylglucosamine, apo(a) secretion was found to be decreased by 50%. Extracellular association with LDL was not affected by the carbohydrate moiety of r-apo(a), indicating a protein-protein interaction between r-apo(a) and apoB. These results show that, besides kringle IV-36, other kringle IV sequences are necessary for the extracellular association of r-apo(a) with LDL. Changes in the carbohydrate moiety of apo(a), however, do not affect complex formation

Intermediate filament cytoskeleton of the liver in health and disease

Intermediate filaments (IFs) represent the largest cytoskeletal gene family comprising ~70 genes expressed in tissue specific manner. In addition to scaffolding function, they form complex signaling platforms and interact with various kinases, adaptor, and apoptotic proteins. IFs are established cytoprotectants and IF variants are associated with >30 human diseases. Furthermore, IF-containing inclusion bodies are characteristic features of several neurodegenerative, muscular, and other disorders. Acidic (type I) and basic keratins (type II) build obligatory type I and type II heteropolymers and are expressed in epithelial cells. Adult hepatocytes contain K8 and K18 as their only cytoplasmic IF pair, whereas cholangiocytes express K7 and K19 in addition. K8/K18-deficient animals exhibit a marked susceptibility to various toxic agents and Fas-induced apoptosis. In humans, K8/K18 variants predispose to development of end-stage liver disease and acute liver failure (ALF). K8/K18 variants also associate with development of liver fibrosis in patients with chronic hepatitis C. Mallory-Denk bodies (MDBs) are protein aggregates consisting of ubiquitinated K8/K18, chaperones and sequestosome1/p62 (p62) as their major constituents. MDBs are found in various liver diseases including alcoholic and non-alcoholic steatohepatitis and can be formed in mice by feeding hepatotoxic substances griseofulvin and 3,5-diethoxycarbonyl-1,4-dihydrocollidine (DDC). MDBs also arise in cell culture after transfection with K8/K18, ubiquitin, and p62. Major factors that determine MDB formation in vivo are the type of stress (with oxidative stress as a major player), the extent of stress-induced protein misfolding and resulting chaperone, proteasome and autophagy overload, keratin 8 excess, transglutaminase activation with transamidation of keratin 8 and p62 upregulation