115 research outputs found

    A chemical, mechanical, and tribological analysis of DLC coatings deposited by magnetron sputtering

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    Diamond-like carbon is one of the most studied and used solid lubricants on the market. Despite this large use and its outstanding mechanical and tribological properties, there are still some unclear aspects related to its self-lubricant properties, and some drawbacks in the deposition methods. We deposited soft DLC films on Si(100), iron, and stainless steel substrates by PVD magnetron sputtering technique with a Cr/CrN adhesive interlayer. The DLC films were characterized from a chemical, mechanical, and tribological point of view. Our aim was to connect the coating chemical and mechanical characteristics to the different conditions used for the deposition, such as discharge power and substrate-target distance. We found a stronger sp(3) dependence on the discharge power for DLC deposited closer to the target. The tribological results did not depend on the chosen substrate-target distance, but rather on the hardness of the substrate. This could be ascribed to the better mechanical coupling of soft DLC films on harder substrates

    Identification of Protein Tyrosine Phosphatase Receptor Gamma Extracellular Domain (sPTPRG) as a Natural Soluble Protein in Plasma

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    BACKGROUND:PTPRG is a widely expressed protein tyrosine phosphatase present in various isoforms. Peptides from its extracellular domain have been detected in plasma by proteomic techniques. We aim at characterizing the plasmatic PTPRG (sPTPRG) form and to identify its source.METHODOLOGY/PRINCIPAL FINDINGS:The expression of sPTPRG was evaluated in human plasma and murine plasma and tissues by immunoprecipitation and Western blotting. The polypeptides identified have an apparent Mr of about 120 kDa (major band) and 90 kDa (minor band) respectively. Full length PTPRG was identified in the 100.000 7g pelleted plasma fraction, suggesting that it was present associated to cell-derived vesicles (exosomes). The release of sPTPRG by HepG2 human hepatocellular carcinoma cell line was induced by ethanol and sensitive to metalloproteinase and not to Furin inhibitors. Finally, increased levels of the plasmatic 3c120 kDa isoform were associated with the occurrence of liver damage.CONCLUSIONS:These results demonstrate that sPTPRG represent a novel candidate protein biomarker in plasma whose increased expression is associated to hepatocyte damage. This observation could open a new avenue of investigation in this challenging field

    Toward molecular wires confined in zeolite channels for an effective transport of electronic excitation energy.

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    Sunlight is the fundamental energy source sustaining life on Earth. Green plants are provided of very sophisticated and highly efficient tools to exploit light, they are able to harvest sunlight and to transport electronic excitation energy by means of a particular “antenna system” to reaction centres (natural photosynthesis). The antenna consists of regular arrangements of chlorophyll molecules held at fixed positions by means of proteins. Light absorbed by any of these molecules is transported - by radiationless energy transfer (FRET) - to reaction centres, providing the energy necessary for the chemical processes to be initiated. A green leaf consists of millions of such well-organized antenna devices. A long-standing challenge has been the development of an artificial system able to mimic the photosynthetic system. Artificial antenna systems can be realized once several organized chromophores are able to absorb the incident light and to channel the excitation energy to a common acceptor component1-3. Artificial antenna can be built by incorporating dyes into the one-dimensional channels of zeolite L (ZL). ZL crystals feature strictly parallel nano sized channels arranged in hexagonal symmetry. These channels can be filled with high concentration of suitable guests. The geometric constraints imposed by the host structure allow achieving supramolecular organization of photoactive guests1. It has been shown2,that the properties of the dye-ZL systems depend on the molecular packing inside the channels, controlling the intermolecular and the dyes/framework interactions In this work we presents a study on the optical properties of a two –dyes antenna system in which fluorenone molecules (donor molecule) and thionine(acceptor molecule) are organized in Zeolite L porosities. To interpret the optical properties of the hybrids a detailed structural study at atomistic level was mandatory. Due to the impossibility of studying from the structural point of view a two –dyes systems, two “one-dye” hybrids (ZL/fluorenone and ZL/thionine) were firstly synthesized and characterized to investigate the intermolecular and the dyes/framework interactions4. The results of thermogravimetric, IR, and X-ray structural refinements carried out for the one-dye system ZL/FL established that 1.5 molecules per unit cell is the maximum FL loading , in contrast with the data reported previously in literature5 and that the FL carbonyl group strong interact with a K+ of the ZL. The FL distribution at maximum loading can be consider as a self-assembly of planar dye molecules into a noncovalent nanoladder. FL molecules organized in such a single, continuous nanostructure of dye molecules did not exhibit significant electronic interactions. Indeed, both absorption (recorded in the diffuse reflectance mode) and photoemission electronic spectra of ZL/FL systems with different FL loading scaled almost linearly in intensity with the amount dye hosted in the unit cell (ranging from 0.5 to 1.5), without significant changes of the spectral profiles. Noticeably, the combination and steady state and time resolved photoluminescence data indicated that even at the maximum loading ca. 90% of FL molecules are photoluminescent, with significant increase in the average quantum yield with respect to FL molecules in solution. Such a finding clearly indicates that excited states coupling (Davydov splitting) is not contributing to the optical properties of the material. The structural study of the ZL/TH system revealed that the maximum possible loading of TH is equal to 0.3 molecules per unit cell in agreement with the TGA and literature data6. Short distances between the carbon, sulfur and nitrogen atoms and two water molecule sites , in turn at bond distance from the oxygen atoms of the main channel, suggested a water-mediated Th-ZL interactions7. Moreover, IR spectroscopy provided evidence of the interaction of the aromatic rings with the environment. This likely resulted in an increase of the rate of non-radiative decay of Th molecules in the electronic excited state, because only ca. 5% of Th molecules hosted in the ZL channel appeared photoluminescent. The occurrence of energy transfer from excited FL molecules forming the noncovalent nanoladder in the ZL channels and Th, in the ground state, deposited on the external surface of ZL particles are currently under investigation. In conclusion, we have here presented a study on the physico-chemical properties of dense molecular wires encapsulated in the one-dimensional pores arrays of Zeolite L. Concerning the optical properties of our composites, no evidence of Davydov splitting emerged from our study, indicating that one of the main competitors of the FRET mechanism is not operative notwithstanding the close packed arrangement of FL. We believe that this feature is of overwhelming relevance in view of application of such a system in artificial antenna systems

    Molecular wires confined in zeolite L channels for an effective transport of electronic excitation energy: a synchrotron structural study.

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    Sunlight is the fundamental energy source sustaining life on Earth. Green plants are provided of very sophisticated and highly efficient tools to exploit light, they are able to harvest sunlight and to transport electronic excitation energy by means of a particular \u201cantenna system\u201d to reaction centers (natural photosynthesis).The development of an artificial system able to mimic the natural phenomenon has been a long-standing challenge. Artificial antenna systems can be realized once several organized chromophores are able to absorb the incident light and to channel the excitation energy to a common acceptor component [1-3]. The optical properties of the systems depend on the molecular packing inside the channels. Artificial antenna can be built by incorporating suitable guests into the one-dimensional channels of zeolite L (ZL). In this work we present a detailed structural study of two hybrid systems in which dyes (fluorenone and thionine) are encapsulated in zeolite L channels. These two molecules were chosen since it has been demonstrated that a \u201ctwo \u2013dyes antenna system\u201d - in which fluorenone (FL) (donor molecule) and thionine (Th) (acceptor molecule) are organized in Zeolite L porosities - shows remarkable optical properties. Due to the impossibility of studying, from the structural point of view a \u201ctwo \u2013dyes systems\u201d, two \u201cone-dye\u201d hybrids (ZL/fluorenone and ZL/thionine) were firstly synthesized and characterized [4]. The results of thermogravimetric, IR, and X-ray structural refinements carried out for the one-dye ZL/FL and ZL/Th systems established that 1.5 molecules of FL and 0.3 molecules of Th per unit cell is the maximum loading, respectively. The FL carbonyl group strong interacts with a K+ of the ZL. On the other hand, short distances between the carbon, sulfur and nitrogen atoms of Th and two water molecule sites, in turn at bond distance from the oxygen atoms of the main channel, suggested a water-mediated Th-ZL interactions. The energy transfer from excited FL molecules, forming the non-covalent nano-ladder in the ZL channel, and Th, deposited on the external surface of ZL particles, is currently under investigation. In conclusion concerning the optical properties of our composites, no evidence of Davydov splitting emerged from our study, indicating that one of the main competitors of the FRET mechanism is not operative notwithstanding the close packed arrangement of FL. We believe that this feature is of overwhelming relevance in view of application of such a system in artificial antenna devices. The authors acknowledge the Italian Ministry of Education, MIUR-Project: \u201cFuturo in Ricerca 2012 - ImPACT- RBFR12CLQD\u201d

    Distribution of different isoforms of receptor protein tyrosine phosphatase \u3b3 (Ptprg-RPTP \u3b3) in adult mouse brain: upregulation during neuroinflammation.

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    The receptor protein tyrosine phosphatase \u3b3 (Ptprg-RPTP\u3b3) is a receptor protein widely expressed in many tissues, including the central nervous system (CNS). Several RPTP\u3b3 isoforms are expressed in the brain during development and in adulthood, but their distribution and role are unknown. In this study, we investigated the distribution of some RPTP\u3b3 isoforms in the adult brain using antibodies against the epitopes localized in the C- and in the N-terminal domains of the full length isoform of RPTP\u3b3. We found a predominant and widespread neuronal positivity throughout the neocortex, hippocampus, striatum and in many nuclei of the brainstem and cerebellum. At least 2 distinct isoforms that can co-exist in various compartments in the same cell are detectable in different neuron types. Immunopositivity for epitopes located in both the N- and C-terminus domains were found in the neuropil of cortical and hippocampal neurons, whereas the N-terminal domain positivity was found in the soma, often without colocalization with its C-terminal counterpart. Among glial cells, some protoplasmic and perivascular astrocytes and the cerebellar Bergmann glia, express RPTP\u3b3. The astrocytic expression of RPTP\u3b3 and putative processing isoforms of 120 and 80 kDa increases during neuroinflammation, in particular 24 h after LPS treatment. Activated astrocytes were found to be strongly positive for RPTP\u3b3 also in a mice model of Alzheimer's disease. Our results confirm previous findings and enrich the current knowledge of RPTP\u3b3 distribution in the CNS, highlighting a role of RPTP\u3b3 during neuroinflammation processes

    Dye Loading influence on performances of Fluorenone/zeoliteL Light Harvester

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    Zeolite L (LTL), is an appealing and excellent host for the supramolecular organization of different kinds of molecules and complexes. However, relatively few experimental structural information is available about the orientation and alignment of the dye molecules in the zeolite pores. Hence, a detailed structural characterization is of great importance for understanding the functionality of these host-guest systems. Between all the possible guests, neutral dye fluorenone (C13H8O) (FL) has received a considerable attention [1,2] because of its ability to form a host-guest complex with LTL, stable if exposed at the atmosphere. Moreover, the fluorescent nature of fluorenone makes this complex interesting as a component of the energy relay system in artificial antennas. Although a detailed structural characterization is still lacking, theoretical studies have shown as the orientation of fluorenone is especially interesting as it is directly related to the light harvesting properties of fluorenone [3]. Moreover, it has shown as the presence of water can influence on the electronic spectra of this host-guest complex and then affect its performances as light harvester [3]. In this study, three different FL/K-LTL materials characterized by an increasing loading of FL have been synthesized by mixing in inert atmosphere the dehydrated K-LTL and FL powder in ratio of 0.5, 1.0, 1.5 and 2.0 molecules/unit cell, and then heating the samples at 120°C in air for 24 h. The vials were maintained under continuous rotation during the heating in order to optimize the contact between the zeolite and the dye. The samples so obtained were characterized by means of X-ray powder diffraction, thermo-gravimetric analysis, IR and UV-vis spectroscopies, fluorescence and nitrogen adsorption. The incorporation of FL into the K-LTL channels was confirmed by a significant change of the unit cell parameters and by drastic decrease in the K-LTL surface area also at low FL loading. The strong interaction between FL carbonyl group and the extraframework potassium cation predicted by theoretical modelling [1] was confirmed by the short bond distances (2.77 Å), evidenced in the Rietveld refined structure, and by the shift of the C=O stretching frequency evidenced in the IR spectra. Such an interaction explains why FL is not displaced by water molecules when FL/K-LTL hybrid is re-exposed to the air [1]. Interestingly, although the UV-vis absorption spectrum was almost unaffected by the FL loading, the corresponding emission spectrum evidenced a strong influence: the optimum FL/K-LTL ratio was then determined in order to optimize the performances of the device as light harvester. The structural information obtained theoretically and from XRD allowed also to explain the loading dependence of the optical properties of the material and to correlate it with the relative orientation of the fluorenone molecules in the zeolite channels

    Rapid recognition of drug-resistance/sensitivity in leukemic cells by Fourier transform infrared microspectroscopy and unsupervised hierarchical cluster analysis.

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    We tested the ability of Fourier Transform (FT) InfraRed (IR) microspectroscopy (microFTIR) in combination with unsupervised Hierarchical Cluster Analysis (HCA) in identifying drug-resistance/sensitivity in leukemic cells exposed to tyrosine kinase inhibitors (TKIs). Experiments were carried out in a well-established mouse model of human Chronic Myelogenous Leukemia (CML). Mouse-derived pro-B Ba/F3 cells transfected with and stably expressing the human p210(BCR-ABL) drug-sensitive wild-type BCR-ABL or the V299L or T315I p210(BCR-ABL) drug-resistant BCR-ABL mutants were exposed to imatinib-mesylate (IMA) or dasatinib (DAS). MicroFTIR was carried out at the Diamond IR beamline MIRIAM where the mid-IR absorbance spectra of individual Ba/F3 cells were acquired using the high brilliance IR synchrotron radiation (SR) via aperture of 15 7 15 \u3bcm(2) in sizes. A conventional IR source (globar) was used to compare average spectra over 15 cells or more. IR signatures of drug actions were identified by supervised analyses in the spectra of TKI-sensitive cells. Unsupervised HCA applied to selected intervals of wavenumber allowed us to classify the IR patterns of viable (drug-resistant) and apoptotic (drug-sensitive) cells with an accuracy of >95%. The results from microFTIR + HCA analysis were cross-validated with those obtained via immunochemical methods, i.e. immunoblotting and flow cytometry (FC) that resulted directly and significantly correlated. We conclude that this combined microFTIR + HCA method potentially represents a rapid, convenient and robust screening approach to study the impact of drugs in leukemic cells as well as in peripheral blasts from patients in clinical trials with new anti-leukemic drugs

    Defective CFTR Expression and Function Are Detectable in Blood Monocytes: Development of a New Blood Test for Cystic Fibrosis

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    BACKGROUND: Evaluation of cystic fibrosis transmembrane conductance regulator (CFTR) functional activity to assess new therapies and define diagnosis of cystic fibrosis (CF) is cumbersome. It is known that leukocytes express detectable levels of CFTR but the molecule has not been characterized in these cells. In this study we aim at setting up and validating a blood test to evaluate CFTR expression and function in leukocytes. DESCRIPTION: Western blot, PCR, immunofluorescence and cell membrane depolarization analysis by single-cell fluorescence imaging, using the potential-sensitive DiSBAC(2)(3) probe were utilized. Expression of PKA phosphorylated, cell membrane-localized CFTR was detected in non-CF monocytes, being undetectable or present in truncated form in monocytes derived from CF patients presenting with nonsense mutations. CFTR agonist administration induced membrane depolarization in monocytes isolated from non-CF donors (31 subjects) and, to a lesser extent, obligate CFTR heterozygous carriers (HTZ: 15 subjects), but it failed in monocytes from CF patients (44 subjects). We propose an index, which values in CF patients are significantly (p<0.001) lower than in the other two groups. Nasal Potential Difference, measured in selected subjects had concordant results with monocytes assay (Kappa statistic 0.93, 95%CI: 0.80-1.00). RESULTS AND SIGNIFICANCE: CFTR is detectable and is functional in human monocytes. We also showed that CFTR-associated activity can be evaluated in 5 ml of peripheral blood and devise an index potentially applicable for diagnostic purposes and both basic and translational research: from drug development to evaluation of functional outcomes in clinical trials
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