Carbon Nanotubes Synthesized in Channels of Alpo4-5 Single Crystals : First X-Ray Scattering Investigations

Following the synthesis of aligned single-wall carbon nanotubes in the channels of AlPO4-5 zeolite single crystals, we present the first X-ray diffraction and diffuse scattering results. They can be analysed in terms of a partial filling of the zeolite channels by nanotubes with diameter around 4A. The possible selection of only one type of nanotube during the synthesis, due to the constraints imposed by the zeolite host, is discussed.Comment: to appear in Solid State Com

Host-derived viral transporter protein for nitrogen uptake in infected marine phytoplankton

This is the author's accepted manuscriptFinal version available from NAS via the DOI in this recordPhytoplankton community structure is shaped by both bottom–up factors, such as nutrient availability, and top–down processes, such as predation. Here we show that marine viruses can blur these distinctions, being able to amend how host cells acquire nutrients from their environment while also predating and lysing their algal hosts. Viral genomes often encode genes derived from their host. These genes may allow the virus to manipulate host metabolism to improve viral fitness. We identify in the genome of a phytoplankton virus, which infects the small green alga Ostreococcus tauri, a host-derived ammonium transporter. This gene is transcribed during infection and when expressed in yeast mutants the viral protein is located to the plasma membrane and rescues growth when cultured with ammonium as the sole nitrogen source. We also show that viral infection alters the nature of nitrogen compound uptake of host cells, by both increasing substrate affinity and allowing the host to access diverse nitrogen sources. This is important because the availability of nitrogen often limits phytoplankton growth. Collectively, these data show that a virus can acquire genes encoding nutrient transporters from a host genome and that expression of the viral gene can alter the nutrient uptake behavior of host cells. These results have implications for understanding how viruses manipulate the physiology and ecology of phytoplankton, influence marine nutrient cycles, and act as vectors for horizontal gene transfer.A.M. and T.A.R. are funded by the Royal Society, through Newton and University Research fellowships, respectively. This work is supported in part by research grants from The Gordon and Betty Moore Foundation (GBMF5514), Leverhulme Trust (PLP-2014-147), and the University of Exeter. The University of Exeter OmniLog facility is supported by a Wellcome Trust Institutional Strategic Support Award WT105618MA. Phylogenetic reconstructions were computed on the Data Intensive Academic Grid (National Science Foundation, MRI-R2 Project DBI-0959894)

Raman spectroscopy on carbon nanotubes at high pressure

Raman spectroscopy has been the most extensively employed method to study carbon nanotubes at high pressures. This review covers reversible pressure-induced changes of the lattice dynamics and structure of single- and multi-wall carbon nanotubes as well as irreversible transformations induced by high pressures. The interplay of covalent and van-der-Waals bonding in single-wall nanotube bundles and a structural distortion near 2 GPa are discussed in detail. Attempts of transforming carbon nanotubes into diamond and other "superhard" phases are reviewed critically.Comment: 33 pages, 20 figures, review article, to appear in J. Raman Spectroscop

Contemporaneous cell spreading and phagocytosis: Magneto-resistive real-time monitoring of membrane competing processes

Shoshi A, Schotter J, Schroeder P, et al. Contemporaneous cell spreading and phagocytosis: Magneto-resistive real-time monitoring of membrane competing processes. Biosensors And Bioelectronics. 2013;40(1):82-88.Adhesion and spreading of cells strongly depend on the properties of the underlying surface, which has significant consequences in long-term cell behavior adaption. This relationship is important for the understanding of both biological functions and their bioactivity in disease-related applications. Employing our magnetic lab-on-a-chip system, we present magnetoresistive-based real-time and label-free detection of cellular phagocytosis behavior during their spreading process on particle-immobilized sensor surfaces. Cell spreading experiments carried out on particle-free and particle-modified surfaces reveal a delay in spreading rate after an elapsed time of about 2.2 h for particle-modified surfaces due to contemporaneous cell membrane loss by particle phagocytosis. Our associated magnetoresistive measurements show a high uptake rate at early stages of cell spreading, which decreases steadily until it reaches saturation after an average elapsed time of about 100 min. The corresponding cellular average uptake rate during the entire cell spreading process accounts for three particles per minute. This result represents a four times higher phagocytosis efficiency compared to uptake experiments carried out for confluently grown cells, in which case cell spreading is already finished and, thus, excluded. Furthermore, other dynamic cell-surface interactions at nano-scale level such as cell migration or the dynamics of cell attachment and detachment are also addressable by our magnetic lab-on-a-chip approach. (C) 2012 Elsevier B.V. All rights reserved

Magnetoresistive-based real-time cell phagocytosis monitoring

Shoshi A, Schotter J, Schroeder P, et al. Magnetoresistive-based real-time cell phagocytosis monitoring. Biosensors and Bioelectronics. 2012;36(1):116-122.The uptake of large particles by cells (phagocytosis) is an important factor in cell biology and also plays a major role in biomedical applications. So far, most methods for determining the phagocytic properties rely on cell-culture incubation and end-point detection schemes. Here, we present a lab-on-a-chip system for real-time monitoring of magnetic particle uptake by human fibroblast (NHDF) cells. It is based on recording the time evolution of the average position and distribution of magnetic particles during phagocytosis by giant-magnetoresistive (GMR) type sensors. We employ particles with a mean diameter of 1.2 mu m and characterize their phagocytosis-relevant properties. Our experiments at physiological conditions reveal a cellular uptake rate of 45 particles per hour and show that phagocytosis reaches saturation after an average uptake time of 27.7 h. Moreover, reference phagocytosis experiments at 4 degrees C are carried out to mimic environmental or disease related inhibition of the phagocytic behavior, and our measurements clearly show that we are able to distinguish between cell-membrane adherent and phagocytosed magnetic particles. Besides the demonstrated real-time monitoring of phagocytosis mechanisms, additional nano-biointerface studies can be realized, including on-chip cell adhesion/spreading as well as cell migration, attachment and detachment dynamics. This versatility shows the potential of our approach for providing a multifunctional platform for on-chip cell analysis. (C) 2012 Elsevier B.V. All rights reserved