37 research outputs found
Photovoltaic LiNbO3particles: Applications to Biomedicine/Biophotonics
Recently, a novel method to trap and pattern ensembles of nanoparticles has been proposed and
tested. It relies on the photovoltaic (PV) properties of certain ferroelectric crystals such as LiNbO3 [1,2].
These crystals, when suitably doped, develop very high electric fields in response to illumination with
light of suitable wavelength. The PV effect lies in the asymmetrical excitation of electrons giving rise to
PV currents and associated space-charge fields (photorefractive effect). The field generated in the bulk
of the sample propagates to the surrounding medium as evanescent fields. When dielectric or metal
nanoparticles are deposited on the surface of the sample the evanescent fields give rise to either
electrophoretic or dielectrophoretic forces, depending on the charge state of the particles, that induce
the trapping and patterning effects [3,4].
The purpose of this work has been to explore the effects of such PV fields in the biology and
biomedical areas. A first work was able to show the necrotic effects induced by such fields on He-La
tumour cells grown on the surface of an illuminated iron-doped LiNbO3 crystal [5]. In principle, it is
conceived that LiNbO3 nanoparticles may be advantageously used for such biomedical purposes
considering the possibility of such nanoparticles being incorporated into the cells. Previous experiments
using microparticles have been performed [5] with similar results to those achieved with the substrate.
Therefore, the purpose of this work has been to fabricate and characterize the LiNbO3 nanoparticles and
assess their necrotic effects when they are incorporated on a culture of tumour cells.
Two different preparation methods have been used: 1) mechanical grinding from crystals, and 2)
bottom-up sol-gel chemical synthesis from metal-ethoxide precursors. This later method leads to a more
uniform size distribution of smaller particles (down to around 50 nm). Fig. 1(a) and 1(b) shows SEM
images of the nanoparticles obtained with both method.
An ad hoc software taking into account the physical properties of the crystal, particullarly donor
and aceptor concentrations has been developped in order to estimate the electric field generated in
noparticles. In a first stage simulations of the electric current of nanoparticles, in a conductive media,
due to the PV effect have been carried out by MonteCarlo simulations using the Kutharev 1-centre
transport model equations [6] . Special attention has been paid to the dependence on particle size and
[Fe2+]/[Fe3+]. First results on cubic particles shows large dispersion for small sizes due to the random
number of donors and its effective concentration (Fig 2).
The necrotic (toxicity) effect of nanoparticles incorporated into a tumour cell culture subjected to
30 min. illumination with a blue LED is shown in Fig.3. For each type of nanoparticle the percent of cell
survival in dark and illumination conditions has been plot as a function of the particle dilution factor. Fig.
1a corresponds to mechanical grinding particles whereas 1b and 1c refer to chemically synthesized
particles with two oxidation states. The light effect is larger with mechanical grinding nanoparticles, but
dark toxicity is also higher. For chemically synthesized nanoparticles dark toxicity is low but only in
oxidized samples, where the PV effect is known to be larger, the light effect is appreciable.
These preliminary results demonstrate that Fe:LiNbO· nanoparticles have a biological damaging
effect on cells, although there are many points that should be clarified and much space for PV
nanoparticles optimization. In particular, it appears necessary to determine the fraction of nanoparticles
that become incorporated into the cells and the possible existence of threshold size effects.
This work has been supported by MINECO under grant MAT2011-28379-C03
Optoelectronic generation of bio-aqueous femto-droplets based on the bulk photovoltaic effect
"© 2020 Optical Society of America. One print or electronic copy may be made for personal use only. Systematic reproduction and distribution, duplication of any material in this paper for a fee or for commercial purposes, or modifications of the content of this paper are prohibited"The generation and manipulation of small aqueous droplets is an important issue for nano- and biotechnology, particularly, when using microfluidic devices. The production of very small droplets has been frequently carried out by applying intense local electric fields to the fluid, which requires power supplies and metallic electrodes. This procedure complicates the device and reduces its versatility. In this work, we present a novel and flexible, to the best of our knowledge, electrodeless optoelectronic method for the production of tiny droplets of biologically friendly aqueous fluids. Our method takes advantage of the photoinduced electric fields generated by the bulk photovoltaic effect in iron-doped lithium niobate crystals. Two substrate configurations, presenting the polar ferroelectric axis either parallel or perpendicular to the active surface, have been successfully tested. In both crystal geometries, small droplets on the femtoliter scale have been obtained, although with a different spatial distributions correlated with the symmetry of the photovoltaic fields. The overall results demonstrate the effectiveness of the optoelectronic method to produce femtoliter droplets, both with pure water and with aqueous solutions containing biological materialMinisterio de Ciencia, Innovación y Universidades of Spain (MAT2017-83951-R); Marie Sklodowska-Curie Action COFUND (713366-InterTalentum
The C-type lectin homologue gene (EP153R) of African swine fever virus inhibits apoptosis both in virus infection and in heterologous expression
AbstractThe open reading frame EP153R of African swine fever virus (ASFV) encodes a nonessential protein that has been involved in the hemadsorption process induced in virus-infected cells. By the use of a virus deletion mutant lacking the EP153R gene, we have detected, in several virus-sensitive cells, increased levels of caspase-3 and cell death as compared with those obtained after infection with the parental BA71V strain. Both transient and stable expression of the EP153R gene in Vero or COS cells resulted in a partial protection of the transfected lines from the apoptosis induced in response to virus infection or external stimuli. The presence of gene EP153R resulted in a reduction of the transactivating activity of the cellular protein p53 in Vero cell cultures in which apoptosis was induced by virus infection or staurosporine treatment. This is to our knowledge the first description of a viral C-type lectin with anti-apoptotic properties
Antiviral activity of lauryl gallate against animal viruses
BACKGROUND: Antiviral compounds are needed in the control of many animal and human diseases. METHODS: We analysed the effect of the antitumoural drug lauryl gallate on the infectivity of the African swine fever virus among other DNA (herpes simplex and vaccinia) and RNA (influenza, porcine transmissible gastroenteritis and Sindbis) viruses, paying attention to its effect on the viability of the corresponding host cells. RESULTS: Viral production was strongly inhibited in different cell lines at non-toxic concentrations of the drug (1-10 microM), reducing the titres 3->5 log units depending on the multiplicity of infection. In our model system (African swine fever virus in Vero cells), the addition of the drug 1 h before virus adsorption completely abolished virus productivity in a one-step growth virus cycle. Interestingly, no inhibitory effect was observed when lauryl gallate was added after 5-8 h post-infection. Both cellular and viral DNA synthesis and late viral transcription were inhibited by the drug; however, the early viral protein synthesis and the virus-mediated increase of p53 remained unaffected. Activation of the apoptotic effector caspase-3 was not detected after lauryl gallate treatment of Vero cells. Furthermore, the presence of the drug abrogated the activation of this protease induced by the virus infection. CONCLUSIONS: Lauryl gallate is a powerful antiviral agent against several pathogens of clinical and veterinary importance. The overall results indicate that a cellular factor or function might be the target of the antiviral action of alkyl gallates.This work was supported by grants from Ministerio de Educación y Ciencia, Spain (BFU2004-00298/BMC), Laboratorios del Dr Esteve, Barcelona, Spain and by institutional grants from Fundación Ramón Areces, Madrid, Spain and Banco Central Hispano, Madrid, Spain. CH was a fellow from Fundación Ramón Areces. AGG was funded by Centro de Investigación en Sanidad Animal (CISA), Valdeolmos, Spain.N
A framework to move forward on the path to eco-innovation in the construction industry: implications to improve firms´ sustainable orientation
This paper examines key aspects in the innovative behavior of the
construction firms that determine their environmental orientation while innovating.
Structural equation modeling was used and data of 222 firms retrieved from the
Spanish Technological Innovation Panel (PITEC) for 2010 to analyse the drivers of
environmental orientation of the construction firms during the innovation process.
The results show that the environmental orientation is positively affected by the
product and process orientation of construction firms during the innovation process.
Furthermore, the positive relation between the importance of market information
sources and environmental orientation, mediated by process and product orientation,
is discussed. Finally, a model that explains these relations is proposed and validated.
Results have important managerial implications for those companies worried about
their eco-innovative focus as the types of actions and relations within firms most
suitable for improving their eco-innovative orientation are highlighted.The authors would like to thank the Spanish Economy and Competitiveness Ministry for its support through the research project (EC02011-27369) and also the Universitat Politecnica de Valencia (SP20140647).Segarra Oña, MDV.; Peiró Signes, A.; Cervelló Royo, RE. (2015). A framework to move forward on the path to eco-innovation in the construction industry: implications to improve firms´ sustainable orientation. Science and Engineering Ethics. 21(6):1469-1484. https://doi.org/10.1007/s11948-014-9620-2S14691484216Amara, N., & Landry, R. (2005). Sources of information as determinants of novelty of innovation in manufacturing firms: evidence from the 1999 statistics Canada innovation survey. Technovation, 25(3), 245–259.Anderson, J. C., & Gerbing, D. W. (1988). Structural equation modeling in practice: A review and recommended two- step approach. Psychological Bulletin, 103(3), 411–423.Ang, G. K. I. (2004). 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Glutathione in Cancer Cell Death
Glutathione (L-γ-glutamyl-L-cysteinyl-glycine; GSH) in cancer cells is particularly relevant in the regulation of carcinogenic mechanisms; sensitivity against cytotoxic drugs, ionizing radiations, and some cytokines; DNA synthesis; and cell proliferation and death. The intracellular thiol redox state (controlled by GSH) is one of the endogenous effectors involved in regulating the mitochondrial permeability transition pore complex and, in consequence, thiol oxidation can be a causal factor in the mitochondrion-based mechanism that leads to cell death. Nevertheless GSH depletion is a common feature not only of apoptosis but also of other types of cell death. Indeed rates of GSH synthesis and fluxes regulate its levels in cellular compartments, and potentially influence switches among different mechanisms of death. How changes in gene expression, post-translational modifications of proteins, and signaling cascades are implicated will be discussed. Furthermore, this review will finally analyze whether GSH depletion may facilitate cancer cell death under in vivo conditions, and how this can be applied to cancer therapy
African Swine Fever Virus IAP-Like Protein Induces the Activation of Nuclear Factor Kappa B
African swine fever virus (ASFV) encodes a homologue of the inhibitor of apoptosis (IAP) that promotes cell survival by controlling the activity of caspase-3. Here we show that ASFV IAP is also able to activate the transcription factor NF-κB. Thus, transient transfection of the viral IAP increases the activity of an NF-κB reporter gene in a dose-responsive manner in Jurkat cells. Similarly, stably transfected cells expressing ASFV IAP have elevated basal levels of c-rel, an NF-κB-dependent gene. NF-κB complexes in the nucleus were increased in A224L-expressing cells compared with control cells upon stimulation with phorbol myristate acetate (PMA) plus ionomycin. This resulted in greater NF-κB-dependent promoter activity in ASFV IAP-expressing than in control cells, both in basal conditions and after PMA plus ionophore stimulation. The elevated NF-κB activity seems to be the consequence of higher IκB kinase (IKK) basal activity in these cells. The NF-κB-inducing activity of ASFV IAP was abrogated by an IKK-2 dominant negative mutant and enhanced by expression of tumor necrosis factor receptor-associated factor 2
Apoptosis Induced in an Early Step of African Swine Fever Virus Entry into Vero Cells Does Not Require Virus Replication
AbstractPermissive Vero cells develop apoptosis, as characterized by DNA fragmentation, caspases activation, cytosolic release of mitochondrial cytochrome c, and flow cytometric analysis of DNA content, upon infection with African swine fever virus (ASFV). To determine the step in virus replication that triggers apoptosis, we used UV-inactivated virus, inhibitors of protein and nucleic acid synthesis, and lysosomotropic drugs that block virus uncoating. ASFV-induced apoptosis was accompanied by caspase-3 activation, which was detected even in the presence of either cytosine arabinoside or cycloheximide, indicating that viral DNA replication and protein synthesis were not required to activate the apoptotic process. The activation of caspase-3 was released from chloroquine inhibition 2 h after virus absorption, while the infection with UV-inactivated ASFV did not induce the activation of the caspase cascade. We conclude that ASFV induces apoptosis in the infected cell by an intracellular pathway probably triggered during the process of virus uncoating
Antigenic Properties and Diagnostic Potential of African Swine Fever Virus Protein pp62 Expressed in Insect Cells
African swine fever (ASF) is an infectious and economically important disease of domestic pigs. The absence of vaccine renders the diagnostic test the only tool that can be used for the control of new outbreaks of the disease. At present, the enzyme-linked immunosorbent assay (ELISA) test is the most useful method for large-scale ASF serological studies, although false positives have been detected, mainly on poorly preserved sera. In order to improve the current diagnostic test available for ASF, we have studied the antigenic properties of the ASF virus polyprotein pp62 and its suitability for use in a novel ELISA. Two well-known antigenic proteins of ASF virus, p32 and p54, were also included in this study. These proteins were expressed in the baculovirus expression system and used as antigens in ASF serological tests. Our results indicate that the use of these recombinant proteins as antigens in the ELISAs improves the sensitivity and specificity obtained with the conventional diagnosis test used to detect antibodies against ASF virus. Furthermore, the use of polyprotein pp62 in an ELISA for testing poorly preserved sera allows performance of the diagnosis of ASF without the need to confirm the results by the immunoblot test. These features make pp62 one of the most interesting viral proteins to be used for serological ASF diagnosis
Modulation of p53 Cellular Function and Cell Death by African Swine Fever Virus
Modulation of the activity of tumor suppressor p53 is a key event in the replication of many viruses. We have studied the function of p53 in African swine fever virus (ASFV) infection by determining the expression and activity of this transcription factor in infected cells. p53 levels are increased at early times of infection and are maintained throughout the infectious cycle. The protein is transcriptionally active, stabilized by phosphorylation, and localized in the nucleus. p53 induces the expression of p21 and Mdm2. Strikingly, these two proteins are located at the cytoplasmic virus factories. The retention of Mdm2 at the factory may represent a viral mechanism to prevent p53 inactivation by the protein. The expression of apoptotic proteins, such as Bax or active caspase-3, is also increased following ASFV infection, although the increase in caspase-3 does not appear to be, at least exclusively, p53 dependent. Bax probably plays a role in the induction of apoptosis in the infected cells, as suggested by the release of cytochrome c from the mitochondria. The significance of p21 induction and localization is discussed in relation to the shutoff of cellular DNA synthesis that is observed in ASFV-infected cells