186 research outputs found

    A time‐course study of the expression level of synaptic plasticity‐associated genes in un‐lesioned spinal cord and brain areas in a rat model of spinal cord injury: A bioinformatic approach

    Get PDF
    open8noFunding: This research was funded by the POR-FESR 2019-21, project “Mat2Rep”, Emilia Romagna Region (L.C.) and by the Cluster Tecnologici Nazionali, project IRMI, MIUR (L.C.). Marco Sanna is receiving a fellowship from the program “Alte Competenze” by Emilia Romagna Region. The contribution of “Fondazione Montecatone”, Imola (Italy) is also gratefully acknowledged.“Neuroplasticity” is often evoked to explain adaptation and compensation after acute lesions of the Central Nervous System (CNS). In this study, we investigated the modification of 80 genes involved in synaptic plasticity at different times (24 h, 8 and 45 days) from the traumatic spinal cord injury (SCI), adopting a bioinformatic analysis. mRNA expression levels were analyzed in the motor cortex, basal ganglia, cerebellum and in the spinal segments rostral and caudal to the lesion. The main results are: (i) a different gene expression regulation is observed in the Spinal Cord (SC) segments rostral and caudal to the lesion; (ii) long lasting changes in the SC includes the extracellular matrix (ECM) enzymes Timp1, transcription regulators (Egr, Nr4a1), second messenger associated proteins (Gna1, Ywhaq); (iii) long‐lasting changes in the Motor Cortex includes transcription regulators (Cebpd), neurotransmitters/neuromodulators and receptors (Cnr1, Gria1, Nos1), growth factors and related receptors (Igf1, Ntf3, Ntrk2), second messenger associated proteins (Mapk1); long lasting changes in Basal Ganglia and Cerebellum include ECM protein (Reln), growth factors (Ngf, Bdnf), transcription regulators (Egr, Cebpd), neurotransmitter receptors (Grin2c). These data suggest the molecular mapping as a useful tool to investigate the brain and SC reorganization after SCI.openBaldassarro V.A.; Sanna M.; Bighinati A.; Sannia M.; Gusciglio M.; Giardino L.; Lorenzini L.; Calzà LauraBaldassarro V.A.; Sanna M.; Bighinati A.; Sannia M.; Gusciglio M.; Giardino L.; Lorenzini L.; Calzà Laur

    Control of vibration using compliant actuators

    Get PDF
    This work proposes a method for controlling vibration using compliant-based actuators. The compliant actuator combines a conventional actuator with elastic elements in a series configuration. The benefits of compliant actuators for vibration control applications, demonstrated in this work, are twofold: (i) vibration reduction over a wide frequency bandwidth by passive control means; (ii) improvement of vibration control performance when active control is applied using the compliant actuator. The vibration control performance is compared with the control performance achieved using the well-known vibration absorber and conventional rigid actuator systems. The performance comparison showed that the compliant actuator provided a better flexibility in achieving vibration control over a certain frequency bandwidth. The passive and active control characteristics of the compliant actuator are investigated, which shows that the control performance is highly dependent on the compliant stiffness parameter. The active control characteristics are analyzed by using the Proportional and Derivative (PD) control strategy which demonstrated the capability of effectively changing the respective effective stiffness and damping of the system. These attractive dual passive-active control characteristics are therefore advantageous for achieving an effective vibration control system, particularly for controlling the vibration over a specific wide frequency bandwidth

    Association of kidney disease measures with risk of renal function worsening in patients with type 1 diabetes

    Get PDF
    Background: Albuminuria has been classically considered a marker of kidney damage progression in diabetic patients and it is routinely assessed to monitor kidney function. However, the role of a mild GFR reduction on the development of stage 653 CKD has been less explored in type 1 diabetes mellitus (T1DM) patients. Aim of the present study was to evaluate the prognostic role of kidney disease measures, namely albuminuria and reduced GFR, on the development of stage 653 CKD in a large cohort of patients affected by T1DM. Methods: A total of 4284 patients affected by T1DM followed-up at 76 diabetes centers participating to the Italian Association of Clinical Diabetologists (Associazione Medici Diabetologi, AMD) initiative constitutes the study population. Urinary albumin excretion (ACR) and estimated GFR (eGFR) were retrieved and analyzed. The incidence of stage 653 CKD (eGFR < 60 mL/min/1.73 m2) or eGFR reduction > 30% from baseline was evaluated. Results: The mean estimated GFR was 98 \ub1 17 mL/min/1.73m2 and the proportion of patients with albuminuria was 15.3% (n = 654) at baseline. About 8% (n = 337) of patients developed one of the two renal endpoints during the 4-year follow-up period. Age, albuminuria (micro or macro) and baseline eGFR < 90 ml/min/m2 were independent risk factors for stage 653 CKD and renal function worsening. When compared to patients with eGFR > 90 ml/min/1.73m2 and normoalbuminuria, those with albuminuria at baseline had a 1.69 greater risk of reaching stage 3 CKD, while patients with mild eGFR reduction (i.e. eGFR between 90 and 60 mL/min/1.73 m2) show a 3.81 greater risk that rose to 8.24 for those patients with albuminuria and mild eGFR reduction at baseline. Conclusions: Albuminuria and eGFR reduction represent independent risk factors for incident stage 653 CKD in T1DM patients. The simultaneous occurrence of reduced eGFR and albuminuria have a synergistic effect on renal function worsening

    ICAROS (Italian survey on CardiAc RehabilitatiOn and Secondary prevention after cardiac revascularization): Temporary report of the first prospective, longitudinal registry of the cardiac rehabilitation network GICR/IACPR

    Get PDF

    Intensification of bioconversion processes: design and development of reactors with high biocatalyst loading

    No full text
    The aim of the research program was to address some open issues related to immobilization of biological systems (enzymes, microrganisms) for bioprocess applications. The research pathway is ultimately targetted at the development of novel and effective tools for bioprocess intensification based on the use of immobilizer biocatalysts. The attention has been specifically focused on two processes: an enzymatic and a microbial process. Conversion of the synthetic dye Remazol Brilliant Blue R (RBBR) by means of crude laccase mixtures from Pleurotus ostreatus. The study aimed at the optimization of the enzymes immobilization protocol and at the characterization of the RBBR conversion by means of free and immobilizer enzymes. The immobilization process was optimized with reference to the covalent binding on granular supports - EUPERGIT C 250L©. In particular, operating conditions were selected so as to maximize the immobilization yield. A reactor for the activity assay of the immobilised enzymes was designed and set-up. The kinetics of RBBR conversion by means of immobilized laccase mixtures was characterised using a purposely designed fixed bed reactor. A kinetic model has been best-fitted against experimental data relative to conversion degree and reactor space-time to assess kinetic parameters. The role of mass transport phenomena between the phases and of adsorption during heterogeneous enzymatic conversion of the dye were investigated. Based on data collected in the experimental campaign and on kinetic models developed, two alternative processes for remediation of dye-bearing wastewaters have been assessed: i) a batch Stirred Tank Reactor (STR) operated with a homogeneous liquid phase containing both the crude laccase mixture and the dye; ii) a Continuous Fixed Bed Reactor (CFBR) loaded with laccases immobilised on EUPERGIT© and continuously fed with the dye-bearing liquid stream. The results highlighted the role played by biocatalyst stability and immobilisation yield on the selection of the best option in terms of the volume of wastewater cumulatively treated in either option. Conversion of the phenol by means of Pseudomonas sp. OX1 biofilm in threephase bioreactors. The study has addressed both experimental and theoretical aspects of the problem. The experimental study has been directed to the assessment of the growth of P. sp OX1 biofilm on silica-based granular supports. Two bench-scale reactor typologies were investigated: a three Phase Circulating (3PC) reactor and an Internal Loop Airlift (ILA) reactor. Tests with the 3PC reactor were directed to optimize the conditions for biofilm growth. Tests with the ILA reactor were aimed at investigating the effect of dilution rate on the performance of the system operated with a mature biofilm that had been previously partly grown up on the solid carrier. The theoretical work has addressed the analysis of the bifurcational and dynamic patterns of an ILA reactor operated with biofilm of P. sp. OX1 attached on granular solids. The role of the growth rate of suspended and immobilised cells using phenol as carbon source, the adhesion rate of suspended cells on carrier surface and the detachment rate of biofilm from the solids carrier were investigated. The dependence of bifurcational patterns on detachment coefficient and dilution rate has been analysed. Results from the theoretical study and from tests carried out with the ILA reactor were compared: the model properly reproduces the functional dependence of the steady state behaviour of the biofilm on the dilution rate observed during the tests

    Recombinant expression of Pleurotus ostreatus laccases in Kluyveromyces lactis and Saccharomyces cerevisiae

    No full text
    Heterologous expression of Pleurotus ostreatus POXC and POXA1b laccases in two yeasts, Kluyveromyces lactis and Saccharomyces cerevisiae, was performed. Both transformed hosts secreted recombinant active laccases, although K. lactis was much more effective than S. cerevisiae. rPOXA1b transformants always had higher secreted activity than rPOXC transformants did. The lower tendency of K. lactis with respect to S. cerevisiae to hyperglycosylate recombinant proteins was confirmed. Recombinant laccases from K. lactis were purified and characterised. Specific activities of native and recombinant POXA1b are similar. On the other hand, rPOXC specific activity is much lower than that of the native protein, perhaps due to incomplete or incorrect folding. Both recombinant laccase signal peptides were correctly cleaved, with rPOXA1b protein having two C-terminal amino acids removed. The availability of the established recombinant expression system provides better understanding of laccase structure-function relationships and allows the development of new oxidative catalysts through molecular evolution techniques

    Recombinant expression of Pleurotus ostreatus laccases in Kluyveromyces lactis and Saccharomyces cerevisiae

    No full text
    Heterologous expression of Pleurotus ostreatus POXC and POXA1b laccases in two yeasts, Kluyveromyces lactis and Saccharomyces cerevisiae, was performed. Both transformed hosts secreted recombinant active laccases, although K. lactis was much more effective than S. cerevisiae. rPOXA1b transformants always had higher secreted activity than rPOXC transformants did. The lower tendency of K. lactis with respect to S. cerevisiae to hyperglycosylate recombinant proteins was confirmed. Recombinant laccases from K. lactis were purified and characterised. Specific activities of native and recombinant POXA1b are similar. On the other hand, rPOXC specific activity is much lower than that of the native protein, perhaps due to incomplete or incorrect folding. Both recombinant laccase signal peptides were correctly cleaved, with rPOXA1b protein having two C-terminal amino acids removed. The availability of the established recombinant expression system provides better understanding of laccase structure-function relationships and allows the development of new oxidative catalysts through molecular evolution techniques
    • 

    corecore