Mcintoshlong3176

Rhamnogalaturonans I (RGI) pectins, which are a major component of the plant primary cell wall, can be recalcitrant to digestion by commercial enzymatic cocktails, in particular during fruit juice clarification process. To overcome these problems and get better insights into RGI degradation, three RGI degrading enzymes (RHG Endo-rhamnogalacturonase; ABF α-Arabinofuranosidases; GAN Endo-β-1,4-galactanase) from Aspergillus aculeatinus were expressed in Pichia pastoris, purified and fully biochemically characterized. All three enzymes showed acidic pH optimum, and temperature optima between 40-50 °C. The Km values were 0.5 mg.ml-1, 1.64 mg.ml-1 and 3.72 mg.ml-1 for RHG, ABF, GAN, respectively. NMR analysis confirmed an endo-acting mode of action for RHG and GAN, and exo-acting mode for ABF. The application potential of these enzymes was assessed by measuring changes in viscosity of RGI-rich camelina mucilage, showing that RHG-GAN enzymes induced a decrease in viscosity by altering the structures of the RGI backbone and sidechains.This study presented a novel utilization of biomass solid waste, named Polyalthia longifolia (Mast tree) seed as a reinforcement in a composite, using a compression molding technique. An attempt was made to reinforce vinyl ester matrix (VE) with Polyalthia longifolia seed filler (PLSF), ranging from 5 to 50 wt% loadings. Mechanical properties of the fabricated Polyalthia longifolia seed filler/vinyl ester (PLSF-VE) composite samples were tested and analyzed. The results showed that the PLSF-VE composite exhibited optimum mechanical properties at 25 % wt of filler loading; ultimate tensile strength and modulus were approximately 32.50 MPa and 1.23 GPa, respectively. The ultimate flexural, impact strengths and hardness were observed around 125 MPa, 31.09 kJ/m2 and 36.50, respectively. The heat deflection test and thermo-gravimetric analysis depicted that the PLSF-VE composites withstood up to 66 °C and 430 °C, respectively. Furthermore, the PLSF and its various composite samples were studied, using energy-dispersive X-ray (EDX), X-ray diffraction (XRD), Fourier transform infrared spectroscopy (FTIR) and scanning electron microscope (SEM).Carboxylated bacterial cellulose (OBC) was fabricated by oxidation with nitrogen dioxide in chloroform/cyclohexane and employed as a carrier for sustained release of antitumor substance cisplatin (CDDP). The influence of removing water method, solvent used in the synthesis, concentration of N2O4, and duration of the oxidation on content of carboxyl groups in reaction products was established. Due to the possibility of nitrogen dioxide to penetrate into cellulose crystallites, the carboxyl group content of the OBC reaches high values up to 4 mmol/g. In vitro degradation of OBC was determined under simulated physiological conditions. The immobilization of CDDP on OBC was studied in detail. The initial burst release of the drug from the polymer was depressed. The cytotoxicity of CDDP-loaded OBC was evaluated with HeLa cells. The unique structure and properties of OBC make it a great candidate as drug delivery carrier.This work aimed to produce and characterize cellulose nanofibers obtained from cassava peel with a combination of pre-treatments with acid hydrolysis or TEMPO-mediated oxidation and ultrasonic disintegration. All nanofibers presented nanometric diameter (5-16 nm) and high negative zeta potential values (around -30 mV). Oscillatory rheology showed a gel-like behavior of the aqueous suspensions of nanofibers (1.0-1.8 % w/w), indicating their use as reinforcement for nanocomposite or as a thickening agent. Additionally aqueous suspensions of nanofibers obtained by acid hydrolysis presented higher gel strength than those produced by TEMPO-mediated oxidation. However, ultrasound application increased even more viscoelastic properties. Flow curves showed that suspensions of nanofibers obtained by acid hydrolysis presented a thixotropy behavior and viscosity profile with three regions. Therefore our results showed that it is possible to tune mechanical properties of cellulose nanofibers choosing and modifying chemical and physical process conditions in order to allow a number of applications.The exopolymer (EPSp) produced by the strain B. licheniformis IDN-EC was isolated and characterized using different techniques (MALDI-TOF, NMR, ATR-FTIR, TGA, DSC, SEM). The results showed that the low molecular weight EPSp contained a long polyglutamic acid and an extracellular teichoic acid polysaccharide. The latter was composed of poly(glycerol phosphate) and was substituted at the 2-position of the glycerol residues with a αGal and αGlcNH2. The αGal O-6 position was also found to be substituted by a phosphate group. The antiviral capability of this EPSp was also tested on both enveloped (herpesviruses HSV, PRV and vesicular stomatitis VSV) and non-enveloped (MVM) viruses. The EPSp was efficient at inhibiting viral entry for the herpesviruses and VSV but was not effective against non-enveloped viruses. The in vivo assay of the EPSp in mice showed no signs of toxicity which could allow for its application in the healthcare sector.Herein, a nanotherapeutic delivery method was presented for co-delivery of doxorubicin (DOX) and aptamer against Forkhead box M1 (FOXM1 Apt) to cancer cells. Firstly, the vehicle composed of chitosan (CS)-Gold nanoparticles (AuNPs) conjugate was prepared. Nucleolin aptamer (AS1411) and FOXM1 Apt were loaded onto the CS-AuNPs and formed Aptamers (Apts)-CS-AuNPs. Subsequently, DOX was added to the Apts-CS-AuNPs to obtain the DOX-Apts-CS-AuNPs complex for synergistic treatment of tumor. selleck The data of flow cytometry analysis and fluorescence imaging displayed that the complex was effectively internalized into target cells (A549 and 4T1 cells, nucleolin+) but not into CHO cells as nontarget cells. The results of the MTT assay showed that the complex significantly increased cell mortality in 4T1 and A549 cells compared to CHO cells treated with the complex. The in vivo studies demonstrated that the DOX-Apts-CS-AuNPs complex exhibited more tumor inhibitory effect and less distribution in other organs compared to free DOX.