Copper(II) complexes of hydroxyflavone derivatives as potential bioactive molecule to combat antioxidants: synthesis,characterization and pharmacological activities

A variety of novel copper complexes were synthesized and characterized of the formulae [Cu(L¹)(OAc)], [CuL²(H₂O)], [CuL³(H₂O)], [CuL⁴(OAc)], [CuL⁵(H₂O)] [CuL⁶], [CuL⁷], [CuL⁸](OAc) and [CuL⁹], where L¹ L⁹ represents Schiff base ligands [derived by the condensation of 5‐hydroxyflavone with 4‐aminoantipyrine (L¹), o‐aminophenol (L²), o‐aminobenzoic acid (L³), o‐aminothiazole (L⁴), thiosemicarbazide (L⁵), 4‐aminoantipyrine‐o‐aminophenol (L⁶), 4‐aminoantipyrine‐o‐aminobenzoic acid (L⁷), 4‐aminoantipyrine‐o‐aminothiazole(L⁸) and 4‐aminoantipyrine‐thiosemicarbazide (L⁹)]. The spectral and magnetic results of the Cu(II) complexes exhibit square planar geometry. The DNA binding properties of copper complexes were studied by using electronic absorption spectra, viscosity and thermal denaturation experiments. The results show that the complexes were interacting with calf thymus (CT DNA). The in vitro antimicrobial activities of the investigated compounds were tested against the bacterial species and fungal species. Superoxide dismutase and antioxidant activities of the copper complexes have also been studied. Copyright © 2011 John Wiley & Sons, Ltd.     

Synthesis,characterization and molecular docking of new C,N‐palladacycles containing pyridinium‐derived ligands: DNA and BSA interaction studies and evaluation as anti‐tumor agents

Four new monomeric Pd (II) complexes with formulas [Pd(C,N)‐(2′‐NH₂C₆H₄)C₆H₄ (N₃)(L)] ( A ), ( B ) and [Pd(C,N)‐C₆H₄CH₂NH(C₄H₉)(N₃)(L)] ( C ), ( D ), [L = isonicotinamide for ( A ) and ( C ), L = 4‐N,N‐dimethylaminopyridine for ( B ) and ( D )] have been synthesized using four initial dimers [Pd₂{(C,N)‐(2′‐NH₂C₆H₄)C₆H₄}₂(μ‐OAc)₂] ( 1 ), [Pd₂{(C,N)‐ (2′‐NH₂C₆H₄)C₆H₄}₂(μ‐N₃)₂] ( 3 ) for A and C , and [Pd₂{(C,N)‐C₆H₄CH₂NH(C₄H₉)}₂(μ‐OAc)₂] ( 2 ) and [Pd₂{(C,N)‐C₆H₄CH₂NH(C₄H₉)}₂(μ‐N₃)₂] ( 4 ) for B and D . Then synthesized complexes have been characterized by Fourier transform‐infrared, NMR spectroscopy and thermal gravimetric‐differential thermal analysis. Furthermore, UV–Vis spectroscopy, fluorescence spectroscopy, circular dichroism (CD) and helix melting temperature measurements have been employed to study the binding interaction of them with calf thymus‐deoxyribonucleic acid (DNA). The results reveal that all synthesized complexes can interact with DNA via groove‐binding mode. Bovine serum albumin (BSA)‐binding studies have been carried out using UV–Vis spectroscopy, emission titration and CD. However, competitive binding studies using warfarin, ibuprofen and digoxin on site markers demonstrated that the complexes bind to different sites on BSA. The results also indicated that the binding site was mainly located within site‐III for complex A , and site‐I for complexes B , C and D of BSA. In addition, molecular docking studies have been executed to determine the binding site of the DNA and BSA with complexes. Eventually, in vitro cytotoxicity of synthesized palladium complexes and cisplatin were carried out against human promyelocytic leukemia cancer (Hela) and breast cancer (MCF‐7) cell lines. Pursuant to the IC₅₀ values, the cytotoxicity of complexes against MCF‐7 was more than Hela.     

Protein Denaturation Through the Use of Magnetic Molecularly Imprinted Polymer Nanoparticles

The inhibition of the protein function for therapeutic applications remains challenging despite progress these past years. While the targeting application of molecularly imprinted polymer are in their infancy, no use was ever made of their magnetic hyperthermia properties to damage proteins when they are coupled to magnetic nanoparticles. Therefore, we have developed a facile and effective method to synthesize magnetic molecularly imprinted polymer nanoparticles using the green fluorescent protein (GFP) as the template, a bulk imprinting of proteins combined with a grafting approach onto maghemite nanoparticles. The hybrid material exhibits very high adsorption capacities and very strong affinity constants towards GFP. We show that the heat generated locally upon alternative magnetic field is responsible of the decrease of fluorescence intensity.     

High quality drug screening by capillary electrophoresis: A review

High quality assays are needed in drug discovery to reduce the high attrition rate of lead compounds during primary screening. Capillary electrophoresis (CE) represents a versatile micro-separation technique for resolution of enzyme-catalyzed reactions, including substrate(s), product(s), cofactor(s) and their stereoisomers, which is needed for reliable characterization of biomolecular interactions in free solution. This review article provides a critical overview of new advances in CE for drug screening over the past five years involving biologically relevant enzymes of therapeutic interest, including transferases, hydrolases, oxidoreductases, and isomerases. The basic principles and major configurations in CE, as well as data processing methods needed for rigorous characterization of enzyme inhibition are described. New developments in functional screening of small molecules that modulate the activity of disease-related enzymes are also discussed. Although inhibition is a widely measured response in most enzyme assays, other important outcomes of ligand interactions on protein structure/function that impact the therapeutic potential of a drug will also be highlighted, such as enzyme stabilization, activation and/or catalytic uncoupling. CE offers a selective platform for drug screening that reduces false-positives while also enabling the analysis of low amounts of complex sample mixtures with minimal sample handling.     

温度对猪血提取超氧化物歧化酶的影响

用不同的温度与不同的时间对猪血超氧化物歧化酶液进行处理，结果表明：随着温度的升高和处理时间的延长，酶活性和杂蛋白均呈下降趋势，但从此活性上看，猪血SOD的处理以变性温度55－65℃，变性时间为15－26min最适宜，酶纯度最高。     

Heat Denaturation of Protein Structures and Chlorophyll States in PSII Membranes

IntroductionPhotosystem II (PSII) is a large supramolecularpigment-protein complex found in the thylakoidmembranes of green plants,algae andcyanobacteria.Its main role is to drive light-induced electron transfer from water toplastoquinone with a concomitant production ofmolecular oxygen.PSII membranes consist of anouter antenna portion of light-harvestingchlorophyll (Chl) a/b binding complexes (LHCII)and a core fraction.The core fraction is composedof an inner antenna of membrane-bound …     

球状功能性烟草花叶病毒纳米颗粒的制备及表征

烟草花叶病毒(TMV)由于其良好的生物相容性、单分散性、多价性、低成本等优点,已作为功能材料的基本构筑单元应用于光电器件、组织工程、疫苗载体,无机纳米材料制备等研究领域。然而,相比于棒状的TMV,球状TMV纳米颗粒无核酸分子,抗环境影响能力更强,比表面积更大。本文利用蛋白质的热致变性原理,对经基因和化学改性后的棒状TMV如半胱氨酸突变体(TMV-Cys)、赖氨酸突变体(TMV-EPMK)和β-环糊精(β-CD)修饰的TMV(TMV-β-CD)进行热变性处理,探究其形成球型纳米颗粒(TMV-SNP)的能力及功能性。结果显示,改性后的TMV经历热变性后可得到形貌均一的球型纳米颗粒,且其暴露在纳米颗粒表面的功能基团Cys、Lys和β-CD仍具有反应活性。     

Antimicrobial and inhibition on heat-induced protein denaturation of constituents isolated from Polygonatum verticillatum rhizomes

This study was designed to assess the susceptibility of various microorganisms and inhibition on heat-induced protein denaturation against diosgenin and santonin, isolated from Polygonatum verticillatum rhizomes. Both diosgenin and santonin showed significant zone of inhibition when studied against various Gram-positive (Bacillus subtilis, Bacillus cereus, Staphylococcus aureus and Staphylococcus epidermidis) and Gram-negative bacteria (Escherichia coli and Salmonella typhi). In antifungal assay, only santonin exhibited profound sensitivity against various fungi (Aspergillus flavus, Aspergillus niger, Trichoderma harzianum and Fusarium oxysporum) used in the test. Both diosgenin and santonin also exhibited marked attenuation on heat-induced protein denaturation in a concentration-dependent manner with EC₅₀ values of 375 and 310 μg/mL, respectively. In conclusion, both the isolated compounds have antimicrobial potential supported by strong inhibition on protein denaturation and thus support the antimicrobial uses of plant in traditional system of treatment.     

FTIR‐ATR Study of pH Effects on Egg Albumin Secondary Structure

Abstract

The pH effects on the secondary structures of egg albumin were investigated using Fourier transform infrared–attenuated total reflection (FTIR‐ATR) technique with a single‐bounce diamond crystal. The albumin was first denatured in a series of solutions with pH ranging from 1 to 12. The albumin film was then cast on the ATR crystal from the albumin solution for the IR spectrum collection. Significant secondary structure spectral differences were observed for these films. The findings are presented in terms of the shape and position of the albumin amide I band between 1600 and 1700 cm^?1.