Dual‐energy CT imaging of nasopharyngeal cancer cells using multifunctional gold nanoparticles

The purpose of this study is to measure the concentration of gold nanoparticles (AuNPs) attached to folic acid through cysteamin as the linker (FA‐Cys‐AuNPs) and AuNPs in KB human nasopharyngeal cancer cells using dual‐energy CT (DECT). In this study, nanoparticles with a size of ∼15 nm were synthesized and characterised using UV‐Vis, TEM, FTIR and ICP‐OES analyses. The non‐toxicity of nanoparticles was confirmed by MTT assay under various concentrations (40– 100 µg/ml) and incubation times (6, 12 and 24 h). To develop an algorithm for revealing different concentrations of AuNPs in cells, a corresponding physical phantom filled with 0.5 ml vials containing FA‐Cys‐AuNPs was used. The CT scan was performed at two energy levels (80 and 140 kVp). One feature of DECT is material decomposition, which allows separation and identification of different elements. The values obtained from the DECT algorithm were compared with values quantitatively measured by ICP‐OES. Cells were also incubated with AuNPs and FA‐Cys‐AuNPs at different concentrations and incubation times. Subsequently, by increasing the incubation time in the presence of FA‐Cys‐AuNPs, in comparison with AuNPs, DECT pixels were increased. Thus, FA‐Cys‐AuNPs could be a suitable candidate for targeted contrast agent in DECT molecular imaging of nasopharyngeal cancer cells.Inspec keywords: biomedical materials, phantoms, nanoparticles, computerised tomography, nanomedicine, cancer, toxicology, nanofabrication, gold, cellular biophysics, ultraviolet spectra, visible spectra, transmission electron microscopy, Fourier transform infrared spectraOther keywords: Au, time 24.0 hour, time 12.0 hour, time 6.0 hour, head cancer cells, DECT molecular imaging, DECT algorithm, material decomposition, physical phantom, MTT assay, ICP‐OES analyses, FTIR spectra, TEM, UV‐vis spectrophotometry, cysteamin, folic acid, gold nanoparticle concentration, nasopharyngeal cancer cells, dual‐energy CT imaging, neck cancer cells, KB human nasopharyngeal cancer cells, multifunctional gold nanoparticles     

Surface‐functionalised hybrid nanoparticles for targeted treatment of cancer

Cancer is a leading cause of death worldwide. Despite the great advancement in understanding the pharmacology and biology of cancer, it still signifies one of the most serious human‐health related problems. The current treatments for cancer may include surgery, radiotherapy, and chemotherapy, but these procedures have several limitations. Current studies have shown that nanoparticles (NPs) can be used as a novel strategy for cancer treatment. Developing nanosystems that allow lower doses of therapeutic agents, as well as their selective release in tumour cells, may resolve the challenges of targeted cancer therapy. In this review, the authors discuss the role of the size, shape, and surface modifications of NPs in cancer treatment. They also address the challenges associated with cancer therapies based on NPs. The overall purpose of this review is to summarise the recent developments in designing different hybrid NPs with promising therapeutic properties for different types of cancer.Inspec keywords: tumours, reviews, patient treatment, nanomedicine, surgery, radiation therapy, cellular biophysics, nanobiotechnology, nanoparticles, cancerOther keywords: current treatments, cancer treatment, targeted cancer therapy, cancer therapies, surface‐functionalised hybrid nanoparticles, targeted treatment, serious human‐health related problems     

Colorimetric‐based detection of Ureaplasma urealyticum using gold nanoparticles

Ureaplasma urealyticum (uu) is one of the most common agents of urogenital infections and is associated with complications such as infertility, spontaneous abortion and other sexually transmitted diseases. Here, a DNA sensor based on oligonucleotide target‐specific gold nanoparticles (AuNPs) was developed, in which the dispersed and aggregated states of oligonucleotide‐functionalised AuNPs were optimised for the colorimetric detection of a polymerase chain reaction (PCR) amplicon of U. urealyticum DNA. A non‐cross‐linking approach utilising a single Au‐nanoprobe specific of the urease gene was utilised and the effect of a PCR product concentration gradient evaluated. Results from both visual and spectral analyses showed that target–Au‐nanoprobe hybrids were stable against aggregation after adding the inducer. Furthermore, when a non‐target PCR product was used, the peak position shifted and salt‐induced aggregation occurred. The assay''s limit of detection of the assay was 10 ng with a dynamic range of 10–60 ng. This procedure provides a rapid, facile and low‐cost detection format, compared to methods currently used for the identification of U. urealyticum.Inspec keywords: patient diagnosis, diseases, enzymes, nanosensors, microorganisms, molecular biophysics, DNA, nanoparticles, aggregation, cellular biophysics, colorimetry, genetics, gold, nanomedicineOther keywords: urogenital infections, infertility, spontaneous abortion, sexually transmitted diseases, DNA sensor, oligonucleotide target‐specific gold nanoparticles, oligonucleotide‐functionalised AuNPs, colorimetric detection, polymerase chain reaction amplicon, noncross‐linking approach, single Au‐nanoprobe specific, urease gene, visual analyses, spectral analyses, target–Au‐nanoprobe hybrids, nontarget PCR product, salt‐induced aggregation, rapid cost detection format, facile cost detection format, low‐cost detection format, PCR product concentration, Ureaplasma urealyticum DNA, Au     

Cu‐induced assembly of methanobactin‐modified gold nanoparticles and its peroxidase mimic activity

Methanobactin (Mb) is a small copper‐chelating molecule that functions as an agent for copper acquisition, uptake and copper‐containing methane monooxygenase catalysis in methane‐oxidising bacteria. The UV–visible spectral and fluorescence spectral suggested that Mb/Cu coordination complex as a monomer (Mb‐Cu), dimmer (Mb₂ ‐Cu) and tetramer (Mb₄ ‐Cu) could be obtained at different ratios of Mb to Cu (II). The kinetics of the oxidation of hydroquinone with hydrogen peroxide catalysed by the different Mb/Cu coordination complex were investigated. The results suggested that Mb₂ ‐Cu coordination form has highest catalytic capacity. Further, Mb‐modified gold nanoparticles (AuNPs) were obtained by ligand exchange and assembled into two‐ and three‐D nanocluster structure by metal‐organic coordination as driving force. It has been found that AuNPs increased the catalytic activity of Mb₂ ‐Cu on AuNPs. The more significant catalytic activity was exhibited by the nanocluster assembly with multi‐catalytic centres. This may be attributed to the multivalent collaborative characteristics of the catalytic active centres in the nanocluster network assembly. The assembly of Mb‐modified AuNPs can act as excellent nanoenzyme models for imitating peroxidase.Inspec keywords: nanoparticles, catalysis, oxidation, enzymes, microorganisms, nanobiotechnology, gold, organic compounds, reduction (chemical), visible spectra, molecular biophysics, ultraviolet spectra, biochemistry, copper, nanofabrication, fluorescenceOther keywords: Mb‐modified gold nanoparticles, catalytic active centres, Mb‐modified AuNPs, Cu‐induced assembly, methanobactin‐modified gold nanoparticles, peroxidase mimic activity, copper‐chelating molecule, copper‐containing methane monooxygenase catalysis, methane‐oxidising bacteria, fluorescence, Mb/Cu coordination complex, catalytic activity, UV–visible spectra, nanocluster assembly, Cu, Au     

Treatment of tumour tissue with radio‐frequency hyperthermia (using antibody‐carrying nanoparticles)

Intelligent inorganic nanoparticles were designed and produced for use in imaging and annihilating tumour cells by radio‐frequency (RF) hyperthermia. Nanoparticles synthesised to provide RF hyperthermia must have magnetite properties. For this purpose, magnetite nanoparticles were first synthesised by the coprecipitation method (10–15 NM). These superparamagnetic nanoparticles were then covered with gold ions without losing their magnetic properties. In this step, gold ions are reduced around the magnetite nanoparticles. Surface modification of the gold‐coated magnetic nanoparticles was performed in the next step. A self‐assembled monolayer was created using cysteamine (2‐aminoethanethiol) molecules, which have two different end groups (SH and NH₂). These molecules react with the gold surface by SH groups. The NH₂ groups give a positive charge to the nanoparticles. After that, a monoclonal antibody (Monoclonal Anti‐N‐CAM Clone NCAM‐OB11) was immobilised by the 1‐ethyl‐3‐(3‐dimethylaminopropyl)carbodiimide/N‐hydroxysuccinimide method. Then, the antenna RF system (144.00015 MHz) was created for RF hyperthermia. The antibody‐nanoparticle binding rate and cytotoxicity tests were followed by in vitro and in vivo experiments. As the main result, antibody‐bound gold‐coated magnetic nanoparticles were successfully connected to tumour cells. After RF hyperthermia, the tumour size decreased owing to apoptosis and necrosis of tumour cells.     

Synthesis,characterisation and anti‐tumour activity of biopolymer based platinum nanoparticles and 5‐fluorouracil loaded platinum nanoparticles

A facile and green synthesis of platinum nanoparticles [gum kondagogu platinum nanoparticles (GKPtNP)] using biopolymer‐ gum kondagogu was developed. The formation of GKPtNP was confirmed by ultraviolet (UV)–visible spectroscopy, scanning electron microscopy–energy dispersive X‐ray spectroscopy, transmission electron microscopy, X‐ray diffraction, Zeta potential, Fourier transform infrared, inductively coupled plasma mass spectroscopy. The formed GKPtNP are well dispersed, homogeneous with a size of 2–4 ± 0.50 nm, having a negative zeta potential (−46.1 mV) indicating good stability. 5‐Fluorouracil (5FU) was loaded onto the synthesised GKPtNP, which leads to the development of a new combination of nanomedicine (5FU–GKPtNP). The in vitro drug release studies of 5FU–GKPtNP in pH 7.4 showed a sustained release profile over a period of 120 min. Agrobacterium tumefaciens induced in vitro potato tumour bioassay was employed for screening the anti‐tumour potentials of GKPtNP, 5FU, and 5FU–GKPtNP. The experimental results suggested a complete tumour inhibition by 5FU–GKPtNP at a lower concentration than the GKPtNP and 5FU. Furthermore, the mechanism of anti‐tumour activity was assessed by their interactions with DNA using agarose gel electrophoresis and UV‐spectroscopic analysis. The electrophoresis results revealed that the 5FU–GKPtNP totally diminishes DNA and the UV‐spectroscopic analysis showed a hyperchromic effect with red shift indicating intercalation type of binding with DNA. Over all, the present study revealed that the combined exposure of the nanoformulation resulted in the enhanced anti‐tumour effect. Inspec keywords: nanoparticles, transmission electron microscopy, biomedical materials, tumours, ultraviolet spectra, DNA, drugs, electrophoresis, polymers, platinum, pH, drug delivery systems, biochemistry, X‐ray chemical analysis, microorganisms, molecular biophysics, electrokinetic effects, X‐ray diffraction, scanning electron microscopy, cancer, nanofabrication, visible spectra, nanomedicine, Fourier transform infrared spectra, materials preparationOther keywords: 5FU–GKPtNP, 5‐fluorouracil loaded platinum nanoparticles, gum kondagogu platinum nanoparticles, antitumour activity, scanning electron microscopy‐energy dispersive X‐ray spectroscopy, biopolymer‐based platinum nanoparticles, biopolymer‐based platinum nanoparticles, ultraviolet‐visible spectroscopy, UV‐visible spectroscopy, transmission electron microscopy, X‐ray diffraction, zeta potential, Fourier transform infrared spectroscopy, inductively coupled plasma mass spectroscopy, nanomedicine, in vitro drug release studies, sustained release profile, Agrobacterium tumefaciens, in vitro potato tumour bioassay, tumour inhibition, tumour activity, agarose gel electrophoresis, UV‐spectroscopic analysis, DNA, time 120.0 min, Pt     

Biogenic gold nanoparticles for reduction of 4‐nitrophenol to 4‐aminophenol: an eco‐friendly bioremediation

The present study investigated the synthesis of gold nanoparticles (AuNPs) using mangrove plant extract from Avicennia marina as bioreductant for eco‐friendly bioremediation of 4‐nitrophenol (4‐NP). The AuNPs synthesised were confirmed by UV spectrum, transmission electron microscopy (TEM), X‐ray diffraction, Fourier transmission infrared spectroscopy (FTIR), dynamic light scattering (DLS), and zeta potential. The AuNPs were found to be spherical in shape with size ranging from 4 to 13 nm, as evident by TEM and DLS. Further, the AuNPs were encapsulated with sodium alginate in the form of gold nano beads and used as heterogeneous catalyst and degrading agent to reduce 4‐NP. This reduction in 4‐NP into 4‐aminophenol was confirmed by UV and FTIR. The aqueous solution of 4‐NP peaked its absorbance at 320 nm, and shifted to 400 nm, with an intense yellow colour, appeared due to formation of 4‐nitrophenolate ion. After the addition of AuNps, the 4‐NP solution became colourless and peaked at 400 nm and reduced to 290 nm corresponding to the formation of 4‐aminophenol. Hence, the present work suggested the AuNPs as the potent, eco‐friendly bionanocomposite catalyst for bioremediation of 4‐NP.Inspec keywords: gold, nanoparticles, nanobiotechnology, nanofabrication, ultraviolet spectra, transmission electron microscopy, X‐ray diffraction, Fourier transform spectra, infrared spectra, electrokinetic effects, catalysts, nanocomposites, biochemistryOther keywords: biogenic gold nanoparticles, 4‐nitrophenol, 4‐aminophenol, eco‐friendly bioremediation, mangrove plant extract, Avicennia marina, bioreductant, UV spectrum, transmission electron microscopy, TEM, X‐ray diffraction, Fourier transmission infrared spectroscopy, FTIR, dynamic light scattering, DLS, zeta potential, degrading agent, 4‐nitrophenolate, bionanocomposite catalyst, size 4 nm to 13 nm, wavelength 400 nm, wavelength 290 nm, Au     

An adaptive dynamic combined energy minimization model for few‐view computed tomography reconstruction

Recently, the potential harm of electromagnetic radiation used in computed tomography (CT) scanning has been paid much attention to. This makes the few‐view CT reconstruction become an important issue in medical imaging. In this article, an adaptive dynamic combined energy minimization model is proposed for few‐view CT reconstruction based on the compress sensing theory. The L2 energy of the image gradient and the total variation (TV) energy are combined, and the working regions of them are separated adaptively with a dynamic threshold. With the proposed model, the TV model's disadvantageous tendency of uniformly penalize the image gradient irrespective of the underlying image structures is overcome. Numerical experiments of the proposed model are performed with various insufficient data problems in fan‐beam CT and suggest that both the reconstruction speed and quality of the results are generally improved. © 2013 Wiley Periodicals, Inc. Int J Imaging Syst Technol, 23, 44–52, 2013.     

Phyto‐mediated synthesis,biological and catalytic activity studies of gold nanoparticles

In the present study, a phyto‐mediated synthesis of gold nanoparticles (AuNPs) using an isoflavone, Dalspinosin (5,7‐dihydroxy‐6,3′,4′‐trimethoxy isoflavone) isolated from the alcoholic extract of roots of Dalbergia coromandeliana is reported. It is observed that Dalspinosin itself acts both as a reducing and a capping agent in the synthesis of the nanoparticles (NPs). An ultraviolet–visible (UV–Vis) spectral study showed a surface plasmon resonance band at 526 nm confirming the formation of AuNPs. The NPs formed were characterised by UV–Vis spectroscopy, Fourier transform‐infrared spectroscopy, X‐ray diffraction (XRD), high‐resolution transmission electron microscopy (HR‐TEM) with energy‐dispersive x‐ray spectroscopy (EDX) and dynamic light scattering. HR‐TEM analysis showed the synthesised AuNPs were spherical in shape with a size of 7.5 nm. The AuNPs were found to be stable for seven months when tested by in vitro methods showed good antioxidant and anti‐inflammatory activities. They also showed moderate anti‐microbial activities when tested against Gram positive (Staphylococcus aureus and Streptococcus sp), Gram negative bacterial strains (Klebsiella pneumonia and Klebsiella terrigena) and fungal strain (Candida glabrata). The biosynthesised AuNPs showed significant catalytic activity in the reduction of methylene blue with NaBH₄ to leucomethylene blue.Inspec keywords: biomedical materials, catalysis, Fourier transform infrared spectra, gold, light scattering, microorganisms, nanomedicine, nanoparticles, spectrochemical analysis, surface plasmon resonance, transmission electron microscopy, ultraviolet spectra, visible spectra, X‐ray chemical analysis, X‐ray diffractionOther keywords: phyto‐mediated synthesis, biological activity studies, catalytic activity studies, dalspinosin (5,7‐dihydroxy‐6,3′,4′‐trimethoxy isoflavone), alcoholic extract, roots, Dalbergia coromandeliana, ultraviolet‐visible spectral study, surface plasmon resonance band, UV‐Vis spectroscopy, Fourier transform‐infrared spectroscopy, X‐ray diffraction, high‐resolution transmission electron microscopy, EDX analysis, dynamic light scattering, HR‐TEM analysis, antioxidant activities, antiinflammatory activities, antimicrobial activities, Gram positive bacterial strains, Staphylococcus aureus, Streptococcus sp, Gram negative bacterial strains, wavelength 526 nm, size 7.5 nm, time 7 month, Au     

Trastuzumab‐conjugated nanoparticles composed of poly(butylene adipate‐co ‐butylene terephthalate) prepared by electrospraying technique for targeted delivery of docetaxel

Human epidermal growth factor receptor 2 (HER‐2) is overexpressed in 20–30% of human breast cancers, associated with poor prognosis and tumour aggression. The aim of this study was the production of trastuzumab‐targeted Ecoflex nanoparticles (NPs) loaded with docetaxel and in vitro evaluation of their cytotoxicity and cellular uptake. The NPs were manufactured by electrospraying and characterised regarding size, zeta potential, drug loading, and release behaviour. Then their cytotoxicity was evaluated by MTT assay against an HER‐2‐positive cell line, BT‐474, and an HER‐2‐negative cell line, MDA‐MB‐468. The cellular uptake was studied by flow cytometry and fluorescent microscope. The particle size of NPs was in an appropriate range, with relatively high drug entrapment and acceptable release efficiency. The results showed no cytotoxicity for the polymer, but the significant increment of cytotoxicity was observed by treatment with docetaxel‐loaded NPs in both HER‐2‐positive and HER‐2‐negative cell lines, in comparison with the free drug. The trastuzumab‐targeted NPs also significantly enhanced cytotoxicity against BT‐474 cells, compared with non‐targeted NPs.Inspec keywords: cancer, proteins, biomedical materials, nanofabrication, drug delivery systems, cellular biophysics, biological organs, nanomedicine, toxicology, tumours, nanoparticles, biomedical optical imaging, fluorescence, particle sizeOther keywords: human breast cancers, tumour aggression, trastuzumab‐targeted Ecoflex nanoparticles, cellular uptake, zeta potential drug loading, HER‐2‐positive cell line, HER‐2‐negative cell line, MDA‐MB‐468, particle size, trastuzumab‐conjugated nanoparticles, electrospraying technique, human epidermal growth factor receptor, cytotoxicity, nontargeted nanoparticles, butylene adipate‐co‐butylene terephthalate, trastuzumab‐targeted NP, docetaxel‐loaded NP     

Nano‐biosensor based on reduced graphene oxide and gold nanoparticles,for detection of phenylketonuria‐associated DNA mutation

Phenylketonuria (PKU)‐associated DNA mutation in newborn children can be harmful to his health and early detection is the best way to inhibit consequences. A novel electrochemical nano‐biosensor was developed for PKU detection, based on signal amplification using nanomaterials, e.g. gold nanoparticles (AuNPs) decorated on the reduced graphene oxide sheet on the screen‐printed carbon electrode. The fabrication steps were checked by field emission scanning electron microscope imaging as well as cyclic voltammetry analysis. The specific alkanethiol single‐stranded DNA probes were attached by self‐assembly methodology on the AuNPs surface and Oracet blue was used as an intercalating electrochemical label. The results showed the detection limit of 21.3 fM and the dynamic range of 80–1200 fM. Moreover, the selectivity results represented a great specificity of the nano‐biosensor for its specific target DNA oligo versus other non‐specific sequences. The real sample simulation was performed successfully with almost no difference than a synthetic buffer solution environment.Inspec keywords: biosensors, nanosensors, nanoparticles, graphene compounds, gold, nanomedicine, DNA, molecular biophysics, biomedical equipment, electrochemical sensors, electrochemical electrodes, field emission scanning electron microscopy, voltammetry (chemical analysis), self‐assembly, biochemistryOther keywords: reduced graphene oxide, gold nanoparticles, phenylketonuria‐associated DNA mutation, newborn children, electrochemical nanobiosensor, signal amplification, nanomaterials, reduced graphene oxide sheet, screen‐printed carbon electrode, field emission scanning electron microscopy imaging, cyclic voltammetry, alkanethiol single‐stranded DNA probes, self‐assembly methodology, Oracet blue, intercalating electrochemical label, Au‐CO     

Sustained delivery of olanzapine from sunflower oil‐based polyol‐urethane nanoparticles synthesised through a cyclic carbonate ring‐opening reaction

The forefront horizon of biomedical investigations in recent decades is parcelling‐up and delivery of drugs to achieve controlled/targeted release. In this regard, developing green‐based delivery systems for a spatiotemporal controlling therapeutic agent have drawn a lot of attention. A facile route based on cyclic carbonate ring‐opening reaction has been utilised to synthesise a bio‐based polyol‐containing urethane bond [polyol‐urethane (POU)] as a nanoparticulate drug delivery system of olanzapine in order to enhance its bioavailability. After characterisation, the nanoparticles were also estimated for in vitro release, toxicity, and pharmacokinetic studies. As olanzapine has shown poor bioavailability and permeability in the brain, the sustained release of olanzapine from the designed carriers could enhance pharmacokinetic effectiveness. POU in the aqueous solution formed micelles with a hydrophobic core and embedded olanzapine under the influence of its hydrophobic nature. Drug release from the nanoparticles (90 ± 0.43 nm in diameter) indicated a specific pattern with initial burst release, and then a sustained release behaviour (82 ± 3% after 168 h), by the Higuchi‐based release mechanism. Pharmacokinetics assessments of POU‐olanzapine nanoparticles were carried in male Wistar rats through intravenous administration. The obtained results paved a way to introduce the POU as an efficient platform to enhance the bioavailability of olanzapine in therapeutic methods.Inspec keywords: hydrophobicity, nanomedicine, nanofabrication, nanoparticles, drug delivery systems, biomedical materials, polymers, brainOther keywords: cyclic carbonate ring‐opening reaction, nanoparticulate drug delivery system, bioavailability, drug release, initial burst release, Higuchi‐based release mechanism, POU‐olanzapine nanoparticles, sunflower oil‐based polyol‐urethane nanoparticles, forefront horizon, biomedical investigations, green‐based delivery systems, spatiotemporal controlling therapeutic agent, bio‐based polyol‐containing urethane bond, polyol‐urethane, toxicity, pharmacokinetic studies, olanzapine, aqueous solution, micelles, hydrophobic core, Pharmacokinetics, male Wistar rats, brain     

Cross‐linking gold nanoparticles aggregation method based on localised surface plasmon resonance for quantitative detection of miR‐155

MiR‐155 plays a critical role in the formation of cancers and other diseases. In this study, the authors aimed to design and fabricate a biosensor based on cross‐linking gold nanoparticles (AuNPs) aggregation for the detection and quantification of miR‐155. Also, they intended to compare this method with SYBR Green real‐time polymerase chain reaction (PCR). Primers for real‐time PCR, and two thiolated capture probes for biosensor, complementary with miR‐155, were designed. Citrate capped AuNPs (18.7 ± 3.6 nm) were synthesised and thiolated capture probes immobilised to AuNPs. The various concentrations of synthetic miR‐155 were measured by this biosensor and real‐time PCR method. Colorimetric changes were studied, and the calibration curves were plotted. Results showed the detection limit of 10 nM for the fabricated biosensor and real‐time PCR. Also, eye detection using colour showed the weaker detection limit (1 µM), for this biosensor. MiR‐133b as the non‐complementary target could not cause a change in both colour and UV–visible spectrum. The increase in hydrodynamic diameter and negative zeta potential of AuNPs after the addition of probes verified the biosensor accurately fabricated. This fabricated biosensor could detect miR‐155 simpler and faster than previous methods.Inspec keywords: RNA, molecular biophysics, biochemistry, cancer, nanoparticles, gold, aggregation, surface plasmon resonance, molecular configurations, nanosensors, enzymes, calibration, ultraviolet spectra, visible spectra, eye, hydrodynamics, electrokinetic effects, biosensors, nanofabricationOther keywords: cross‐linking gold nanoparticles aggregation method, localised surface plasmon resonance, quantitative detection, cancers, diseases, biosensor, miR‐155 detection, miR‐155 quantification, SYBR green real‐time polymerase chain reaction, thiolated capture probes, citrate capped AuNPs, synthetic miR‐155, real‐time PCR method, colorimetric changes, calibration curves, eye detection, colour, detection limit, MiR‐133b, noncomplementary target, UV‐visible spectrum, hydrodynamic diameter, negative zeta potential, Au     

Fabrication of microcapsules with core‐shell structure for oral delivery of dual drugs and real‐time computed tomography imaging

Although multidrug combinations are an effective therapeutic strategy for serious disease in clinical practice, their therapeutic effect may be reduced because they conflict with each other medicinally in certain cases. Hence, there is an urgent need to develop a single drug carrier for precise multidrug delivery to avoid this interference. A reverse coordination method is reported that fabricates a double‐layer barium sulphate microcapsule (DL@BS MS) for two drugs separately loading simultaneously. In addition, BS nanoclusters were synthesised in situ inside the DL@BS MSs for real‐time computed tomography (CT) imaging. The results showed that the DL@BS MSs with a particle size of approximately 2 mm exhibited a uniform sphere. Because BS nanoclusters have a high X‐ray attenuation coefficient, the retention of DL@BS MSs in the digestive tract could be monitored through CT imaging in real time. More important, the core‐shell structure of DL@BS MSs encapsulating two different drugs could be released in spatiotemporal order in an acidic stomach environment. The as‐synthesis DL@BS MSs with a core‐shell structure and real‐time imaging performance provide an ideal carrier for the oral administration of multiple drugs simultaneously loaded but sequentially released.     

In vitro biological evaluation of anti‐diabetic activity of organic–inorganic hybrid gold nanoparticles

Diabetes mellitus has been considered as a heterogeneous metabolic disorder characterised by complete or relative impairment in the production of insulin by pancreatic β‐cells or insulin resistance. In the present study, propanoic acid, an active biocomponent isolated from Cassia auriculata is employed for the synthesis of propanoic acid functionalised gold nanoparticles (Pa@AuNPs) and its anti‐diabetic activity has been demonstrated in vitro. In vitro cytotoxicity of synthesised Pa@AuNPs was performed in L6 myotubes. The mode of action of Pa@AuNPs exhibiting anti‐diabetic potential was validated by glucose uptake assay in the presence of Genistein (insulin receptor tyrosine kinase inhibitor) and Wortmannin (Phosphatidyl inositide kinase inhibitor). Pa@AuNPs exhibited significant glucose uptake in L6 myotubes with maximum uptake at 50 ng/ml. Assays were performed to study the potential of Pa@AuNPs in the inhibition of protein‐tyrosine phosphatase 1B, α‐glucosidases, and α‐amylase activity.Inspec keywords: molecular biophysics, biomedical materials, sugar, enzymes, nanofabrication, gold, patient treatment, organic‐inorganic hybrid materials, biochemistry, diseases, cellular biophysics, nanoparticles, toxicology, nanomedicineOther keywords: glucose uptake assay, α‐amylase activity, organic–inorganic hybrid gold nanoparticles, diabetes mellitus, heterogeneous metabolic disorder, pancreatic β‐cells, insulin resistance, propanoic acid, antidiabetic potential, antidiabetic activity, in vitro cytotoxicity, L6 myotubes, Genistein, IRTK inhibitor, Wortmannin, P13K inhibitor, protein‐tyrosine phosphatase 1B, α‐glucosidases, Cassia auriculata, Au     

Gentamicin‐gold nanoparticles conjugate: a contrast agent for X‐ray imaging of infectious foci due to Staphylococcus aureus

There is no optimal imaging method for the detection of unknown infectious foci in some diseases. This study introduces a novel method in X‐ray imaging of infection foci due to Staphylococcus aureus by developing a contrast agent based on gold nanoparticles (GNPs). GNPs in spherical shape were synthesised by the reduction of tetrachloroauric acid with sodium citrate. Then gentamicin was bound directly to citrate functionalised GNPs and the complex was stabilised by polyethylene glycol. The interaction of gentamicin with GNPs was confirmed by ultraviolet–visible and Fourier transform infrared spectroscopies. The stability of complex was studied in human blood up to 6 h. The stability of conjugate was found to be high in human blood with no aggregation. The biodistribution study showed localisation of gentamicin–GNPs conjugate at the site of Staphylococcal infection. The infection site was properly visualised in X‐ray images in mouse model using the gentamicin–GNPs conjugate as a contrast agent. The results demonstrated that one may consider the potential of new nanodrug as a contrast agent for X‐ray imaging of infection foci in human beings which needs more investigations.Inspec keywords: drugs, nanomedicine, nanoparticles, nanofabrication, diagnostic radiography, microorganisms, diseases, polymers, ultraviolet spectra, visible spectra, Fourier transform infrared spectra, goldOther keywords: gentamicin‐gold nanoparticle conjugate, contrast agent, X‐ray imaging, Staphylococcus aureus, disease, tetrachloroauric acid reduction, sodium citrate, polyethylene glycol, ultraviolet‐visible spectroscopy, Fourier transform infrared spectroscopy, human blood, Staphylococcal infection, X‐ray images, murine model, nanodrug     

5 Fluorouracil‐loaded biosynthesised gold nanoparticles for the in vitro treatment of human pancreatic cancer cell

In this study, green synthesis of gold nanoparticles (AuNPs) was performed by a sunlight irradiation method using the Borassus flabellifer fruit extract as a reducing agent. 5‐Fluorouracil (5‐FU)‐loaded GG capped AuNPs (5FU‐G‐AuNPs) was prepared. The nanoparticles was further characterised by UV‐visible spectra, particle size analysis, zeta potential, SAED, HRTEM, and XRD. The MTT assay results showed the suitability 5‐FU‐G‐AuNPs. In this study, 5‐FU‐G‐AuNPs exhibited potential cytotoxic and apoptotic effects on (MiaPaCa‐2) cell line.Inspec keywords: gold, biochemistry, X‐ray diffraction, nanofabrication, biomedical materials, transmission electron microscopy, toxicology, electrokinetic effects, particle size, nanoparticles, cancer, visible spectra, cellular biophysics, ultraviolet spectra, nanomedicine, patient treatment, organic compoundsOther keywords: 5FU‐G‐AuNPs, suitability 5‐FU‐G‐AuNPs, human pancreatic cancer cell, green synthesis, sunlight irradiation method, 5‐Fluorouracil‐loaded GG, in vitro treatment, 5 fluorouracil‐loaded biosynthesised gold nanoparticles, borassus flabellifer fruit extract, reducing agent, UV‐visible spectra, particle size analysis, zeta potential, SAED, HRTEM, XRD, MTT assay, apoptotic effects, cytotoxic effects, MiaPaCa‐2 cell line, Au     

Assessment of in‐vivo biocompatibility evaluation of phytogenic gold nanoparticles on Wistar albino male rats

Nanomedicine is an interdisciplinary approach that involves toxicology and other medicinal applications. Gold nanoparticles (AuNPs) may serve as a promising model to address the size and shape‐dependent biological response because they show good biocompatibility. This study is to prepare phytosynthesis AuNPs from ten different Cassia sp. Among them, the aqueous leaf extract of C. roxburghii produced greater efficient and stable AuNPs. The AuNPs were optimised for different physicochemical conditions. Highly stable AuNPs were synthesised at pH 7.0, 37°C, 1.0 ml of C. roxburghii leaf extract and 1.0 mM concentration of HAuCl₄ with the particle size of ∼50 nm and these AuNPs were stable up to 12 months. To determine the safety profile of AuNPs in‐vivo, the nanoparticles were injected intravenously into male Wistar albino rats in varying dosages. The authors noticed no significant difference in body weights, haematological and biochemical parameters and the histopathological sections of all vital organs. Highest accumulation was seen in spleen and least in brain. The authors’ results show that the AuNPs were biocompatible and did not produce any adverse or abnormalities in‐vivo. The implications of the bioaccumulation of AuNPs need to be further studied to rule out any adverse effects on long‐term exposure.Inspec keywords: blood, nanoparticles, cellular biophysics, pH, nanomedicine, particle size, nanofabrication, gold, biomedical materialsOther keywords: in‐vivo biocompatibility evaluation, phytogenic gold nanoparticles, phytosynthesis AuNPs, physicochemical conditions, Wistar albino male rats, nanomedicine, Cassia sp., aqueous leaf extract, C. roxburghii leaf extract, particle size, bioaccumulation, temperature 37.0 degC, Au     

Determination of the potency of hexyl‐ciprofloxacin molecules that interact with gold nanoparticles in a reversible manner

This work determined the potency of hexyl‐ciprofloxacin molecules that reversibly interact with gold nanoparticles (AuNPs) passivated with 11‐mercaptoundecanoic acid (MUA) on Escherichia coli cells. For this, partition of modified antibiotic between different compartments of the gold colloid was determined using analytical techniques. First, concentration of hexyl‐ciprofloxacin was determined in the continuous phase of the colloid. Subsequently, the colloid was exposed to a volume of organic immiscible solvent and concentration of the transferred molecules was determined in the organic phase. Comparison of the amount of hexyl‐ciprofloxacin in each phase revealed that interaction between molecules and nanoparticles was reversible. Later, this work determined the potency of a population of hexyl‐ciprofloxacin molecules contained in a volume of the colloid, and the potency of other population of molecules that only interact with the continuous phase of the colloid. The absolute difference between these two values was proportional to the potency of a number of molecules that interact with the nanoparticles of the colloid.Inspec keywords: organic compounds, nanoparticles, gold, colloids, microorganisms, molecular biophysics, drug delivery systems, nanomedicineOther keywords: continuous phase, hexyl‐ciprofloxacin molecules, gold nanoparticles, gold colloid, 11‐mercaptoundecanoic acid, Escherichia coli cells, modified antibiotics, RP‐HPLC, organic immiscible solvent, reversible interaction, Au     

CdO nanoparticles,c‐MWCNT nanoparticles and CdO nanoparticles/c‐MWCNT nanocomposite fibres: in vitro assessment of anti‐proliferative and apoptotic studies in HeLa cancer cell line

A simple ultrasonic assisted chemical technique was used to synthesise cadmium oxide (CdO) nanoparticles (NPs) and CdO NPs/c‐Multiwalled carbon nanotube (c‐MWCNT) nanocomposite fibres.To confirm the physio‐chemico properties and to analyse surface morphology of the obtained nanomaterials X‐Ray Diffraction (XRD), Fourier Transform Infrared Spectroscopy (FTIR) and field emission scanning electron microscopy (FESEM) were performed. To evaluate the anti‐cancer property of CdO NPs, c‐MWCNT NPs and CdO NPs/c‐MWCNT nanocomposite fibres, an anti‐proliferative assay test (Methylthiazolyl diphenyl‐ tetrazolium bromide ‐ MTT assay) were performed on HeLa cells which further estimated IC50 value (Least concentration of sample in which nearly 50% of cells remain alive) under in‐vitro conditions. On comparison, CdONPs/c‐MWCNT based system was found to be superior by achieving 52.3% cell viability with its minimal IC50 value of 31.2 μg/ml. Lastly, the CdO NPs based system was taken up for an apoptotic study using DNA fragmentation assay for estimating its ability to cleave the DNA of the HeLa cells into internucleosomal fragments using the agarose gel electrophoresis method. In conclusion, based on our observations, CdO NPs/c‐MWCNT hybrid based system can be further used for the development of efficient drug delivery and therapeutic systems.Inspec keywords: drug delivery systems, electrophoresis, oxidation, toxicology, DNA, nanoparticles, drugs, field emission electron microscopy, scanning electron microscopy, nanofabrication, surface morphology, cancer, X‐ray diffraction, nanomedicine, cellular biophysics, filled polymers, biomedical materials, molecular biophysics, biochemistry, Fourier transform infrared spectra, multi‐wall carbon nanotubesOther keywords: c‐MWCNT nanoparticles, apoptotic study, HeLa cancer cell line, cadmium oxide nanoparticles, c‐MWCNT NPs, anti‐proliferative assay test [methyl thiazolyl diphenyl‐tetrazolium bromide assay], human epithelioid cervix carcinoma cells, live cells, CdO NP‐based system, IC50 concentration, HeLa cell line, cell deaths, CdO‐C