Radiocarbon Determination of the Carbon-Based Biomass Blending Ratio by Analysing Flue Gas Emitted from Coupled Combustion

The determination of carbon-based biomass blending ratio was a prerequisite for the large-scale development of the coupled combustion technology of biomass and coal. In this study, the experimental system of the radiocarbon method to detect the carbon-based biomass blending ratio by analyzing the flue gases produced during coupled combustion was built, and the calculation model of the carbon-based biomass blending ratio was proposed, and the accuracy and precision of the radiocarbon method were evaluated. The results showed that there was a good linear relationship between the 14C concentration of CO2 samples and biogenic fractions in flue gas. The application of the new calculation model improved the accuracy of the 14C determination method, and the relative error increased as the carbon-based biomass blending ratio decreased in the 14C method: the minimum relative error of the carbon-based biomass blending ratio with carbon-based assay was 15.16%,12.21%, 9.61%, 7.96% and 3.13% when considering coal and air simultaneously in AMS analysis. This further validated the 14C determination method as an accurate method for identifying the carbon-based biomass blending ratio in biomass and coal coupled combustion.

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Simplified isoelectric focusing/immunoblotting determination of apoprotein E phenotype

Clinical Chemistry ◽

10.1093/clinchem/40.1.11 ◽

1994 ◽

Vol 40 (1) ◽

pp. 11-13 ◽

Cited By ~ 68

Author(s):

S Kataoka ◽

M Paidi ◽

B V Howard

Keyword(s):

Isoelectric Focusing ◽

Large Scale ◽

Population Studies ◽

Accurate Method ◽

Tween 20 ◽

Neuraminidase Treatment ◽

Require Time ◽

Scale Population ◽

Apoprotein E

Abstract We developed a rapid, accurate method for phenotyping apoprotein E that can be used for large-scale population studies. In this method, adapted from the method of Kamboh et al. (J Lipid Res 1988;29:1535-43), 10-microL plasma samples are incubated with dithiothreitol and Tween-20 for 15 min and then applied to 5% polyacrylamide gels containing ampholyte (pH 4.5-8) and urea (3 mol/L). After 2 h of isoelectric focusing, the apoprotein E bands are made visible by immunoblotting. Utilizing whole plasma, this method does not require time-consuming ultracentrifugation, delipidation of samples, or dialysis. Small amounts of plasma are required, electrofocusing time is short, and as many as 160 samples can be processed per day. Identification of phenotype is easily accomplished by noting the location and number of protein bands instead of their intensity. Because identification of phenotype is not affected by sialylation, neuraminidase treatment is not necessary. Agreement in identification of 301 individuals from blinded duplicates was 96%, and there was 98% concordance of results for 431 samples that had undergone genetic typing. This method is thus well suited for large-scale population studies.

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Large-scale Motion of Solar Filaments

International Astronomical Union Colloquium ◽

10.1017/s0252921100064502 ◽

2000 ◽

Vol 179 ◽

pp. 205-208

Author(s):

Pavel Ambrož ◽

Alfred Schroll

Keyword(s):

Magnetic Flux ◽

Proper Motion ◽

Time Scale ◽

Large Scale ◽

Accuracy Of Measurements ◽

Solar Filaments ◽

General Movement ◽

Scale Motion ◽

Velocity Scatter

AbstractPrecise measurements of heliographic position of solar filaments were used for determination of the proper motion of solar filaments on the time-scale of days. The filaments have a tendency to make a shaking or waving of the external structure and to make a general movement of whole filament body, coinciding with the transport of the magnetic flux in the photosphere. The velocity scatter of individual measured points is about one order higher than the accuracy of measurements.

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Stationary source emissions. Determination of PM10/PM2,5 mass concentration in flue gas. Measurement at higher concentrations by use of virtual impactors

10.3403/30204377u ◽

2015 ◽

Keyword(s):

Flue Gas ◽

Mass Concentration ◽

Stationary Source ◽

Gas Measurement ◽

Virtual Impactors

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Stationary source emissions. Sampling and determination of mercury compounds in flue gas using gold amalgamation trap

10.3403/30349188 ◽

2020 ◽

Keyword(s):

Flue Gas ◽

Mercury Compounds ◽

Stationary Source

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Stationary source emissions � Determination of the mass concentration of carbon monoxide, carbon dioxide and oxygen in flue gas � Performance characteristics of automated measuring systems

10.3403/30354887u ◽

2019 ◽

Keyword(s):

Carbon Dioxide ◽

Carbon Monoxide ◽

Flue Gas ◽

Mass Concentration ◽

Performance Characteristics ◽

Measuring Systems ◽

Stationary Source

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Methods for the Quantification of Salivary Cortisol and of a-amylase in Biosensors and Portable Devices

Revista de Chimie ◽

10.37358/rc.17.12.5994 ◽

2018 ◽

Vol 68 (12) ◽

pp. 2857-2859

Author(s):

Cristina Mihaela Ghiciuc ◽

Andreea Silvana Szalontay ◽

Luminita Radulescu ◽

Sebastian Cozma ◽

Catalina Elena Lupusoru ◽

...

Keyword(s):

Real Time ◽

Medical Practice ◽

Salivary Cortisol ◽

Clinical Studies ◽

Large Scale ◽

Psychological Research ◽

Portable Devices ◽

Salivary Amylase ◽

Specificity And Sensitivity

There is an increasing interest in the analysis of salivary biomarkers for medical practice. The objective of this article was to identify the specificity and sensitivity of quantification methods used in biosensors or portable devices for the determination of salivary cortisol and salivary a-amylase. There are no biosensors and portable devices for salivary amylase and cortisol that are used on a large scale in clinical studies. These devices would be useful in assessing more real-time psychological research in the future.

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Identification of N-Substituted Triazolo-azetidines as Novel Antibacterials using pDualrep2 HTS Platform

Combinatorial Chemistry & High Throughput Screening ◽

10.2174/1386207322666190412165316 ◽

2019 ◽

Vol 22 (5) ◽

pp. 346-354

Author(s):

Yan A. Ivanenkov ◽

Renat S. Yamidanov ◽

Ilya A. Osterman ◽

Petr V. Sergiev ◽

Vladimir A. Aladinskiy ◽

...

Keyword(s):

Antibacterial Activity ◽

Large Scale ◽

Underlying Mechanism ◽

Luciferase Assay ◽

Reporter System ◽

E Coli ◽

Starting Point ◽

High Concentrations ◽

Mic Value

Aim and Objective: Antibiotic resistance is a serious constraint to the development of new effective antibacterials. Therefore, the discovery of the new antibacterials remains one of the main challenges in modern medicinal chemistry. This study was undertaken to identify novel molecules with antibacterial activity. Materials and Methods: Using our unique double-reporter system, in-house large-scale HTS campaign was conducted for the identification of antibacterial potency of small-molecule compounds. The construction allows us to visually assess the underlying mechanism of action. After the initial HTS and rescreen procedure, luciferase assay, C14-test, determination of MIC value and PrestoBlue test were carried out. Results: HTS rounds and rescreen campaign have revealed the antibacterial activity of a series of Nsubstituted triazolo-azetidines and their isosteric derivatives that has not been reported previously. Primary hit-molecule demonstrated a MIC value of 12.5 µg/mL against E. coli Δ tolC with signs of translation blockage and no SOS-response. Translation inhibition (26%, luciferase assay) was achieved at high concentrations up to 160 µg/mL, while no activity was found using C14-test. The compound did not demonstrate cytotoxicity in the PrestoBlue assay against a panel of eukaryotic cells. Within a series of direct structural analogues bearing the same or bioisosteric scaffold, compound 2 was found to have an improved antibacterial potency (MIC=6.25 µg/mL) close to Erythromycin (MIC=2.5-5 µg/mL) against the same strain. In contrast to the parent hit, this compound was more active and selective, and provided a robust IP position. Conclusion: N-substituted triazolo-azetidine scaffold may be used as a versatile starting point for the development of novel active and selective antibacterial compounds.

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Development of an HPLC-UV Method for Quantification of Stattic

Current Pharmaceutical Analysis ◽

10.2174/1573412914666180523092957 ◽

2019 ◽

Vol 15 (6) ◽

pp. 568-573

Author(s):

Soheil Sedaghat ◽

Ommoleila Molavi ◽

Akram Faridi ◽

Ali Shayanfar ◽

Mohammad Reza Rashidi

Keyword(s):

High Performance ◽

Accurate Method ◽

Plasma Samples ◽

Promising Target ◽

Relative Standard ◽

Dimerization Inhibitor ◽

Oncogenic Protein ◽

First Time ◽

Transcription 3

Background: Signal transducer and activator of transcription 3 (STAT3), an oncogenic protein found constitutively active in many types of human malignancies, is considered to be a promising target for cancer therapy. Objective: In this study for the first time, a simple and accurate method has been developed for the determination of a STAT3 dimerization inhibitor called stattic in aqueous and plasma samples. Methods: A reverse-phase high-performance liquid chromatography (RP-HPLC) composed of C18 column as stationary phase, and the mixture of acetonitrile (60%) and water (40%) as mobile phase with a UV detection at 215 nm were applied for quantification of stattic. The developed method was validated by Food and Drug Administration (FDA) guideline. Results: The method provided a linear range between 1-40 and 2.5-40 µg mL-1 for aqueous and plasma samples, respectively, with a correlation coefficient of 0.999. The accuracy (as recovery) of the developed method was found to be between 95-105% for aqueous medium and 85-115% for plasma samples. The precision (as relative standard deviation) for aqueous and plasma samples was less than 6% and 15%, respectively. The sensitivity of the developed method based on FDA guideline was 1 µg mL-1 for aqueous and 2.5 µg mL-1 for plasma samples. Conclusion: These results show that the established method is a fast and accurate quantification for stattic in aqueous and plasma samples.

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Is it necessary to calculate Young’s modulus in AFM nanoindentation experiments regarding biological samples?

Micro and Nanosystems ◽

10.2174/1876402912666200214123734 ◽

2020 ◽

Vol 12 ◽

Author(s):

S.V. Kontomaris ◽

A. Malamou ◽

A. Stylianou

Keyword(s):

Young’S Modulus ◽

Biological Samples ◽

Young's Modulus ◽

Reference Sample ◽

Nonlinear Behavior ◽

Accurate Method ◽

Accurate Solution ◽

Hertz Model ◽

Work Done

Background: The determination of the mechanical properties of biological samples using Atomic Force Microscopy (AFM) at the nanoscale is usually performed using basic models arising from the contact mechanics theory. In particular, the Hertz model is the most frequently used theoretical tool for data processing. However, the Hertz model requires several assumptions such as homogeneous and isotropic samples and indenters with perfectly spherical or conical shapes. As it is widely known, none of these requirements are 100 % fulfilled for the case of indentation experiments at the nanoscale. As a result, significant errors arise in the Young’s modulus calculation. At the same time, an analytical model that could account complexities of soft biomaterials, such as nonlinear behavior, anisotropy, and heterogeneity, may be far-reaching. In addition, this hypothetical model would be ‘too difficult’ to be applied in real clinical activities since it would require very heavy workload and highly specialized personnel. Objective: In this paper a simple solution is provided to the aforementioned dead-end. A new approach is introduced in order to provide a simple and accurate method for the mechanical characterization at the nanoscale. Method: The ratio of the work done by the indenter on the sample of interest to the work done by the indenter on a reference sample is introduced as a new physical quantity that does not require homogeneous, isotropic samples or perfect indenters. Results: The proposed approach, not only provides an accurate solution from a physical perspective but also a simpler solution which does not require activities such as the determination of the cantilever’s spring constant and the dimensions of the AFM tip. Conclusion: The proposed, by this opinion paper, solution aims to provide a significant opportunity to overcome the existing limitations provided by Hertzian mechanics and apply AFM techniques in real clinical activities.

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Synthesis and solvatochromic studies of 2- amino-3-phenolazo1-(4-sulfophenyl)-3-methyi-5-pyrozolone and use it for the determination of trace amount of Nickel (II) in blood samples

International Journal of Bioassays ◽

10.21746/ijbio.2016.10.001 ◽

2016 ◽

Vol 5 (10) ◽

pp. 4920

Author(s):

Amar M. Ali ◽

Hussain. J. Mohammed*

Keyword(s):

Stability Constant ◽

Trace Amount ◽

Benzenesulfonic Acid ◽

Determination Method ◽

Blood Samples ◽

Determination Of Nickel ◽

Normal Human ◽

The Stability ◽

Normal Human Blood

A new, simple, sensitive and rapid spectrophotometric method is proposed for the determination of trace amount of Nickel (II). The method is based on the formation of a 1:2 complex with 4-(4-((2-hydroxy-6-nitrophenyl) diazenyl) -3-methyl-5-oxo-2, 5-dihydro-1H-pyrazol-1-yl) benzenesulfonic acid (2-ANASP) as a new reagent is developed. The complex has a maximum absorption at 516 nm and εmax of 1. 84 X 105 L. mol-1. cm-1. A linear correlation (0. 25 – 4. 0μg. ml-1) was found between absorbance at λmax and concentration. The accuracy and reproducibility of the determination method for various known amounts of Nickel (II) were tested. The results obtained are both precise (RSD was 1. 2 %) and accurate (relative error was 0. 787 %). The effect of diverse ions on the determination of Nickel (II) to investigate the selectivity of the method were also studied. The stability constant of the product was 0. 399 X 106 L. mol-1. The proposed method was successfully applied to the analysis of diabetes blood and normal human blood.

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