Single-cycle kinetics for QCM biosensors for high throughput nanoparticle characterization application

Boström, Fredrik

January 2016

Characterizing nanoparticles to be able to understand how they functions in the body is important for development of drugs. Furthermore with increasing number of nanoparticle product the nanotoxicity of nanoparticles is important to understand. This report is a part of the EU-project Nanoclassifier which purpose is to “develop a cost effective, high throughput screening platform for characterization of the bionanointerface and its cell-binding partners”. Single-cycle kinetic was used to determine the number of binding epitopes on polystyrene nanoparticle with transferrin corona. The number of available epitopes describes how active the Nanoparticle will be in the body. For this purpose Single-cycle kinetic methodology was successfully used on nanoparticles. Single-cycle kinetic methodology has great potential to become the standard method for high throughput nanoparticle epitope characterization.

Single-cycle kinetics

kinetic titration

kinetics

image analysis

cell counting

nanoparticles

protein corona

method development

Multi-cycle kinetics

QCM biosensor

Method development and Validation for the determination of selected Polycyclic Aromatic Hydrocarbons (PAHs) in water by Solid Phase Extraction and High Performance Liquid Chromatography

Xoliswa, Madlanga

12 February 2014

Polycyclic Aromatic Hydrocarbons (PAHs) are one of the pollutants in the environment. They are organic compounds that consist of more than one aromatic ring (Kanchanamayoon & Tatrahun 2008). Due to less information forthcoming regarding the levels of PAHs in Vaal area, this study is to evaluate the levels of PAHs in the rivers around Vaal Triangle. Three river sites such as Vaal, Barrage and Klip Rivers were selected to investigate the concentration of polycyclic aromatic hydrocarbons in water. Validation of an analytical method is the process by which it is established by laboratory studies, that the performance characteristics of the method meet the requirements for the intended analytical application. (Stockl et al 2009). The validation parameters tested were, linearity detection limit of quantitation, sensitivity, accuracy, specificity, selectivity, robustness and ruggedness. PAHs can be determined using High Performance Liquid Chromatography (HPLC) which is a technique for separation, identification and quantification of components in a mixture. The following ten compounds were identified and quantified with a HPLC: naphthalene, acenaphthylene, phenanthrene, anthracene, fluoranthene, benzo(b)fluoranthene, benzo(k)fluoranthene, benzo(a)pyrene, dibenzo(a,h) anthracene and indeno(1,2,3-cd)pyrene. The linear calibration ranges from 0.1-5ppm.The linearity ranges between 0.9993-0.9999.Three reversed sorbent phases (Strata-X, MFC18 and C18) were tested for PAH retention efficiency. An optimised reverse solid phase extraction (SPE) method was used after conditioning the sorbent to extract and collect compounds of polycyclic aromatic hydrocarbons (PAHs) in river water samples. LC18 sorbent showed good recoveries after extracting PAHs standard mixture of 1 mg/l. The best performing eluting solvent was acetonitrile and very good percentage recoveries that ranged from 70% to over 100 % were obtained for eight compounds. Poor recoveries were also obtained for phenanthrene (61%) and benzo(b)fluoranthene (48%). The standard deviation ranged from 0.01 to 0.05 and the detection limits ranging from 0.01 – 0.17 mg/l were obtained. Average concentration ranges of PAHs identified within the study area were: phenanthrene (0.02 – 0.42 mg/l); anthracene (0.37 – 0.39 mg/l), fluoranthene (0.11 – 0.15 mg/l); benzo(b)fluoranthene (0.09 mg/l) and indeno(1,2,3-cd)pyrene (0.26 mg/l). However, naphthalene, acenaphthylene, benzo(k)fluoranthene, benzo(a)pyrene and dibenzo(a,h)anthracene were not detected.

Stratégies chromatographiques en phase liquide et supercritique pour l'analyse de candidats médicaments / Liquid and supercritical chromatographic strategies for analysis of drug candidates

Lemasson, Elise

18 January 2018

Le profilage d’impuretés de candidats médicaments est une préoccupation majeure des industries pharmaceutiques. L’identification et la quantification des impuretés doivent être strictement contrôlées pour assurer l’efficacité et la toxicité limitée du principe actif. Il est donc nécessaire de disposer de méthodes analytiques performantes afin de s’assurer que l’ensemble des impuretés est identifié. L’HPLC phase inverse sur phase C18 reste aujourd’hui la méthode de choix pour cette tâche. Cependant, il arrive que cette méthode échoue, notamment lorsque le principe actif n’est pas suffisamment retenu sur la colonne ou que les impuretés ne sont pas parfaitement séparées du composé principal. Il est alors essentiel de pouvoir se tourner vers des méthodes analytiques alternatives et complémentaires.Ce travail de recherche traite du développement et de l’évaluation de méthodes analytiques alternatives à l’HPLC phase inverse sur phase C18 pour le profilage d’impuretés de principes actifs pharmaceutiques. L’HPLC phase inverse sur d’autres phases stationnaires, l’HPLC mixed-mode ainsi que la SFC ont été explorées et leurs performances chromatographiques comparées. La comparaison et l’étude des différentes méthodes ont permis de proposer une stratégie d’analyse du candidat médicament. / Impurity profiling of drug candidates is a significant concern of pharmaceutical industries. The identification and quantification of impurities must be strictly controlled to ensure the efficacy and limited toxicity of the active ingredient. It is therefore necessary to have efficient analytical methods to ensure that all impurities are identified. Today, reversed-phase HPLC with C18 column remains the method of choice for this task. However, this method sometimes fails, particularly when the active pharmaceutical ingredient is not sufficiently retained on the column or when the impurities are not resolved from the main compound. It is therefore essential to turn to alternative and complementary analytical methods.This work deals with the development and evaluation of alternative analytical methods to reversed-phase HPLC on C18 phase for impurity profiling of pharmaceuticals. Reversed-phase HPLC on other stationary phases, mixed-mode HPLC as well as SFC were explored and their chromatographic performances compared. The comparison and the study of the different methods allowed proposing a strategy of analysis of the drug candidate.

Développement de méthodes

HPLC

Mixed-mode

SFC

Candidats médicaments

Method development

HPLC

Mixed-mode

SFC

Drug candidates

547

The synthesis, analysis and characterisation of piperazine based drugs

Kuleya, Chipo

January 2014

This study developed a GC-MS method for the simultaneous detection of piperazines and congeners in street samples of amphetamine type stimulants. This research investigated the clandestine routes of synthesis and chemical profiles of phenylpiperazines, represented by 1- (4-fluorophenyl)piperazine (4-FPP) and 1-(3-trifluoromethylphenyl)piperazine (3-TFMPP). These drugs are part of the increasingly prevalent illicit new psychoactive substances. The presence of (2, 3, 4) FPP and (2, 3, 4) TFMPP positional isomers has been identified by other researchers as a limitation due to their similar chemical profiles. The method was optimized and confirmed as compliant with the International Conference on Harmonisation and the Center for Drug Evaluation and Research guidelines on validation. 4- FPP and 3-TFMPP were synthesised using potential routes for clandestine laboratories. Simple extraction and analysis of 11 street samples was conducted using the method developed. Furthermore, the stability of 22 drugs during analysis was investigated. Limits of detection were in the range 5 – 1.95ng/mL free base on column. The synthesised samples were identified as 4-FPP and 3-TFMPP. Several impurities were observed in the synthesised samples, which were identified and categorised as residual reactants, isomers of 4-FPP and of 3-TFMPP and by-products of synthesis. The percentage yields of the synthesised samples obtained were up to 82.4% 4-FPP and 78.7% 3-TFMPP. The street samples were found to contain MDMA, 3-TFMPP, BZP, caffeine, ephedrine and other impurities. The analytical method simultaneously separates 19 of the most common drugs found in piperazine samples and achieves for the first time the GC-MS separation of (i) 2-FPP, 3-FPP and 4-FPP and (ii) 2-TFMPP, 3-TFMPP and 4-TFMPP at the same time from a sample matrix containing all the 19 compounds. This method provides operational laboratories with a more effective method for the chemical characterisation of street samples of piperazines and also provides novel stability data.

615.7

Method development for investigation of real effects on flow around vanes

Mårtensson, Jonathan

January 2010

<p>In the development of turbo machinery components it's desirable to not spend more time than necessary when setting up aero-thermal calculations to investigate uncertainties in the design. This report aims to describe general thoughts used in the development of an ICEM-mesh script and the possible configurations in the script file which enables the user to build mesh-grids with/without clearance gap at the hub and/or shroud for different blade geometries. It also aims to illustrate the performance analysis made on the Vinci LH2 turbine, a next generation upper stage engine to the Ariane 5 rocket, in which the effect of the tip gap size on the efficiency has been studied.</p><p>The calculations made have shown good agreement with experimental data. The efficiency loss due to the mixing of fluid where leakage flow passes the tip gap, which results in growth of a strong vortex, and the fluid passing the blade tip, with almost no work extracted from it, has shown a quite linear efficiency dependence depending on the tip gap size.</p>

Master's Thesis

Method Development

Real effects

Turbomachinery

Turbine Flow

Secondary Flow

ICEM

Block Mesh Topology

Tip Gap

Fluid mechanics

Strömningsmekanik

The Development of Novel Protein Topology Mapping Strategies using Crosslinking, Cyanogen Bromide Cleavage, and Mass Spectrometry

Weerasekera, Rasanjala Kumari

11 January 2012

Advances in protein topology mapping methods are urgently needed to complement the wealth of interactome data that is presently being generated at a rapid pace. Chemical crosslinking followed by mass spectrometry (MS) has evolved over the last decade as an attractive method for protein topology and interface mapping, and holds great promise as a counterpart to modern interactome studies in the field of proteomics. Furthermore, stabilization of proteins and protein complexes with crosslinking offers many advantages over high-resolution structural mapping methods, including the ability to study protein topologies in vivo. The reliance on direct detection of crosslinked peptides, however, continues to pose challenges to protein topology and interface mapping with chemical crosslinking plus MS. The present body of work aimed to develop a novel generic methodology that utilizes chemical crosslinking, cyanogen bromide (CNBr) cleavage and MS for the low-resolution mapping of protein topologies and interfaces. Through such low-resolution mapping of crosslinked regions, this novel strategy overcomes limitations associated with the direct detection of crosslinked peptides. Following optimization of various steps, the present method was validated with the bacterial DNA-directed RNA polymerase core complex and was subsequently applied to probe the tetrameric assembly of yeast Skp1p-Cdc4p heterodimers. Further improvements were made through the enrichment of crosslinked CNBr-cleaved protein fragments prior to their identification via MS. Two enrichment strategies were developed which depended upon the conjugation of tags to CNBr-cleaved peptide C-termini followed by either tandem affinity purification or tandem reversed-phase HPLC purification. These strategies were successfully applied for the efficient purification of disulfide-linked peptides from peptide mixtures. It is expected that the potential to achieve sensitive mapping of topologies and interfaces of multi-subunit protein complexes in vivo, in combination with further enhancements to permit studies on complex protein samples, will extend the utility of this method to complement large-scale interactome studies.

protein structure

mass spectrometry

chemical crosslinking

interface mapping

proteomics

protein topology mapping

cyanogen bromide

interactome

method development

HPLC

0307

Analysis of Biodiesel Quality Using Reversed Phase High-Performance Liquid Chromatography

Murphy, Kellyann M

13 May 2012

The alternative fuel biodiesel is produced from the transesterification of vegetable oils or animal fat to fatty acid methyl esters. Pomona has a reactor on campus that can be used to run this reaction and produce biodiesel. The use of biodiesel has been found to lower air pollutant and greenhouse gas emissions, but can be potentially harmful to the engines if it contains impurities. This paper proposes a method using high-performance liquid chromatography to test the quality of biodiesel. This method utilizes instrumentation and materials that are available in Pomona College's Chemistry Department, requires very little sample preparation, and is relatively safe, as long as general lab safety practices are followed. This method can also be used to optimize the procedure used to make the biodiesel. An optimized production procedure and a test method to assess the final product will ensure high quality fuel that can be used with confidence in diesel engines. This will likely add strength to proposals to increase the use of the on-campus reactor and produce biodiesel for campus grounds equipment from waste vegetable oil.

biodiesel

hplc

liquid chromatography

method development

chemistry

Analytical Chemistry

Environmental Chemistry

Laboratory and Basic Science Research

Other Environmental Sciences

The Development of Novel Protein Topology Mapping Strategies using Crosslinking, Cyanogen Bromide Cleavage, and Mass Spectrometry

Weerasekera, Rasanjala Kumari

11 January 2012

Advances in protein topology mapping methods are urgently needed to complement the wealth of interactome data that is presently being generated at a rapid pace. Chemical crosslinking followed by mass spectrometry (MS) has evolved over the last decade as an attractive method for protein topology and interface mapping, and holds great promise as a counterpart to modern interactome studies in the field of proteomics. Furthermore, stabilization of proteins and protein complexes with crosslinking offers many advantages over high-resolution structural mapping methods, including the ability to study protein topologies in vivo. The reliance on direct detection of crosslinked peptides, however, continues to pose challenges to protein topology and interface mapping with chemical crosslinking plus MS. The present body of work aimed to develop a novel generic methodology that utilizes chemical crosslinking, cyanogen bromide (CNBr) cleavage and MS for the low-resolution mapping of protein topologies and interfaces. Through such low-resolution mapping of crosslinked regions, this novel strategy overcomes limitations associated with the direct detection of crosslinked peptides. Following optimization of various steps, the present method was validated with the bacterial DNA-directed RNA polymerase core complex and was subsequently applied to probe the tetrameric assembly of yeast Skp1p-Cdc4p heterodimers. Further improvements were made through the enrichment of crosslinked CNBr-cleaved protein fragments prior to their identification via MS. Two enrichment strategies were developed which depended upon the conjugation of tags to CNBr-cleaved peptide C-termini followed by either tandem affinity purification or tandem reversed-phase HPLC purification. These strategies were successfully applied for the efficient purification of disulfide-linked peptides from peptide mixtures. It is expected that the potential to achieve sensitive mapping of topologies and interfaces of multi-subunit protein complexes in vivo, in combination with further enhancements to permit studies on complex protein samples, will extend the utility of this method to complement large-scale interactome studies.

protein structure

mass spectrometry

chemical crosslinking

interface mapping

proteomics

protein topology mapping

cyanogen bromide

interactome

method development

HPLC

0307

Method development for investigation of real effects on flow around vanes

Mårtensson, Jonathan

January 2010

In the development of turbo machinery components it's desirable to not spend more time than necessary when setting up aero-thermal calculations to investigate uncertainties in the design. This report aims to describe general thoughts used in the development of an ICEM-mesh script and the possible configurations in the script file which enables the user to build mesh-grids with/without clearance gap at the hub and/or shroud for different blade geometries. It also aims to illustrate the performance analysis made on the Vinci LH2 turbine, a next generation upper stage engine to the Ariane 5 rocket, in which the effect of the tip gap size on the efficiency has been studied. The calculations made have shown good agreement with experimental data. The efficiency loss due to the mixing of fluid where leakage flow passes the tip gap, which results in growth of a strong vortex, and the fluid passing the blade tip, with almost no work extracted from it, has shown a quite linear efficiency dependence depending on the tip gap size.

Master's Thesis

Method Development

Real effects

Turbomachinery

Turbine Flow

Secondary Flow

ICEM

Block Mesh Topology

Tip Gap

Fluid mechanics

Strömningsmekanik

Improved analytical methods for perfluoroalkyl acids (PFAAs) and their precursors – a focus on human dietary exposure

Ullah, Shahid

January 2013

Per- and polyfluoroalkyl substances are a large group of global environmental contaminants. They can be divided into two sub-groups, 1) perfluoroalkyl acids (PFAAs) and 2) so called precursors, i.e. compounds that can potentially be transformed to form PFAAs. PFAAs are today ubiquitous in wildlife and humans. Food and drinking water are assumed to be the dominant human exposure pathways for PFAAs. The main aim of this doctoral thesis was to develop highly sensitive and fully validated analytical methods for the determination of a range of PFAAs and selected precursors in dietary samples. The methods were based on liquid chromatography coupled to mass spectrometry. Samples were extracted by solvent extraction followed by a cleanup step employing solid phase extraction. The cleanup step could at the same time be used as a fractionation of ionic PFAAs and neutral precursors. Paper I and II describe the development of methods for simultaneous analysis of three groups of PFAAs including perfluoroalkyl phosphonic acids (PFPAs) in drinking water and food. Methyl piperidine was used as ion pairing agent, leading to highly sensitive analysis of PFPAs. A first screening of tap water samples and different food items revealed that human dietary exposure to PFPAs in Europe is currently not of concern. A novel method for simultaneous analysis of perfluoroalkyl carboxylic acids (PFCAs) and polyfluoroalkyl phosphate esters (PAPs) in food and packaging materials is described in paper III. Targeted food samples and their packaging were analyzed. The results showed that PAPs may contribute to human exposure to PFCAs. In paper IV temporal trends (1991-2011) of perfluorooctane sulfonic acid (PFOS) and its precursors in herring were investigated. Rapidly decreasing trends were found for precursors, whereas PFOS did not show a significant change over time. Precursors in fish may have played an important role for human exposure to PFOS in the 1990s but are probably negligible today. / <p>At the time of the doctoral defense, the following paper was unpublished and had a status as follows: Paper 4: Manuscript.</p> / PERFOOD project (KBBE-227525)

Environmental Science

PFASs

PFAAs

PFOA

PFOS

Precursor

FOSA

PAPs

Method development

LC-MS

SPE

Dietary sample

Drinking water

Human exposure