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Dive into the research topics where Silvija Abele is active.

Publication


Featured researches published by Silvija Abele.


Analyst | 2008

UV-LED photopolymerised monoliths

Silvija Abele; Fu-Qiang Nie; František Foret; Brett Paull; Mirek Macka

For the first time photopolymerisation of polymer monoliths has been realised with UV-light emitting diodes (LEDs) as light source and demonstrated with polymethacrylate monoliths created in fused silica capillaries and plastic chips.


Journal of Chromatography A | 2011

Polymerisation and surface modification of methacrylate monoliths in polyimide channels and polyimide coated capillaries using 660 nm light emitting diodes

Zarah Walsh; Paul A. Levkin; Silvija Abele; Silvia Scarmagnani; Dominik Heger; Petr Klán; Dermot Diamond; Brett Paull; Frantisek Svec; Miroslav Macka

An investigation into the preparation of monolithic separation media utilising a cyanine dye sensitiser/triphenylbutylborate/N-methoxy-4-phenylpyridinium tetrafluoroborate initiating system activated by 660 nm light emitting diodes is reported. The work demonstrates multiple uses of red-light initiated polymerisation in the preparation of monolithic stationary phases within polyimide and polyimide coated channels and the modification of monolithic materials with molecules which absorb strongly in the UV region. This initiator complex was used to synthesise poly(butyl methacrylate-co-ethylene dimethacrylate) and poly(methyl methacrylate-co-ethylene dimethacrylate) monolithic stationary phases in polyimide coated fused silica capillaries of varying internal diameters, as well as within polyimide micro-fluidic chips. The repeatability of the preparation procedure and resultant monolithic structure was demonstrated with a batch of poly(butyl methacrylate-co-ethylene dimethacrylate) monoliths in 100 μm i.d. polyimide coated fused silica capillary, which were applied to the separation of a model protein mixture (ribonuclease A, cytochrome C, myoglobin and ovalbumin). Taking an average from 12 chromatograms originating from each batch, the maximum relative standard deviation of the retention factor (k) for the protein separations was recorded as 0.53%, the maximum variance for the selectivity factor (α) was 0.40% while the maximum relative standard deviation in peak resolution was 8.72%. All maxima were recorded for the Ribonuclease A/Cytochrome C peaks. Scanning electron microscopy confirmed the success of experiments in which poly(butyl methacrylate-co-ethylene dimethacrylate) monoliths were prepared using the same initiation approach in capillary and micro-fluidic chips, respectively. The initiating system was also applied to the photo-initiated grafting of a chromophoric monomer onto poly(butyl methacrylate-co-ethylene dimethacrylate) monoliths within poly(tetrafluoroethylene) coated fused silica capillaries.


Analytical Chemistry | 2009

Development of Microfluidic Chips for Heterogeneous Receptor−Ligand Interaction Studies

Mark Goldberg; Roger C. Lo; Silvija Abele; Miroslav Macka; Frank A. Gomez

A simple microfluidic-based technique to quantitate the binding affinity between the glycopeptide antibiotics teicoplanin from Actinoplanes teicomyceticus and vancomycin from Streptomyces orientalis and 5-carboxyfluorescein-D-Ala-D-Ala-D-Ala (5-FAM-(DA)(3)) is described. In this work, (3-aminopropyl)triethoxysilane is used to modify the surfaces of a series of microchannels, and each channel is subsequently exposed to a solution of antibiotic for a few minutes. The antibiotic is retained after washing through electrostatic interactions, and the series of channels are subsequently exposed to an increasing concentration of 5-FAM-(DA)(3) followed by washing to exclude any nonspecific binding. The extent of fluorescence is quantified using a microscope fitted with a CCD camera. The binding constants for the interaction of teicoplanin and vancomycin with the fluorescent peptide were determined to be 6.03 +/- 0.97 x 10(4) and 4.93 +/- 1.13 x 10(4) M(-1), respectively, in good agreement with previous data. The ease of quantifying the extent of interaction in this microchip technique may prove powerful for exploration of a myriad of receptor-ligand pairs.


Analyst | 2010

Evanescent wave-initiated photopolymerisation as a new way to create monolithic open-tubular capillary columns: use as enzymatic microreactor for on-line protein digestion

Silvija Abele; Petr Smejkal; Oksana Yavorska; František Foret; Mirek Macka


Analyst | 2009

Deep-UV-LEDs in photometric detection: A 255 nm LED on-capillary detector in capillary electrophoresis

Lenka Krčmová; Anna Stjernlof; Sebastien Mehlen; Peter C. Hauser; Silvija Abele; Brett Paull; Mirek Macka


Chemical Communications | 2008

Photoinitiated polymerisation of monolithic stationary phases in polyimide coated capillaries using visible region LEDs

Zarah Walsh; Silvija Abele; Brian Lawless; Dominik Heger; Petr Klán; Michael C. Breadmore; Brett Paull; Mirek Macka


Sensors and Actuators B-chemical | 2010

Photochromic spiropyran monolithic polymers: Molecular photo-controllable electroosmotic pumps for micro-fluidic devices

Zarah Walsh; Silvia Scarmagnani; Fernando Benito-Lopez; Silvija Abele; Fu-Qiang Nie; Conor Slater; Robert Byrne; Dermot Diamond; Brett Paull; Mirek Macka


Archive | 2007

The Potential of Capillary Electrophoresis for the Analysis of Yeast Extracts

Mark Loane; Eva Mendel; Silvija Abele; Brett Paull; Mirek Macka


Archive | 2009

Use of light emitting diodes in the visible region to initiate polymerisation leading to monolithic stationary phases

Zarah Walsh; Dominik Heger; Silvija Abele; Petr Klán; Brett Paull; Pavel A. Levkin; Frantisek Svec; Mirek Macka


Archive | 2008

Method for metal coated porous scaffold material

Mirek Macka; Brett Paull; Marco Grundmann; Zarah Walsh; Silvija Abele

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Brett Paull

University of Tasmania

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Mirek Macka

University of Tasmania

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Zarah Walsh

Dublin City University

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