Dimov, Ivan Krastev (2010) Configurable and Up-Scalable Microfluidic Life Science Platform for Cell Based Assays by Gravity Driven Sequential Perfusion and Diffusion. PhD thesis, Dublin City University.
Abstract
Microfluidics has the potential to significantly change the way modern biology is performed, but for this potential to be realized several on-chip integration and operation
challenges have to be addressed. Critical issues are addressed in this work by first demonstrating an integrated microfluidic tmRNA purification and real time nucleic acid
sequence based amplification (NASBA) device. The device is manufactured using soft lithography and a unique silica bead immobilization method for the nucleic acid micro
purification column. The integrated device produced a pathogen-specific response in < 3 min from the chip-purified RNA. Further enhancements in the device design and operation that allow the on-chip integration of mammalian cell handling and culturing produced a novel integrated NASBA array. This system demonstrated for the first time that it is possible to combine on a single micro-device cell culture and real time NASBA. In order to expand the cell based assay capabilities of the integrated NASBA array and simplify the device operation novel hydrodynamics and cell sedimentation within trench structures and gravity driven sequential perfusion and diffusion mechanisms were developed. These mechanisms were characterized and implemented within an iCell array device. iCell array can completely integrate cell based assays with bio-analytical read-out. The device is highly scalable and can enable the configurable on-chip integration of procedures such as adherent and non-adherent cell-culture, cellstimulation, cell-lysis, cell-fixing, protein-immunoassays, bright field and fluorescent microscopic monitoring, and real time detection of nucleic acid amplification. The device uses on-board gravity driven flow control which makes it simple and economical to operate with dilute samples (down to 5 cells per reaction), low reagent volumes (50 nL per reaction), highly efficient cell capture (100% capture rates) and single cell protein and gene expression sensitivity. The key results from this work demonstrate a novel technology for versatile, fully integrated microfluidic array platforms. By multiplexing this integrated functionality, the device can be used from routine applications in a biology laboratory to high content screenings.
Metadata
Item Type: | Thesis (PhD) |
---|---|
Date of Award: | 29 March 2010 |
Refereed: | No |
Supervisor(s): | Ducrée, Jens and Lee, Luke |
Uncontrolled Keywords: | microfluidics; lab-on-a-chip; µTAS; lab-in-a-trench; cell handling |
Subjects: | Biological Sciences > Biotechnology Physical Sciences > Analytical chemistry Biological Sciences > Biochemistry Physical Sciences > Nanotechnology Biological Sciences > Immunology Biological Sciences > Cell biology Biological Sciences > Molecular biology Physical Sciences > Detectors Medical Sciences > Cancer Physical Sciences > Chemistry Biological Sciences > Biosensors |
DCU Faculties and Centres: | Research Initiatives and Centres > Biomedical Diagnostics Institute (BDI) DCU Faculties and Schools > Faculty of Science and Health > School of Physical Sciences |
Use License: | This item is licensed under a Creative Commons Attribution-NonCommercial-No Derivative Works 3.0 License. View License |
Funders: | SFI |
ID Code: | 15334 |
Deposited On: | 05 Apr 2011 10:01 by Prof. Jens Ducree . Last Modified 19 Jul 2018 14:50 |
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