| dc.contributor.advisor | Hegner, Martin | |
| dc.contributor.author | Wruck, Florian | |
| dc.date.accessioned | 2024-11-26T14:31:59Z | |
| dc.date.available | 2024-11-26T14:31:59Z | |
| dc.date.issued | 2016 | |
| dc.identifier.citation | Florian Wruck, 'Following translation of individual proteins by single ribosomes in real-time using dual-trap optical tweezers', [thesis], Trinity College (Dublin, Ireland). School of Physics, 2016, pp 215 | |
| dc.identifier.other | THESIS 11008 | |
| dc.description.abstract | Gradient force traps (optical tweezers) have found many applications in physics and the life sciences [1-3] ever since Arthur Ashkin's first description of optical trapping of dielectric particles in liquid [4], Near-infrared (NIR) gradient force traps made it possible to indirectly apply pN-scale forces on large molecules, nm-sized motor enzymes and ribozymes (e.g. ribosomes), internal parts of cells and whole living cells in their native environment without causing optical damage [5, 6]. The use of optical traps in single molecule biophysics has greatly enhanced our understanding of a wide range of molecular motors found within the cell [7|. Optical trap force spectroscopy has enabled researchers to carry out precise measurements of the minuscule forces and displacements that govern many microbiological processes at the single molecule level [8|. Protein folding and biosynthesis (ribosome translation) in vivo has been researched extensively since the 1960s [9], when Anfinsen postulated that a protein's native structure; is determined only by its amino acid sequence [10]. The protein folding problem is not just of purely scientific interest however, since aggregation of misfolded proteins (polypeptides) is observed in a wide range of pathological disorders in ageing organisms [11]. The aggregation of the protein hTau40 in neurons, for example, has been linked to Alzheimer's disease [12]. A better understanding of the mechanisms of protein synthesis and folding in vivo is highly desirable. The process of co-translational protein synthesis and folding in the crowded environment of the cell is difficult to study using ensemble methods due to the stochastic nature of ribosome translation. In this thesis a custom built high-resolution dual-trap optical tweezers instrument enabled the study of translation kinetics and folding pathways of individual ribosome-bound nascent polypeptide chains (proteins) in real-time, for the first time to our knowledge, using sub-micron-sized surface-modified polystyrene beads as force, displacement and fluid flow sensors. By effectively decoupling the instrument from the environment and by using back-focal-plane interferometry with differential detection, sub-nm displacements and sub-pN forces on ms timescales could be measured without drift over long periods of time [13]... | |
| dc.format | 1 volume | |
| dc.language.iso | en | |
| dc.publisher | Trinity College (Dublin, Ireland). School of Physics | |
| dc.relation.isversionof | http://stella.catalogue.tcd.ie/iii/encore/record/C__Rb16712056 | |
| dc.subject | Physics, Ph.D. | |
| dc.subject | PhD Trinity College Dublin, 2016 | |
| dc.title | Following translation of individual proteins by single ribosomes in real-time using dual-trap optical tweezers | |
| dc.type | thesis | |
| dc.type.supercollection | thesis_dissertations | |
| dc.type.supercollection | refereed_publications | |
| dc.type.qualificationlevel | Doctoral | |
| dc.type.qualificationname | Doctor of Philosophy (Ph.D.) | |
| dc.rights.ecaccessrights | openAccess | |
| dc.format.extentpagination | pp 215 | |
| dc.description.note | TARA (Trinity's Access to Research Archive) has a robust takedown policy. Please contact us if you have any concerns: rssadmin@tcd.ie | |
| dc.identifier.uri | https://hdl.handle.net/2262/110396 | |
