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dc.contributor.advisorGillespie, S. H.
dc.contributor.authorFarmer, Eoghan
dc.coverage.spatial164 p.en_US
dc.date.accessioned2021-09-17T15:30:09Z
dc.date.available2021-09-17T15:30:09Z
dc.date.issued2019-12-03
dc.identifier.urihttps://hdl.handle.net/10023/23983
dc.description.abstractThis study looks to monitor tuberculosis treatment response using molecular techniques. An assay for the detection and enumeration of Mycobacterium tuberculosis already existed in the form of the Mycobacterial Load Assay (MBL). This utilised reverse transcriptase quantitative polymerase chain reaction (RT-qPCR) to detect M. tuberculosis 16S ribosomal RNA (rRNA) and thereby quantify bacillary loads in patient sputa. By measuring labile RNA the assay was thought to only measure viable bacilli. However, unpublished data from the Gillespie lab suggested that 16S rRNA remains stable even once cell are non-viable. Two new markers were sought to represent the viable bacilli: M. tuberculosis precursor 16S rRNA (pre-16S rRNA) and transfer- messenger RNA (tm-RNA). Both of these novel biomarkers were chosen because of their complex secondary structures giving them increased stability allowing for their detection in adverse environments. Development and of a multiplex assay using the same messenger RNA (mRNA) phyB internal control utilised by the MBL assay, then the fielding testing of these multiplex assays was performed with the subsequent failure of the phyB control. The internal control was then redesigned to be more robust and reproducible utilising a novel M. marinum control. The new multiplex assays with 16S rRNA, pre-16S rRNA and tm-RNA with the M. marinum internal control were then tested on 520 patient samples to demonstrate that the assays could be used for monitoring treatment response.en_US
dc.language.isoenen_US
dc.publisherUniversity of St Andrews
dc.subject.lccQR201.T6F2
dc.subject.lcshTuberculosis--Treatmenten
dc.subject.lcshTuberculosis--Molecular aspectsen
dc.subject.lcshBiochemical markersen
dc.titleMonitoring tuberculosis treatment response using molecular techniquesen_US
dc.typeThesisen_US
dc.type.qualificationlevelDoctoralen_US
dc.type.qualificationnameMD Doctor of Medicineen_US
dc.publisher.institutionThe University of St Andrewsen_US
dc.rights.embargoreasonEmbargo period has ended, thesis made available in accordance with University regulationsen
dc.identifier.doihttps://doi.org/10.17630/sta/138


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