Cellular reactivation of foetal haemoglobin transcription by the use of CRISPR/Cas9

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DC Field	Value	Language
dc.date.accessioned	2020-12-03T10:52:46Z	-
dc.date.available	2020-12-03T10:52:46Z	-
dc.date.issued	2020	-
dc.identifier.citation	Kuduzovic, H. (2020). Cellular reactivation of foetal haemoglobin transcription by the use of CRISPR/Cas9 (Master's dissertation).	en_GB
dc.identifier.uri	https://www.um.edu.mt/library/oar/handle/123456789/65161	-
dc.description	M.SC.APPLIED BIOMED.SCI.	en_GB
dc.description.abstract	Sequential expression of embryonic, foetal and adult haemoglobin during human ontogeny has been a focus of numerous studies focusing on mechanisms of target gene switching in order to increase expression of foetal haemoglobin and consequently leading to significant improvement of clinical manifestation of haemoglobinopathies that include sickle cell disease and β-thalassaemia. Understanding the natural switch control from foetal to adult haemoglobin and actions of genes involved could lead to potentially lifesaving therapeutic approach. EKLF also known as KLF1 is an important regulatory protein involved in the γ- to β-globin gene switching mechanism that directly induces the expression of the β-globin gene and conversely represses γ-globin. In this study I sought to test a number of CRISPR/Cas9 systems with the purpose to disrupt the functions of KLF1, LRF and BCL11A genes and inhibit the γ- to β-globin gene switching in K562 cells. Relative quantification was performed for the assessment of all globin including γ globin expression as well as the target genes KLF1, BCL11A and LRF. The BCL11A quantification was not successful due to low expression of the same gene in K562 cells and was therefore not pursued. The levels of γ-globin mRNA varied between 48hrs and 96hrs post differentiation with hemin induction, showing a 1.97-fold induction for KLF1 knockdown by CRISPR/Cas9 as opposed to just after 48hrs and also when compared to untreated cells. The findings obtained in this dissertation support the induction of γ-globin expression upon targeting KLF1 through CRISPR/Cas9 mediated silencing. As a result, the effect of KLF1 inhibitory influence on γ-globin gene expression is removed. The same was not observed upon targeting LRF by CRISPR/Cas9, in which γ-globin remained low. Application of CRISPR technology in adult erythroid progenitors may provide a method for activating foetal haemoglobin expression in individuals with β-thalassaemia or sickle cell disease.	en_GB
dc.language.iso	en	en_GB
dc.rights	info:eu-repo/semantics/restrictedAccess	en_GB
dc.subject	Sickle cell anemia	en_GB
dc.subject	Hemoglobinopathy	en_GB
dc.subject	Gene targeting	en_GB
dc.subject	CRISPR-associated protein 9	en_GB
dc.title	Cellular reactivation of foetal haemoglobin transcription by the use of CRISPR/Cas9	en_GB
dc.type	masterThesis	en_GB
dc.rights.holder	The copyright of this work belongs to the author(s)/publisher. The rights of this work are as defined by the appropriate Copyright Legislation or as modified by any successive legislation. Users may access this work and can make use of the information contained in accordance with the Copyright Legislation provided that the author must be properly acknowledged. Further distribution or reproduction in any format is prohibited without the prior permission of the copyright holder.	en_GB
dc.publisher.institution	University of Malta	en_GB
dc.publisher.department	Faculty of Health Sciences. Department of Applied Biomedical Science	en_GB
dc.description.reviewed	N/A	en_GB
dc.contributor.creator	Kuduzovic, Halida	-
Appears in Collections:	Dissertations - FacHSc - 2020 Dissertations - FacHScABS - 2020

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