MUTATIONS OF FUS CAUSE AGGREGATION OF RNA BINDING PROTEINS, DISRUPTIONS IN PROTEIN SYNTHESIS, AND DYSREGULATION OF NONSENSE MEDIATED DECAY

Kamelgarn, Marisa Elizabeth

01 January 2019

Amyotrophic lateral sclerosis (ALS) is a fatal neurodegenerative disease characterized by motor neuron death and subsequent muscle atrophy. Approximately 15% of ALS cases are inheritable, and mutations in the Fused in Sarcoma (FUS) gene contribute to approximately 5% of these cases, as well as about 2% of sporadic cases. FUS performs a diverse set of cellular functions, including being a major regulator of RNA metabolism. FUS undergoes liquid- liquid phase transition in vitro, allowing for its participation in stress granules and RNA transport granules. Phase transition also contributes to the formation of cytoplasmic inclusions found in the cell bodies of FUS ALS patients motor neurons. The nature of these inclusions has remained elusive, as the proteins localized to them have not been identified. Additionally, the functional consequence of the accumulation of cytoplasmic FUS inclusions has not been established, nor is it understood how they contribute to selective motor neuron death. We carried out two related, but independent studies to characterize the proteins that may be included in FUS-positive inclusions. In this first study, we utilized immunoprecipitation of wild-type and mutant FUS in the presence and absence of RNase, followed by LC MS/MS. The identified proteins represent those that directly or indirectly interact with FUS, with relatively high affinity that can be pulled down with immunoprecipitation. A wide variety of interacting proteins were identified and they are involved in a multitude of pathways including: chromosomal organization, transcription, RNA splicing, RNA transport, localized translation, and stress response. Their interaction with FUS varied greatly in their requirements for RNA. Most notably, FUS interacted with hnRNPA1 and Matrin-3, proteins also known to cause familial ALS. Immunofluorescent staining of proteins interacting with mutant FUS were localized to cytoplasmic inclusions. We concluded that mis-localization of these proteins potentially lead to their dysregulation or loss of function, thus contributing to FUS pathogenesis. In the second study, we developed a protocol to isolate dynamic FUS inclusions and employed LC MS/MS to identify all proteins associated with FUS inclusions. We identified a cohort of proteins involved in translation, splicing, and RNA export to be associated with the FUS inclusions. Further pathway and disease association analysis suggested that proteins associated with translation and RNA quality control pathways may be the most significant. Protein translation assays using both N2A and ALS patient fibroblasts demonstrated suppression of protein biosynthesis in mutant FUS expressing cells. However, translation initiation was not impaired. To understand how protein synthesis is suppressed by mutant FUS mediated defects in RNA metabolism, we examined changes in a well conserved RNA turnover pathway namely: nonsense mediated decay (NMD). We found that NMD is hyperactivated in cells expressing mutant FUS, likely due to chronic suppression of protein translation shifting the pathways autoregulatory circuit to allow for hyperactivation. We concluded that mutant FUS suppresses protein biosynthesis and disrupts NMD regulation. These defects together likely contribute to motor neuron death.

Fused in Sarcoma

Amyotrophic Lateral Sclerosis

RNA binding

Nonsense Mediated Decay

Protein Translation

Biochemistry

Bioinformatics

Cell Biology

Molecular and Cellular Neuroscience

Molecular Biology

Molecular Genetics

Nervous System Diseases

GLS-1, a novel P granule component, modulates a network of conserved RNA regulators to influence germ cell fate decisions

Eckmann, Christian R., Schmid, Mark, Kupinski, Adam P., Jedamzik, Britta, Harterink, Martin, Rybarska, Agata

26 November 2015

Post-transcriptional regulatory mechanisms are widely used to influence cell fate decisions in germ cells, early embryos, and neurons. Many conserved cytoplasmic RNA regulatory proteins associate with each other and assemble on target mRNAs, forming ribonucleoprotein (RNP) complexes, to control the mRNAs translational output. How these RNA regulatory networks are orchestrated during development to regulate cell fate decisions remains elusive. We addressed this problem by focusing on Caenorhabditis elegans germline development, an exemplar of post-transcriptional control mechanisms. Here, we report the discovery of GLS-1, a new factor required for many aspects of germline development, including the oocyte cell fate in hermaphrodites and germline survival. We find that GLS-1 is a cytoplasmic protein that localizes in germ cells dynamically to germplasm (P) granules. Furthermore, its functions depend on its ability to form a protein complex with the RNA-binding Bicaudal-C ortholog GLD-3, a translational activator and P granule component important for similar germ cell fate decisions. Based on genetic epistasis experiments and in vitro competition experiments, we suggest that GLS-1 releases FBF/Pumilio from GLD-3 repression. This facilitates the sperm-to-oocyte switch, as liberated FBF represses the translation of mRNAs encoding spermatogenesis-promoting factors. Our proposed molecular mechanism is based on the GLS-1 protein acting as a molecular mimic of FBF/Pumilio. Furthermore, we suggest that a maternal GLS-1/GLD-3 complex in early embryos promotes the expression of mRNAs encoding germline survival factors. Our work identifies GLS-1 as a fundamental regulator of germline development. GLS-1 directs germ cell fate decisions by modulating the availability and activity of a single translational network component, GLD-3. Hence, the elucidation of the mechanisms underlying GLS-1 functions provides a new example of how conserved machinery can be developmentally manipulated to influence cell fate decisions and tissue development.

info:eu-repo/classification/ddc/610

ddc:610

Charakterizace ABC-F proteinu Sco0636 u Streptomyces coelicolor / Characterization of the ABC-F protein Sco0636 in Streptomyces coelicolor

Pinďáková, Nikola

January 2018

The main topic of this diploma thesis is ARE (resistance) proteins from the ABC-F family of the second class of ABC proteins. ARE proteins confer resistance to antibiotics that bind to a large ribosomal subunit and therefore inhibit proteosynthesis. One of the ARE proteins is the Lmr (C) protein, which is part of the linkomycin biosynthesis cluster of Streptomyces lincolnensis, and according to new results, Lmr (C) does not have to be just resistant protein but may have also regulatory function. We decided to study Sco0636, the closest homologue to Lmr (C) in Streptomyces coelicolor, which is a model organism in the study of secondary metabolism. Thanks to the production of color pigments, it is possible to monitor the effect of ARE proteins on secondary metabolism directly on the plates. I prepared the deletion mutant and the strain with constitutive expression of sco0636, and observed the effect on the phenotype. I followed the production of a blue asset and set a minimum inhibitory concentration to selected antibiotics, which bind to the ribosome. I have found that Sco0636 gives high resistance to tiamulin and so it has been named TiaA. The deletion of gene sco0636 accelerated production of actinorodine, and constitutive expression of this gene slowed down production. Keywords: ABC proteins,...

Charakterizace ABC-F proteinu Sco0636 u Streptomyces coelicolor / Characterization of the ABC-F protein Sco0636 in Streptomyces coelicolor

Pinďáková, Nikola

January 2018

The main topic of this diploma thesis is ARE (resistance) proteins from the ABC-F family of the second class of ABC proteins. ARE proteins confer resistance to antibiotics that bind to a large ribosomal subunit and therefore inhibit proteosynthesis. One of the ARE proteins is the Lmr (C) protein, which is part of the linkomycin biosynthesis cluster of Streptomyces lincolnensis, and according to new results, Lmr (C) does not have to be just resistant protein but may have also regulatory function. We decided to study Sco0636, the closest homologue to Lmr (C) in Streptomyces coelicolor, which is a model organism in the study of secondary metabolism. Thanks to the production of color pigments, it is possible to monitor the effect of ARE proteins on secondary metabolism directly on the plates. I prepared the deletion mutant and the strain with constitutive expression of sco0636, and observed the effect on the phenotype. I followed the production of a blue asset and set a minimum inhibitory concentration to selected antibiotics, which bind to the ribosome. I have found that Sco0636 gives high resistance to tiamulin and so it has been named TiaA. The deletion of gene sco0636 accelerated production of actinorodine, and constitutive expression of this gene slowed down production. Keywords: ABC proteins,...

Functional and inhibition studies on 2-oxoglutarate-dependent oxygenases

Thalhammer, Armin

January 2012

This thesis explores roles of 2-oxoglutarate-dependent (2OG) oxygenases as interfaces that modulate steps in the flow of genetic information in cells in response to oxygen availability. Chapter 1 introduces mechanistic, biochemical and physiological aspects of major subfamilies of 2OG oxygenases, and their established regulatory roles in cells. In addition, structural and functional aspects of the ribosome and the translation process are discussed, with a focus on post-translational ribosome modifications. Chapter 2 investigates histone demethylases, which mediate chromatin-dependent regulation of gene expression and provides proof-of-concept for the rational, structure-guided design of small-molecules for selective inhibition of 2OG oxygenases with roles in cancer and inflammatory disease. Chapter 3 suggests regulatory roles for ten-eleven-translocation (TET)- catalysed DNA hydroxylation; calorimetric and thermal analyses reveal a duplex-stabilizing effect of the epigenetic 5-methylcytosine mark that is reversed upon conversion to 5- hydroxymethylcytosine (also termed the ‘sixth’ DNA base), raising the possibility that 2OG oxygenase catalysis might affect transcription via biophysical effects. Chapter 4 investigates fluoride release assays as a technology to enable medicinal chemistry studies on 2OG oxygenases with roles in fat mass regulation and obesity, cancer and inflammation; studies on the ALKBH5 enzyme show that it is a hypoxically upregulated 2OG oxygenase with a substrate preference distinct from previously characterized ALKBH enzymes. Chapter 5 identifies OGFOD1 as a 2OG-dependent ribosomal protein hydroxylase. OGFOD1 catalysis is conserved from yeast to humans. OGFOD1 catalyses formation of trans-3- hydroxy-L-proline in a highly conserved loop of ribosomal protein S23 proximal to the ribosomal decoding centre, possibly to modulate the interactions of eukaryotic ribosomes with tRNA, mRNA and translation factors in an oxygen-dependent manner. OGFOD1 is the functionally most well-conserved protein-modifying 2OG oxygenase; likewise, ribosomal protein S23 hydroxylation is the most well-conserved post-translational ribosome modification in eukaryotes. Some cell lines require OGFOD1 for proliferation, and scaffolds for OGFOD1- selective inhibitors are developed for use as potential antiproliferative agents and probes for cellular function. Chapter 6 shows the development of assays to investigate whether OGFOD1 catalysis affects ribosome assembly and function, including processivity, accuracy of initiation, elongation and termination, in yeast and mammalian cell lines. Chapter 7 concludes that ribosome hydroxylation might present an additional layer of regulatory complexity by which 2OG oxygenases could enable cells to respond to fluctuating oxygen levels.

572.8

L’angiogénine : un nouveau médiateur de la réponse au stress du Réticulum Endoplasmique / Angiogenin : a novel mediator of the Endoplasmic Reticulum stress response

Mami, Iadh

28 October 2015

Le stress du Réticulum Endoplasmique (RE) est impliqué dans la physiopathologie des maladies rénales, et la réponse UPR (Unfolded Protein Response), qui est activée en réponse à ce stress, joue un rôle important dans l'homéostasie des cellules tubulaires rénales et des podocytes. L’étude des mécanismes moléculaires et des conséquences de l'activation de cette voie est donc importante dans la compréhension de la physiopathologie des maladies rénales et dans la caractérisation de biomarqueurs de lésions évolutives. L’Angiogénine (ANG, appelée également RNase 5) est une ribonucléase secrétée, qui est impliquée dans la réponse à certains stress cellulaires, et permet une adaptation cellulaire et tissulaire.
L'objectif de ce travail a été de mettre en évidence les mécanismes de régulation et les fonctions biologiques de l'ANG en réponse au stress du RE. A partir d'un modèle de cellules tubulaires rénales humaines en culture, nous avons montré que le stress du RE induisait l’expression de l’Angiogénine ainsi que sa sécrétion. Cette observation a été également faite sur différents modèles murins de lésions rénales. Le facteur transcriptionel sXBP1, activé par le transducteur de la réponse UPR, IRE1a, est directement impliqué dans la régulation de l'expression de l'Angiogénine.
Nous avons mis en évidence que l'Angiogénine participait à l’inhibition de la traduction protéique en réponse au stress du RE en produisant des fragments d'ARN de transfert appelés tiRNAs (stress-induced tRNA fragments) qui répriment la traduction des protéines en interférant avec le complexe initiateur de la traduction. L'Angiogénine favorise la survie cellulaire en réduisant l'apoptose induite par le stress du RE, et des souris invalidées pour le gène codant l'Angiogénine sont plus sensibles aux lésions de nécrose tubulaire aigues induites par la Tunicamycine. Outre les propriétés cellulaires "intrinsèques" de l'Angiogénine, nous avons également caractérisé les mécanismes de sécrétion de l'Angiogénine par l'épithélium rénal en situation de stress du RE. La sécrétion épithéliale de l'Angiogénine est sous le contrôle des facteurs transcriptionnels NF-κB et sXBP1, et se produit sous un mode conventionnel, c’est-à-dire dépendant du transit par l'appareil de Golgi. A ce titre, la régulation de l'Angiogénine est similaire à celle de l'Interleukine 6. L'Angiogénine induit une polarisation des macrophages vers un phénotype pro-inflammatoire. Enfin, considérant que l'Angiogénine est secrétée par l'épithélium rénal en situation de stress, nous avons montré que l’Angiogénine peut être un marqueur non invasif de souffrance rénale. L'Angiogénine peut être quantifiée dans les urines de patients porteurs de maladies rénales, et sa concentration est corrélée à la concentration urinaire de Retinol Binding Protein (une protéine de petit poids moléculaire, marqueur de dysfonction tubulaire), mais pas avec celle de l'Albumine. En outre, la concentration urinaire d'Angiogénine est significativement plus élevée dans les urines de patients transplantés rénaux dont la biopsie rénale met en évidence des lésions de tubulite (rejet aigu cellulaire et néphropathie associée au BK virus) que dans les urines de patients indemnes de lésions tubulaires (rejet humoral, ou absence de lésions histologiques). Nous avons mis en évidence par immuno-histochimie un marquage nucléaire du facteur transcriptionnel sXBP1 dans les tubules de reins porteurs de lésions de tubulite, suggérant un lien potentiel entre sécrétion d'Angiogénine et activation du facteur transcriptionnel sXBP1 dans un environnement inflammatoire. En conclusion, nous avons intégré la régulation l'Angiogénine dans la réponse épithéliale rénale au stress du RE, et caractérisé ses fonctions biologiques intracellulaires et paracrines. Notre travail a identifié l'Angiogénine urinaire en étant que potentiel marqueur de lésions rénales tubulaires. / The Endoplasmic Reticulum (ER) stress is involved in the pathophysiology of renal diseases ; the UPR (Unfolded Protein Response), which is activated in response to that stress plays an important role in renal tubular cells and podocytes homeostasis and consequently in tissu homeostasis. Understanding the molecular mechanisms and the consequences of the activation of this pathway is important to characterize the pathophysiology of renal diseases and identification of biomarkers of ongoing lesions. Angiogenin (ANG, also known as RNase 5) is a secreted ribonuclease, which is involved in the cellular stress response, it allows cell and tissue adaptation. The goal of this work was to clarify and identify the mechanisms regulating Angiogenin’s expression and its biological functions during ER stress. Using a human renal tubular cell line, we have shown that ER stress induces the expression of angiogenin and its secretion. This observation was also made on several murine models of renal injury. The transcriptional factor sXBP1 activated by the UPR transducer, IRE1α, is directly involved in regulating the expression of angiogenin. We have shown that angiogenin participates in the inhibition of protein translation in response to ER stress by cleaving transfer RNA and generating tiRNAs (stress-induced tRNA fragments) that suppress protein translation by interfering with the translation initiation complex. Angiogenin promotes cell survival by reducing ER stress-induced apoptosis, ANG knockout mice are more sensitive to acute tubular necrotic lesions induced by tunicamycin. In addition to the cell-autonomous effects of angiogenin, we also characterized the mechanisms by which Angiogenin is secreted by the renal epithelium under ER stress. Angiogenin is secreted in a conventional manner under the control of the transcriptional factors NF-kB and sXBP1. As such, the regulation of angiogenin is similar to Interleukin-6. We also demonstrated that Angiogenin induces macrophage polarization to a pro-inflammatory phenotype. Finally, considering that angiogenin is secreted by the renal epithelium under stress, we have shown that angiogenin may be a noninvasive marker of kidney injury. Angiogenin can be quantified in the urine of patients with kidney disease, its urinary concentration is correlated to the urinary concentration of Retinol Binding Protein (a low molecular weight protein marker of tubular dysfunction), but not with that of Albumin . In addition, the urinary concentration of angiogenin is significantly higher in the urine of renal transplant patients whose renal biopsy highlights tubulitis lesions (cell acute rejection and BK virus associated nephropathy) than in the urine of patients without histological tubular damage (antibody-mediated rejection, or no visible histological lesions). We have demonstrated by immuno-histochemistry a tubular nuclear localization of the activated transcriptional factor sXBP1 in the biopsies of patients with high tubulitis score, suggesting a potential relationship between the secretion of Angiogenin and the activation of transcriptional factor sXBP1 within an inflammatory environment. To conclude, we have described Angiogenin as a new mediator of the integrated ER stress response, and characterized its cell- and non-cell-autonomous biological functions. Our study have identified urinary angiogenin as a potential marker of ongoing kidney tubular injuries.

Insuffisance rénale

Transplantation rénale

Angiogénine/RNase5

Stress du Réticulum Endoplasmique

Unfolded Protein Response

Traduction protéique

Immunité du transplant

Biomarqueurs

Kidney injury

Kidney transplant

Angiogenin/RNase5

Endoplasmic Reticulum stress

Unfolded Protein Response

Protein translation

Transplant immunity

Biomarkers

571.95

Translational Control Of p53 And Its Isoform By Internal Initiation

Grover, Richa

01 January 2008

Tumor suppressor p53, the guardian of the genome, has been intensely studied molecule owing to its central role in maintaining cellular integrity. While the level of p53 protein is maintained low in unstressed conditions, there is a rapid increase in the functional p53 protein levels during stress conditions. It is now well documented in literature that p53 protein accumulates in the cells following DNA damage by posttranslational modifications leading to increased stability and half life of protein. Additionally, recent studies have also highlighted the significance of increased p53 translation during stress conditions. Interestingly, an alternative initiation codon has been shown to be present within the coding region of p53 mRNA. Translation initiation from this internal AUG results in an N-terminally truncated p53 isoform, described as ΔN-p53. However, the mechanisms underlying co-translational regulation of p53 and ΔN-p53 are still poorly understood. Studies have suggested that synthesis of both p53 and its ΔN-p53 isoform is regulated during cell cycle and also stress and cell-type specific manner. Interestingly, reports also demonstrate continued synthesis of both p53 isoforms during stress conditions. In contrast, global rates of cap-dependent translation initiation are shown to be reduced during stress conditions. This translation attenuation is observed mainly due to restricted availability of critical initiation factors. Interestingly, preferential synthesis of a vital pool of survival factors persists even during these circumstances. Studies have suggested that this selective translation is mediated via alternative mechanisms of translation initiation. One of the important mechanisms used for protein synthesis during these conditions is internal initiation. In this mechanism, the ribosomes are recruited to a complex RNA structural element known as ‘Internal Ribosome Entry Site (IRES)’, generally present in the 5’ untranslated region (UTR) of mRNA. Therefore, it is possible that the translation of p53 and ΔN-p53 could also be regulated by IRES mediated translation, especially during stress conditions. In this thesis the role of internal initiation in translational control of p53 and ΔN-p53 has been investigated. Additionally, the putative secondary structure of p53 IRES RNA has been determined. Further, it has been shown that polypyrimidine tract binding (PTB) protein acts as an important regulator of p53 IRES activities. The probable mechanism of action of PTB protein has also been investigated. The results suggest that interaction with PTB alters the p53 IRES conformation which could facilitate translation initiation. Finally, the possible physiological significance of existence of p53 IRES elements has been addressed. In the first part of the thesis, the presence of internal ribosome entry site within p53 mRNA has been investigated. As a first step, the 5’UTRs mediating the translation of both p53 and ΔN-p53 were cloned in the intercistronic regions of bicistronic constructs. Results of in vivo transfection of these bicistronic constructs suggested the presence of two IRES elements within p53 mRNA, with activities comparable to known viral and cellular IRESs. The IRES directing the translation of p53 is in the 5'-untranslated region of the mRNA, whereas the IRES mediating the translation of ΔN-p53 extends further into the protein-coding region. To further validate, stringent assays were performed to rule out the possibility of any cryptic promoter activity, re-initiation/scanning or alternative splicing in the p53 mRNA. Transfection of in vitro synthesized bicistronic RNAs confirmed the presence of IRES elements within p53 mRNA. Incidentally, this constitutes the first report on translational control of p53 by internal initiation. In the second part of the thesis, the secondary structure of p53 IRES RNA has been investigated. Structural analysis of p53 RNA was performed using structure-specific nucleases and modifying chemicals. The results obtained from chemical modification and nuclease probing experiments were used to constrain Mfold predicted structures. Based on this, a putative secondary structure model for p53 IRES RNA has been derived. Sequence alignment suggested that the p53 IRES RNA showed significant sequence conservation across mammalian species. To study the effect of mutations on the IRES structure, mutant p53 IRESs were used that harbor silent mutations at critical locations within the p53 IRES element. Incidentally, one of the mutant constructs used in the study was observed to be a naturally occurring mutation in a chronic lymphocyte leukemia patient. RNA structure analyses of these two mutant p53 IRES RNAs were performed. The nuclease mapping data suggested conformational alteration in these mutant RNAs with respect to wild type. Consistently, a comparative Circular-Dichroism spectroscopy of the Wt and mutant RNAs also validated the conformational alteration of the mutant RNAs. This also suggested that the presence of mutations in p53 IRES might result in decreased induction of p53 protein following DNA damage due to altered RNA structure. This might constitute as one of the mechanisms leading to tumor development in some types of cancers. In the third part of the thesis, the role of important cellular proteins that might modulate p53 IRES mediated translation has been studied. These cellular proteins act as IRES interacting trans-acting factors (ITAFs). Polypyrimidine tract binding (PTB) protein is an important ITAF implicated in regulating IRES mediated gene expression during apoptosis. It was observed that PTB protein specifically interacts with both the IRES elements within p53 mRNA. Interestingly, the affinity of interaction of PTB protein with both p53 IRES RNAs was observed to be significantly different. In order to determine the contact points of PTB on p53 IRES, a foot-printing assay using structure specific nuclease and recombinant-PTB protein was performed on p53 RNA. The data from foot-printing as well as primer extension inhibition assay (toe-printing analysis) suggested the presence of multiple PTB binding sites on p53 IRES RNA. Based on these results, a deletion mutant was generated that showed reduced PTB binding and also reduced IRES activity as compared to wild type. Further, to study the role of PTB in mediating p53 translation, the expression of PTB gene was partially silenced by using PTB specific siRNA. Partial depletion of endogenous PTB protein showed a significant decrease in the p53 IRES activities. These results suggest that PTB protein is essential for the p53 IRES activities. To understand the probable mechanism by which PTB regulates p53 IRES mediated translation, CD spectroscopy analysis of p53 IRES RNA was performed in the absence and presence of PTB protein. Interestingly, CD spectra analysis of the p53 RNA in the presence of PTB suggested a specific conformational change in p53 IRES, which might probably facilitate ribosome loading during internal initiation. This also suggests that abnormal expression of p53 ITAFs might lead to reduced p53 induction following DNA damage conditions. It could also be another event leading to malignant transformation of cells bearing wild type p53. It is highly tempting to speculate that the levels of p53 ITAFs could also be used as tumor biomarkers. In the fourth part of the thesis, the physiological relevance of existence of IRES elements within p53 mRNA has been investigated. The levels of p53 and ΔN-p53 proteins are known to be regulated in a cell cycle phase-dependent manner. The IRES activities of both p53 IRES elements were investigated at different phases of cell cycle. The activity of the IRES responsible for translation of p53 protein was found to be highest at G2-M transition and the maximum IRES activity corresponding to ΔN-p53 synthesis was observed at G1-S transition. These results suggested that the p53 IRES activities are regulated in a cell-cycle phase-dependent manner. Next, the regulation of p53 IRES mediated translation during stress conditions was studied. Human lung carcinoma cell line, A549 cells (that endogenously express both the p53 isoforms), were exposed to DNA damaging drug, doxorubicin. The level of p53 protein was observed to increase in a time-dependent manner. Interestingly, PTB protein, which is predominantly nuclear, was found to translocate to the cytoplasm during stress condition in a time-dependent manner. Under similar conditions, p53 protein was observed to reverse translocate from the cytoplasm to nucleus, probably to function as a transcription factor. Next, the influence of partial PTB silencing on p53 isoforms in the presence of cell stress (mediated by doxorubicin) was investigated. The data indicated reduced levels of both p53 and ΔN-p53 when PTB gene expression was partially silenced. These observations constitute “the proof of concept” that relative abundance of an ITAF, such as PTB protein, might contribute to regulating the coordinated expression of the p53 isoforms. The thesis reveals the presence as well as the physiological relevance of existence of IRES elements within p53 mRNA. The novel discovery of p53 IRES elements may provide new insights into the underlying mechanism of translational regulation. The modulation of the p53 IRES activities by PTB protein suggests that the regulated expression of p53 isoforms depends on the integrity of IRES elements and availability of cellular proteins that can serve as p53 ITAFs. Thus, studies pertaining to the identification of mutations within p53 IRES region as well as abnormal expression of p53 ITAFs such as PTB in cancer cells may have far reaching implications. These studies might lead to further advances in the field of cancer detection, prognosis and design of novel therapeutic strategies.

Ribonucleic Acid (RNA)

Proteins

RNA Viruses

p53 Protein

p53 Protein Isoforms

p53 RNA - Structural Analysis

Protein Translation

Polypyrimidine Tract Binding Protein

Protein Regulation

IRES RNA

PTB Binding

p53 mRNA

Biochemical Genetics