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Physikalische Berechnungen zu Fragen der Tumoren, der Mutationen und der EvolutionDrechsel, Dieter 07 March 2012 (has links)
Bei der Replikation monotoner Sequenzen tritt theoretisch ein Vorgang auf, den wir als „Basenkonkurrenz“ bezeichnen: Da sich an jeder Replikations-Stelle mehrere Basenbausteine bewerben, aber immer nur einer benötigt wird, bewerben sich die übrig gebliebenen Bausteine an den jeweils nächsten Replikations - Positionen und erlangen wegen der fortwährenden Beschleunigung durch elektrostatische Anziehung immer größere kinetische Energien. Das führt dazu, dass an einer bestimmten Stelle der replizierenden monotonen Sequenz der eine Partner der Wasserstoffbrückenbindung ein hohes Energieniveau erreicht.
Es wird berechnet, dass sich dadurch kurzzeitig eine sehr hohe Bindungsenergie zwischen den beiden Partnern der Wasserstoffbrückenbindung einstellt, wodurch der in dieser kurzen Zeitspanne wirkende DNA-Reparaturmechanismus unterdrückt wird.
Die Auswirkungen der hohen Basenkonkurrenz – Energien werden berechnet (hohe Bindungsenergien der Wasserstoffbrückenbindungen, Tunnelvorgänge, irreparable Mutationen). Die Folgen dieser Erscheinung sind Tumorbildung, Alterung, Veränderung der DNA – Struktur, Beeinflussung der Evolution, worauf im Einzelnen eingegangen wird.
Es zeigt sich, dass die negativen Auswirkungen der Basenkonkurrenz vorwiegend bei zu niedriger Viskosität des Zellplasmas auftreten.:1. Basenkonkurrenz 3
1.1. Basenkonkurrenz während des Replikationsvorganges 3
1.2. Der Einfluss der Viskosität des Zytoplasmas 6
1.3. Berechnung der Energiestufen Tk 7
2. Auswirkungen der Basenkonkurrenz auf tautomere Basenpaare 8
2.1. Berechnung der Bindeenergie der Wasserstoffbrückenbindung 8
2.1.1. Normierung der Wellenfunktionen und 12
2.1.1.1.Wasserstoff im Grundzustand (1s) 12
2.1.1.2. Wasserstoff im angeregten Zustand (2p) 13
2.1.1.3. Akzeptor im Grundzustand 13
2.1.2. Darstellung der Energieflächen 14
2.1.3. Berechnung der Bindeenergie, wenn beide Partner sich im
Grundzustand befinden 15
2.1.4. Berechnung der Bindeenergie, wenn sich der Acceptor im
Grundzustand und der Wasserstoff im angeregten Zustand 2p befindet 18
2.2. Falschpaarung durch Basenkonkurrenz bei tautomeren Basenpaaren 20
2.3. Abklingzeit der Basenkonkurrenz – Energie 21
2.4. Entstehung, Vererbung und Löschung eines „Gedächtnisses“
vorgeschädigter DNA 22
2.4.1. Entstehung 22
2.4.2. Vererbung 22
2.4.3. Löschung 22
3. Auswirkung der Basenkonkurrenz auf die DNA – Struktur 23
4. Tunnelvorgänge in biologischen Wasserstoffbrückenbindungen 26
4.1. Berechnung der Tunnel – Wahrscheinlichkeit 27
4.1.1. Ab–initio–Berechnung der Tunnel –Wahrscheinlichkeit 27
4.1.2. Der Protonenstrom 33
4.1.3. Der Einfluss der Temperatur 36
4.1.4. Berechnung der Tunnel – Wahrscheinlichkeit in
Wasserstoffbrückenbindungen bei parabelförmigem Potenzialverlauf. 37
4.1.5. Berechnung des Mindestabstandes zwischen der
Gesamtenergie E und dem Potenzialwall der Wasserstoffbrückenbindung 43
4.1.6. Berechnung der Größe 16/R 44
4.1.7. Die Änderung der Tunnel – Wahrscheinlichkeit durch Temperatur – und
Energieänderung. 46
5. Zufällige Änderung der Basenverteilung der DNA während der Replikation 49
5.1. Aufzählung aller möglichen Verteilungen 49
5.2. Aufzählung aller günstigen Verteilungen und die Chance des
Auftretens hoher Basenkonkurrenz – Energie 51
6. Die Total – Wahrscheinlichkeit der durch Basenkonkurrenz
verursachten Mutation 53
7. Interpretation der Gleichung (93) 55
8. Evolution und Physik 58
9. Mutation und Physik innerhalb kleinerer Zeiträume 58
10. Zusammenfassung 59
Literaturverzeichnis 60
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Towards patient selection for cranial proton beam therapy – Assessment of current patient-individual treatment decision strategiesDutz, Almut 27 November 2020 (has links)
Proton beam therapy shows dosimetric advantages in terms of sparing healthy tissue compared to conventional photon radiotherapy. Those patients who are supposed to experience the greatest reduction in side effects should preferably be treated with proton beam therapy. One option for this patient selection is the model-based approach. Its feasibility in patients with intracranial tumours is investigated in this thesis. First, normal tissue complication probability models for early and late side effects were developed and validated in external cohorts based on data of patients treated with proton beam therapy. Acute erythema as well as acute and late alopecia were associated with high-dose parameters of the skin. Late mild hearing loss was related to the mean dose of the ipsilateral cochlea. Second, neurocognitive function as a relevant side effect for brain tumour patients was investigated in detail using subjective and objective measures. It remained largely stable during recurrence-free follow-up until two years after proton beam therapy. Finally, potential toxicity differences were evaluated based on an individual proton and photon treatment plan comparison as well as on models predicting various side effects. Although proton beam therapy was able to achieve a high relative reduction of dose exposure in contralateral organs at risk, the associated reduction of side effect probabilities was less pronounced. Using a model-based selection procedure, the majority of the examined patients would have been eligible for proton beam therapy, mainly due to the predictions of a model on neurocognitive function.:1. Introduction
2. Theoretical background
2.1 Treatment strategies for tumours in the brain and skull base
2.1.1 Gliomas
2.1.2 Meningiomas
2.1.3 Pituitary adenomas
2.1.4 Tumours of the skull base
2.1.5 Role of proton beam therapy
2.2 Radiotherapy with photons and protons
2.2.1 Biological effect of radiation
2.2.2 Basic physical principles of radiotherapy
2.2.3 Field formation in radiotherapy
2.2.4 Target definition and delineation of organs at risk
2.2.5 Treatment plan assessment
2.3 Patient outcome
2.3.1 Scoring of side effects
2.3.2 Patient-reported outcome measures – Quality of life
2.3.3 Measures of neurocognitive function
2.4 Normal tissue complication probability models
2.4.1 Types of NTCP models
2.4.2 Endpoint definition and parameter fitting
2.4.3 Assessment of model performance
2.4.4 Model validation
2.5 Model-based approach for patient selection for proton beam therapy
2.5.1 Limits of randomised controlled trials
2.5.2 Principles of the model-based approach
3. Investigated patient cohorts
4. Modelling of side effects following cranial proton beam therapy
4.1 Experimental design for modelling early and late side effects
4.2 Modelling of early side effects
4.2.1 Results
4.2.2 Discussion
4.3 Modelling of late side effects
4.3.1 Results
4.3.2 Discussion
4.4 Interobserver variability of alopecia and erythema assessment
4.4.1 Patient cohort and experimental design
4.4.2 Results
4.4.3 Discussion
4.5 Summary
5. Assessing the neurocognitive function following cranial proton beam therapy
5.1 Patient cohort and experimental design
5.2 Results
5.2.1 Performance at baseline
5.2.2 Correlation between subjective and objective measures
5.2.3 Time-dependent score analyses
5.3 Discussion and conclusion
5.4 Summary
6. Treatment plan and NTCP comparison for patients with intracranial tumours
6.1 Motivation
6.2 Treatment plan comparison of cranial proton and photon radiotherapy
6.2.1 Patient cohort and experimental design
6.2.2 Results
6.2.3 Discussion
6.3 Application of NTCP models
6.3.1 Patient cohort and experimental design
6.3.2 Results
6.3.3 Discussion
6.4 Summary
7. Conclusion and further perspectives
8. Zusammenfassung
9. Summary
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Analysis of anti-cancer drug penetration through multicell layers in vitro. The development and evaluation of an in vitro model for assessing the impact of convective fluid flow on drug penetration through avascular cancer tissues.Makeen, Hafiz Antar Mohammad January 2012 (has links)
High interstitial fluid pressure (IFP) in tumours is recognized as a barrier to drug delivery resulting in reduced efficacy. High IFP impedes the normal process of convective fluid flow (CFF) from blood vessels into the interstitium. The aim of this study was to develop an in vitro model that could be used to measure CFF and to study its effects on drug delivery. The model consists of a transwell cell culture insert which supports the growth of multicell layers (MCL) on collagen coated membranes. A graduated tube is inserted into the transwell and a pressure gradient is applied across the membrane by raising the volume of medium in the tube above that of the bottom chamber. CFF is determined by measuring the weight of medium in the bottom chamber as a function of time. CFF was inversely proportional to MCL thickness and 41.1±3.6µm thick MCL has completely stopped CFF. Using a physiologically relevant hydrostatic pressure of 28mmHg, a CFF of 21µL/min was recorded using a DLD-1 MCL that was 12.21±3.2µm thick. Under these conditions, the rates of penetration of doxorubicin, imatinib and gefitinib were respectively 42, 26 and 13 folds greater than when no CFF exists. Reversing the CFF so that it opposed the drug diffusion gradient significantly impairs drug penetration. In conclusion, a novel in vitro model for assessing the impact of CFF on drug delivery has been developed. This model could be used to evaluate strategies designed to increase drug delivery to solid tumours by modifying the CFF.
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MiR-215 regulates differentiation in colorectal cancer stem cellsJones, Matthew January 2014 (has links)
Since the initial description of cancer stem cells (CSCs) as a self-renewing subpopulation of malignant cells with tumor-initiating capacity, a growing body of evidence has supported the existence of CSCs in virtually every tumor type. Our previous work in colorectal cancer has identified the transcription factor CDX1 as a key regulator of colorectal CSC differentiation. CDX1 expression is frequently lost in colorectal cancer, resulting in more aggressive, poorly differentiated tumors with higher proportions of CSCs. Many miRNAs have been implicated in tumor suppression and carcinogenesis, but the roles of miRNAs in differentiation, particularly in colorectal cancer, remain poorly understood. We began by identifying miRNAs downstream of CDX1 by using high-throughput small-RNA sequencing to profile miRNA expression in two pairs of colorectal cancer cell lines with stable CDX1 overexpression or knockdown. Validation of candidates identified by RNAseq in a larger cell line panel revealed miR-215 to be most significantly correlated with CDX1 expression. ChIP-qPCR and promoter reporter assays confirmed that CDX1 directly transactivates miR-215 transcription. MiR-215 is depleted in FACS-enriched CSCs compared to unsorted samples. Overexpression of miR-215 in poorly-differentiated, highly clonogenic cell lines causes growth arrest and a dramatic decrease in colony formation. miR-215 knockdown using a miRNA sponge causes an increase in clonogenicity and impairs differentiation in CDX1-high cell lines. Indeed, the effects of CDX1 expression on both gene expression and colony morphology can be attenuated by miR-215 inhibition, indicating that miR-215 is a functional mediator of CDX1. Microarray studies following miR-215 overexpression indicate that miR-215 induces terminal differentiation-associated growth arrest, due in part to direct silencing of BMI1 expression and de-repression of BMI1 target genes including CDKN1A. Our work situates miR-215 as a link between CDX1 expression and BMI1 repression that governs differentiation in colorectal cancer. We further characterize another miRNA-transcription factor axis in colorectal cancer, and we identify the novel miR-3189-3p as a potent effector of cell death with potential therapeutic implications.
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Anthracycline-induced cardiotoxicity : the role of proteolytic pathwaysSishi, Balindiwe J. N. (Balindiwe Jennifer Nonkosazana) 03 1900 (has links)
Thesis (PhD)--Stellenbosch University, 2012. / ENGLISH ABSTRACT: Introduction: The anthracyclines (ACs), daunorubicin (DNR) and doxorubicin (DXR)
are two of the most effective drugs known for the treatment of systemic neoplasms
and solid tumours. However, their clinical use is often hampered by their dosedependent
cumulative cardiotoxicity, which leads to irreversible and fatal druginduced
congestive heart failure. The mechanism by which ACs induces heart
damage is not fully understood. Recent reports have indicated that DXR activates
autophagy and ubiquitin proteasome-mediated degradation of specific transcription
factors, however, no reports exists on the effect of ACs on the E3 ubiquitin ligases,
MuRF-1 and MAFbx. The aim of the first part of the study was therefore to
investigate the effect of DNR treatment on the protein and organelle degradation
systems in the heart and to elucidate the signalling mechanisms involved.
Although this model was ideal in allowing the investigation of the signalling pathways
which are affected by DNR, it did not allow for further exploration or manipulation of
signalling pathways that may be of potential benefit in this context. The in vitro model
was therefore used to validate the hypothesis that increased autophagy alleviates
AC-induced cardiotoxicity and delays the onset of cardiomyocyte death. The aims for
the second part of the study were (i) to characterize the effect of DXR in H9C2 cells,
(ii) to determine whether the induction/inhibition of autophagy in combination with
DXR alleviates cytotoxicity and (iii) to investigate the influence of
increased/decreased autophagy in combination with DXR on reactive oxygen
species (ROS) production, mitochondrial function, endoplasmic reticulum (ER) stress
and the ubiquitin proteasome pathway. In the final part of this study, an in vivo model
was used to assess the potential benefit of autophagy in a novel GFP-LC-3 tumour
bearing mouse model of acute DXR-induced cardiotoxicity. Material and Methods: Adult rats were divided into two groups where one group
received six intraperitoneal injections of 2 mg/kg DNR on alternate days and the
other group received saline injections as control. Hearts were excised and perfused on a working heart system the day after the last injection and freeze clamped for
biochemical analysis.
H9C2s were cultured and treated with Bafilomycin A1 (10 nM, inhibitor of autophagy)
for 6 hrs, Rapamycin (50 μM, inducer of autophagy) for 24 hrs, DXR (3 μM) for 24
hrs or a combination of these drugs. Following treatment, cells were harvested and
assessed for cell death, proteolytic activity and oxidative stress using western
blotting, fluorescence microscopy and flow cytometry.
In the final phase of the study, twenty-four female mice were injected at 8 weeks with
a mouse breast cancer cell line (EO771) and after observation of tumour growth,
animals were either treated with one injection (i.p.) of Rapamycin (4 mg/kg), two
injections (i.p.) of DXR (10 mg/kg) or a combination of the two drugs. After the
experimental protocol, mice were terminated and their hearts were rapidly excised.
The hearts were divided cross-sectionally and utilized for biochemical and
histological analyses.
Results and Discussion: DNR treatment significantly attenuated myocardial
function and increased apoptosis in the ex vivo heart model. DNR-induced cardiac
cytotoxicity was associated with the upregulation of two E3 ubiquitin ligases, MuRF-1
and MAFbx as well as a significant increase in two markers of autophagy, beclin-1
and LC-3. These changes observed in the heart were also associated with
attenuation of the PI3-kinase/Akt signalling pathway. The augmentation of autophagy with rapamycin before DXR treatment significantly
reduced cell death in the in vitro model. Indeed, rapamycin treatment demonstrated
to be a vital survival mechanism for acute DXR-induced cardiotoxicity as it
decreased cellular ROS production, improved mitochondrial function and prevented
nuclear translocation of DXR. Moreover, these changes in cardiomyocytes were also
associated with a reduction in the ubiquitin-proteasome pathway (UPP). In the final part of this study, a novel tumour bearing GFP-LC3 mouse model was
developed to confirm the results obtained in the in vitro study. It was demonstrated
that acute DXR-induced cardiotoxicity resulted in increased apoptosis, the inhibition
of autophagy and increased proteolysis via the UPP. These findings were associated
with a reduction in body weight and cardiomyocyte cross-sectional area. The
cardiotoxic effects of DXR were substantially reduced when autophagy was induced
with rapamycin. Taken together, our data strongly indicates that it is possible to
attenuate the cardiotoxic effects of doxorubicin in cancer patients by carefully
controlling the levels of autophagy using rapamycin as adjuvant therapy. / AFRIKAANSE OPSOMMING: Inleiding: Die antrasikliene (AC’s), daunorubisien (DNR) en doksorubisien (DKS), is
twee van die mees effektiewe AC wat bekend is vir die behandeling van sistemiese
neoplasmas en soliede tumore. Hulle kliniese gebruik word egter deur dosis
afhanklike kumulatiewe kardiotoksisiteit benadeel, wat tot onomkeerbare en dodelike
kongestiewe hartversaking kan lei. Die meganisme waardeur AC’s hartversaking kan
veroorsaak, word nog nie ten volle verstaan nie. Onlangse navorsing het aangetoon
dat DKS autofagie en die ubikwitienproteosoom-bemiddelde degradasie van
spesifieke transkripsie faktore aktiveer. Daar is egter geen literatuur wat die effek
van AC’s op die E3-ubikwitienligases, MuRF-1 en MAFbx beskryfnie. Die doel van
hierdie eerste afdeling van die studie is om die effek van DNR behandeling op die
proteïen- en organel degradasie sisteme in die hart te ondersoek en om van die
betrokke seinmeganismes te bepaal.
Alhoewel hierdie model ideaal is om sommige seinweë wat deur DNR geaffekteer
word, te ondersoek, kon seinoordragpaaie wat potensieël voordelig in hierdie
konteks is, nie in bg. model gemanipuleer word nie. Die in vitro model is gebruik om
die hipotese dat verhoogde outofagie AC-geïnduseerde kardiotoksisiteit verlaag en
sodoende seldood verminder, te bevestig. Die doel van hierdie afdeling van die
studie was: (i) om die effek van DKS op H9C2 selle te karakteriseer, (ii) om te bepaal
of die induksie/inhibisie van outofagie in kombinasie met DKS kardiotoksisiteit
verbeter (iii) om die invloed van verhoogde/verlaagde outofagie in kombinasie met
DKS op reaktiwe suurstof species (ROS), mitokondriale funksie, endoplasmiese
retikulum (ER) stress en die ubikwitienproteosoompad te ondersoek. In die finale
deel van hierdie studie, is ‘n in vivo model gebruik om die moontlike voordelige effek
van verhoogde outofagie in ‘n GFP-LC-3 tumor-draende muismodel met akute DKSgeïnduseerde
kardiotoksisiteit, ondersoek.
Materiaal en Metodes: Volwasse rotte is in twee groepe verdeel waar een groep
ses intraperitoneale inspuitings van 2 mg/kg DNR op afwissellende dae ontvang het en die andergroep as ‘n kontrole, ‘n soutoplossing gekry het. Die harte is verwyder
en geperfuseer op ‘n werkende hartsisteem een dag na die laaste inspuiting en
gevriesklamp vir biochemiese analises.
H9C2 selle is vir 6 uurgekweek en behandel met Bafilomisien A1 (10 nM, ‘n autofagie
inhibitor), 24 uur met Rapamisien (50 μM, ‘n autofagie induseerder), 24 uur met DKS
(3 μM) of ‘n kombinasie van hierdie middels. Na behandeling is selle ge-oes vir
analises in seldood, proteolitiese aktiwiteit en oksidatiewe stress deur van westelike
kladtegniek, fluoresensie mikroskopie en vloeisitometrie gebruik te maak.
In die finale fase van hierdie studie is vier en twintig, agt weke oue wyfie muise
ingespuit met ‘n muisborskankersellyn (E0771) en is tumorgroei waargeneem; die
diere is of behandel met een rapamisien inspuiting (i.p) (4 mg/kg), of twee DKS
inspuitings (i.p.) (10 mg/kg) of ‘n kombinasie van die twee middels. Na die
eksperimentele protokol, is die muise van kant gemaak en hulle harte vinnig
verwyder. Die harte is in twee verdeel en gebruik vir biochemiese- en histologiese
analises.
Resultate en Bespreking: DNR behandeling het kardiale funksie betekenisvol
verswak en apoptose in die hart verhoog. DNR-geïnduseerde kardiotoksisiteit is
geassosieer met die opregulering van E3-ligases, MuRF-1 en MAFbx en het ook ‘n
betekenisvolle toename in twee outofagie merkers, beclin-1 en LC-3 veroorsaak.
Hierdie veranderinge wat in die hart waargeneem is, is ook geassosieer met ‘n
onderdrukking van die PI3-kinase/Akt seinweg. Die toename in outofagie met rapamisien voor DKS behandeling het seldood in die
vorm van apoptose betekenisvol verlaag. Daarmee saam het verhoogde outofagie ‘n
noodsaaklike oorlewings meganisme vir akute DKS-geïnduseerde kardiotoksisiteit
gedemonstreer. Die rede hiervoor is dat dit ROS produksie verlaag het,
mitokondriale funksie verbeter het en DKS translokasie vanuit die sitoplasma tot binne die nukleus verhoed het. Hierdie veranderinge in kardiomiosiete is ook met ‘n
afname in die ubikwitienproteosoomseinweg (EPS) geassosieer.
In die finale deel van hierdie studie, is ‘n nuwe tumor-draende muismodel ontwikkel
om die resultate wat in die in vitro studie gekry is, te bevestig. Daar is bewys dat
akute DKS-geïnduseerde kardiomiotoksisiteit aanleiding gegee het tot verhoogde
apoptose, outofagie inhibisie en verhoogde proteolise via die EPS. Hierdie
bevindinge is geassosieer met ‘n verlaging in liggaamsgewig en kardiomiosiet
dwarssnit area. Die kardiotoksiese effekte van DKS is insiggewend verminder as
autofagiege ïnduseer is met rapamisien. Om saam te vat: Ons data bevestig dat dit
moontlik is om die kardiotoksiese effekte van DKS in kanker pasiënte te verminder
deur outofagie vlakke te monitor en te kontroleer deur middel van rapamisien
behandeling as bykomende terapie.
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Impact of TMPRSS2-ERG fusion gene on prostate cancer cell response to chemotherapy, radiotherapy and androgen deprivation therapyOvtcharov, Slav January 2015 (has links)
Many aspects of the mechanisms by which prostate cancer (PCa) progresses from being a confined tumour to advanced metastatic and castration-resistant disease remain unclear. The aim of this study is to evaluate in vitro the potential role of the fusion gene TMPRSS2-ERG in the response of PCa cells to ionising radiation (IR) and androgen deprivation therapy (ADT). This research focused on assessing the presence of the TMPRSS2-ERG transcript across various PCa cell lines and identifying any correlation between the TMPRSS2-ERG transcript and other genes, particularly genes related to DNA damage repair pathways. Several genes involved in cell metabolism and development were found to correlate with TMPRSS2-ERG but not genes involved in DNA repair. In accordance with previous reports, this research confirmed a proliferative advantage for cells expressing ERG. However this project also tested the role of ERG-status in response to chemotherapy, radiation and ADT. The data showed that VCaP and DuCaP cells exposed to low-dose radiation demonstrated decreased viability irrespective of their ERG-status. Similarly ADT decreased the viability of VCaP cells and seemed to neutralise the proliferative advantage of TMPRSS2-ERG positive cells. Stimulation with dihydrotestosterone caused increased radioresistance of TMPRSS2-ERG positive cells. Treatment with taxanes showed stronger effect on cells with lower ERG expression. This work suggests that the proliferative advantage conferred by ERG overexpression in in vitro models can be neutralised by castration and IR.
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Neurodegeneration and brain cancer : a longitudinal field study of rest-activity and sleepWams, Emma J. January 2012 (has links)
This thesis investigates rest-activity and sleep profiles in neurodegeneration and brain cancer. Study 1 comprised longitudinal field assessments of rest-activity, sleep and memory in controls and memory-impairment individuals with: subjective memory complaint (SMC), amnestic mild cognitive impairment (aMCI), mild and moderate Alzheimer’s disease (AD). Four questions were addressed: (1) is SMC a prodromal stage of AD? (2) do characteristics of SMC predict future decline? (3) does cholinergic medication (ChEI) impact rest-activity and sleep of moderate AD patients? and (4) are there factors predicting response to ChEI? Study 2 assessed rest-activity and melatonin rhythms in a brain cancer patient (JJB), and post-mortem analysis of brain tissue assessed infiltration of cancer cells on the circadian clock (SCN). Both studies used questionnaires, cognitive tests, electroencephalography and actigraphy simultaneously at patients’ homes. In Study 1, the SMC group showed a reduced activity amplitude to be correlated with increasing memory impairment severity, lower sleep quality and efficiency. Increased sleep fragmentation was observed in all memory-impaired groups, although not correlated to impairment severity. Increased fragmentation of rest-activity rhythm correlated with increasing memory impairment severity in all groups except SMC. Following ChEI medication with donepezil, moderate AD patients showed increased sleep fragmentation, probably due to potentiation of available acetylcholine known to maintain arousal. Higher daytime-activity and lower activity in the rest-phase, when drug-naïve, predicted improved cognition following ChEIs. In Study 2, cancer cell infiltration of the patient’s SCN was confirmed. However, a robust circadian rest-activity period with a misaligned melatonin phase, was recorded, indicating that the effects of partial SCN lesions in humans are complex and this result was possibly in part are due to the masking effect of social behaviour.
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The buckling of capillaries in tumoursMacLaurin, James Normand January 2011 (has links)
Capillaries in tumours are often severely buckled (in a plane perpendicular to the axis) and / or chaotic in their direction. We develop a model of these phenomena using nonlinear solid mechanics. Our model focusses on the immediate surrounding of a capillary. The vessel and surrounding tissue are modelled as concentric annulii. The growth is dependent on the concentration of a nutrient (oxygen) diffusing from the vessel into the tumour interstitium. The stress is modelled using a multiplicative decomposition of the deformation gradient F=F_e F_g. The stress is determined by substituting the elastic deformation gradient F_e (which gives the deformation gradient from the hypothetical configuration to the current configuration) into a hyperelastic constitutive model as per classical solid mechanics. We use a Blatz-Ko model, parameterised using uniaxial compression experiments. The entire system is in quasi-static equilibrium, with the divergence of the stress tensor equal to zero. We determine the onset of buckling using a linear stability analysis. We then investigate the postbuckling behaviour by introducing higher order perturbations in the deformation and growth before using the Fredholm Alternative to obtain the magnitude of the buckle. Our results demonstrate that the growth-induced stresses are sufficient for the capillary to buckle in the absence of external loading and / or constraints. Planar buckling usually occurs after 2-5 times the cellular proliferation timescale. Buckles with axial variation almost always go unstable after planar buckles. Buckles of fine wavelength are initially preferred by the system, but over time buckles of large wavelength become energetically more favourable. The tumoural hoop stress T_{ThetaTheta} is the most invariant (Eulerian) variable at the time of buckling: it is typically of the order of the tumoural Young's Modulus when this occurs.
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Regulation of stemness and differentiation in colorectal cancerGandhi, Shaan-Chirag Chandrahas January 2010 (has links)
The cancer stem cell (CSC) model of carcinogenesis and progression posits that within a tumor lies a subpopulation of cells that solely possess the ability to initiate a tumor and to differentiate into tumor cell lineages. Although the behavior of such cells is known, the challenge is to identify factors that characterize the CSC subpopulation. In this thesis, cell lines were identified that, when grown in three-dimensions, gave rise to organized colonies containing lumens originating from differentiating cells (“lumen lines”) and to densely-packed, spherical colonies originating from non-differentiating cells (“dense lines”). A microarray comparison of the pair identified genes upregulated in dense lines, including CD55 and BMI1, and in lumen lines, including CDX1 (Chapter 3). CD55 was used to isolate CD55high CSCs via flow cytometry that are able to self-renew, differentiate, initiate more colonies, proliferate more rapidly and exhibit an increased G2/M cell cycle population as opposed to unfractionated cells. Furthermore, the CD55high cells were able to give rise to more differentiated, lumen colonies in vitro, indicating that CD55 enriches for cells possessing a capacity to differentiate, and were able to enrich the CD24highCD44high putative CSC population further (Chapter 4). CDNA induction of BMI1 and CDX1 expression led to increased clonogenicity/proliferation and decreased clonogenicity/proliferation, respectively, and incorporation of a CDX1 reporter construct into the SW1222 cell line identified CDX1+ cells as a low-expressing population of CD55 (Chapter 5). Finally, co-culture of cell lines in an in vivo-like environment with intestinal myofibroblasts promoted the CSC population by enhancing clonogenicity, proliferation and expression of CD55 (Chapter 6). The results of this thesis implicate CD55 as a potent marker of colorectal cancer stemness, link the expression of BMI1 and CDX1 to cancer stemness and differentiation, respectively, and identify a role for the in vivo stem cell niche in maintaining the CSC population.
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Modulating the immune system by amino acid depletion : IDO and beyondVallius, Laura I. January 2011 (has links)
Amino acid availability plays an important role in modulating the activity of T-cells. One of the pathways employed by T-cells to sense nutrient levels is the “mammalian target of rapamycin” (mTOR) pathway that is inhibited in response to nutrient depletion. Indoleamine 2,3-dioxygenase (IDO) is the first and rate-limiting enzyme along the tryptophan catabolising kynurenine pathway. T-cells are very sensitive to lack of this essential amino acid in their microenvironment and this confers strong immunomodulatory properties to cells expressing active IDO. It therefore has a significant physiological role as a homeostatic mechanism used in mammalian organisms to dampen excessive activation of the immune system but is also used as an immune evasion mechanism by many cancers. In this study, we investigated the IDO inhibitory properties and mechanism of action of the tryptophan metabolite 3-hydroxyanthranilic acid (3-HAA) that potentially forms a negative feedback loop in the kynurenine pathway. We studied the molecule in enzymatic assays, in live cells and discovered that it inhibits IDO in an indirect way via the formation of hydrogen peroxide. Secondly, we looked at the effects of tryptophan and its metabolites on T-cell proliferation and mTOR activity, and discovered a metabolite that inhibits T-cell proliferation. Lastly we examined mechanisms of T-cell suppression employed by myeloid derived suppressor cells (MDSCs), focusing on their ability to deplete amino acids from their microenvironment. We were able to exclude tryptophan consumption as a suppressive mechanism and established that by manipulating extracellular concentrations of several amino acids other than arginine and cysteine – that are known to be utilised by MDSCs - we were able to reduce their inhibitory properties. In summary, we have described in detail how 3-HAA inhibits IDO in in vitro assays, outlined how some tryptophan metabolites can inhibit T-cell proliferation, and clarified aspects of suppressive mechanism employed by MDSCs.
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