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Apoptosis and apoptosis regulating proteins and factors in small and large cell lung carcinomaEerola, A.-K. (Anna-Kaisa) 30 September 1999 (has links)
Abstract
Aptosis denotes a biochemically and morphologically distinct
chain of events leading to self-destruction of cell. It is pivotal
in the maintenance of tissue homeostasis and also plays a role in neoplasm.
In this work, the extent of apoptosis and apoptosis regulating proteins
and factors was studied in a total of 94 patients operated for lung
carcinoma, including 56 small cell lung carcinomas (SCLC) and 38
large cell lung carcinomas (LCLC). The extent of apoptosis was determined
by detecting and counting the relative and absolute numbers of apoptotic
cells and bodies using 3'- end labelling of the apoptotic
DNA. The extent of apoptosis in SCLC was compared with the cell proliferation
activity as determined by Ki-67 immunohistochemistry, with the volume
density of necrosis and with the occurrence of immunohistochemically
detectable p53 and bcl-2 proteins. In order to test the hypothesis
that increased apoptotic activity is connected with neuroendocrine differentiation
and with low differentiation degree in LCLC and that it is regulated
by bcl-2 family proteins, the extent of apoptosis and tumour necrosis
was analysed in relation to the expression of bcl-2 family proteins
bcl-2, mcl-1, bax and bak. Apoptosis, tumour infiltrating lymphocytes
(TILs), and angiogenesis are important factors that contribute to
tumour growth. In the present study immunohistochemical methods
were used to investigate the relationships of these factors and
their role in the prognosis of the patients with LCLC and SCLC.
A remarkably high apoptotic activity was detected in both
SCLC and LCLC. The mean apoptotic index in SCLC was 2.70 % and
in LCLC 2.49 %. Exceptionally high proliferation activity
and high percentage of tumour necrosis was seen in SCLC. 58 % of
SCLC showed more than 40 % of Ki-67 positive nuclei, and
tumour necrosis was seen in 83 % of the cases. P53 protein
accumulation was detected in 38 % and bcl-2 expression
in 50 % of SCLC. The extent of apoptosis in SCLC was inversely
related to tumour necrosis and p53 protein accumulation. In LCLC,
bcl-2 expression was detected in 40 % of the cases. It
was associated with neuroendocrine differentiation and predicted favourable
prognosis of the patients. A high number of T cells and macrophages
with a small number of B cells was detected in both SCLC and LCLC.
The occurrence of intratumoural cytotoxic CD8 cells was associated
with the occurrence of apoptotic bodies in SCLC. The increased number
of intratumoural T cells, CD8-positive cells and macrophages predicted
favourable prognosis of the patients with SCLC. In LCLC, an increased
number of B cells and macrophages, but not T cells, was associated
with better survival.
Iaddition to tumour cells, numerous apoptotic bodies could
also be found within alveolar macrophages within and close to tumour
tissue. In order to test whether such cells could be found in sputum
smears and if their presence could be utilised as a marker of malignancy
in tumour diagnosis, the occurrence of alveolar macrophages with
apoptotic bodies (AMWABs) was analysed in 84 sputum samples and
13 broncho-alveolar lavage (BAL) specimens from patients with and
without lung carcinoma. AMWABs could be found in cytological samples
of the patients with lung carcinoma. In sputum and BAL specimens,
enhanced apoptosis, as measured by an increased number of AMWABs
reflected and was indicative of malignancy. This was also true for
cytological specimens of the patients even when the actual malignant
cells were not found. Therefore the AMWABs served as a marker of
pulmonary malignancy.
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Prognostic markers in oropharyngeal cancersOguejiofor, Kenneth Kenechukwu January 2016 (has links)
Introduction: Human papillomavirus (HPV) is changing the prevalence, survival and treatment paradigms in oropharyngeal squamous cell carcinoma (OPSCC). Improved survival of patients with HPV positive compared to HPV negative OPSCC has led to trials of treatment de-escalation. Current HPV detection methods are imprecise, therefore standardised assessment of transcriptionally active HPV in OPSCC is required. Furthermore, the differences in immune characteristics and/or the hypoxia response/effects could explain observed differences in prognosis between HPV positive and negative OPSCC. Rigorous HPV detection and subsequent biomarker evaluation should provide additional information required before introduction of treatment de-escalation in broad patient groupings. Methods: The study cohort was 218 patients with OPSCC who received radiotherapy with curative intent. HPV status was determined on pre-treatment, formalin-fixed paraffin-embedded blocks using: 1) polymerase chain reaction (PCR); 2) in-situ hybridisation (ISH) and 3) immuno-histochemistry (IHC). QuantiGene multiplex assay was designed to detect mRNA of reference sequences of the common high-risk HPV types (16, 18, 33, 35, 45, 52 and 58). HPV detection methods were compared with mRNA quantification. Multimarker IHC of immune cell markers using chromogenic and fluorescent staining was performed, analysed and compared with single marker IHC using automated multispectral image analysis. A validated multiplex IHC method was used for a) chromogenic (CD3, CD4, CD8, and FoxP3) and b) fluorescent (CD8, CD68 and PD1/PD-L1) evaluation in tumour and stroma compartments. Single marker IHC was used to investigate tumour hypoxia markers (HIF-1α and CA-IX) in HPV positive and negative OPSCC. Results: p16 IHC and ISH were the most sensitive and specific, respectively, for classifying HPV status. The combination of the three tests had the highest positive/negative predictive values compared with QuantiGene mRNA detection. Multiplex validation showed that, for serial sections up to 6 μm apart, there were highly significant correlations (P<0.0001) between single and multiplex counts for both chromogenic and fluorescent IHC. Overall there was less variation in cell counts with fluorescent staining when compared to chromogenic staining. Multiplex IHC of TILs in HPV positive and negative OPSCC showed higher infiltration in both tumour and stromal areas of CD3+CD4+ and CD3+CD8+ T cells but not CD4+FoxP3 Tregs in HPV positive compared with HPV negative OPSCC. Only CD3+CD8+ stromal and not tumour area infiltration was associated with increased survival (P=0.02). PD-L1 expression was higher in HPV negative OPSCC and this was related to macrophage (CD68) expression of PD-L1. In HPV negative tumours infiltration with CD68+PD-L1 was associated with a good prognosis. HPV negative patients had higher expression of HIF-1α but not CA-IX. High expression of both markers was associated with a poor prognosis irrespective of HPV status. Conclusions: There are other prognostic factors operating in the larger subdivision of HPV positive and negative OPSCC. Precise HPV detection and inclusion of other prognostic factors is required before treatment de-escalation is used. Expression of immune inhibitory factors (PD1/PD-L1) alone without contextualisation with immune cell density is insufficient for patient prognostication and potential selection for therapy using immune checkpoint inhibitors. Hypoxia modification of radiotherapy should be explored in both HPV positive and negative OPSCC.
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CD8+FoxP3+ T cells: A new player in the immune response to ovarian cancerKost, Sara E. F. 28 November 2013 (has links)
Introduction Tumour-infiltrating lymphocytes (TIL) are an important prognostic indicator in high-grade serous ovarian carcinoma (HGSC). Certain types of TIL (in particular CD8+ effector T cells) predict better outcomes, whereas others (most notably CD4+CD25+FoxP3+ regulatory T cells; Tregs) predict worse outcomes. An unconventional subset of CD8+FoxP3+ T cells has been reported to be involved in autoimmunity and in immune response to several cancers. While the functional significance of CD8+FoxP3+ TIL remains poorly understood, they were associated with effective anti-tumour responses in a murine tumour model.
Hypothesis CD8+FoxP3+ TIL are present in a subset of cases of HGSC and correlate with a strong immune response and increased patient survival.
Experimental Design Multi-colour immunohistochemistry (IHC) was performed on a cohort of 44 primary HGSC specimens to enumerate and locate CD8+FoxP3+ TIL in comparison to CD8+FoxP3- and CD8-FoxP3+ TIL. Triple-colour IHC methodology was developed to further assess the phenotype of CD8+FoxP3+ TIL, including the measurement of additional markers CD4 and CD25 (classical markers of Tregs), Ki-67 (a marker of proliferation), and TIA-1 (a marker of cytotoxic potential). Intraepithelial versus stromal location was determined by staining adjacent sections for the epithelial marker pan-cytokeratin. Survival analysis was performed using a cohort of 188 cases of HGSC. Multi-colour staining was resolved using the Nuance™ multispectral imaging system in conjunction with Metamorph™ software. Survival analysis was performed using Kaplan-Meier and log rank tests.
Results CD8+FoxP3+ cells were found in 60% of 44 cases of HGSC, in variable proportions ranging from 0.2 - 7.9% of CD8+ TIL and 0.5 – 12.7% of FoxP3+ TIL. CD8+FoxP3+ TIL were found to be either CD4+ (38.8%) or CD4- (61.2%). The majority of CD8+FoxP3+ TIL were also found to be CD25-TIA-1+Ki-67-, more closely resembling their CD8+FoxP3- counterparts. CD8+FoxP3+ TIL were found mainly in intraepithelial regions and were positively associated with patient survival (progression free survival; P = 0.0396).
Conclusions CD8+FoxP3+ TIL are a component of the host immune response to HGSC. They appear to have a non-proliferative effector phenotype, consistent with an active role in the anti-tumour response. CD8+FoxP3+ TIL are associated with increased patient survival. An improved understanding of this new TIL subset may inform future immunotherapeutic strategies for this challenging malignancy. / Graduate / 0982 / sarakost@hotmail.com
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L'impact de l'infiltration lymphocytaire sur le pronostic de l'adénocarcinome du pancréasMcNicoll, Yannic 06 1900 (has links)
L’objectif principal de cette étude est de déterminer la valeur pronostique de l’infiltrat lymphocytaire dans l’adénocarcinome du pancréas.
Les densités des lymphocytes T CD3+, CD4+, CD8+, FOXP3+ et CD45RO+ intratumoraux (T) et péritumoraux (PT) de 111 spécimens ont été mesurées avec des micromatrices tissulaires. Un Index Lymphocytaire (IL) a été créé basé sur les valeurs des CD4+ T, CD8+ PT et le ratio CD3+ T/PT regroupant les patients selon que les tumeurs présentaient aucune (IL---), 1 à 2 (IL+/-) ou les 3 caractéristiques immunitaires favorables (IL+++). La survie médiane des patients atteints d’un cancer du pancréas est significativement différente selon la catégorie d’index lymphocytaire; elle était de 14 mois pour IL---, de 19 mois pour IL +/- et de 29 mois pour IL+++ (p=0,01). L’IL est un facteur indépendant de survie en analyse multivariée ainsi que la différenciation tumorale et l’utilisation d’un traitement adjuvant.
L’IL est un facteur pronostique de survie des adénocarcinomes du pancréas réséqués et devrait pouvoir permettre une meilleure classification des patients. / The main objective of this project was to determine the prognostic significance of T-lymphocytes densities in pancreatic adenocarcinoma.
Using tissue microarrays, CD3+, CD4+, CD8+, CD45RO+, and FOXP3 T-cells were quantified by immunohistochemistry in the intratumoral (T) and peritumoral (PT) compartments of 111 specimens.
An immune score (IS) based on T CD4+ and PT CD8+ counts and T/PT CD3+ ratio grouped patients into IS---, IS+/- and IS+++ if none, 1 or 2, or all 3 of the favorable immune features were present, respectively. Patients have different overall survival (OS) depending on their IS status. Patients IS--- have a median OS of 14 months and of 19 months and 29 months for those IS+/- and IS+++ respectively (log-rank p=0.01). By multivariate analysis, IS was independently associated with survival as were the histological grade and adjuvant therapy.
An immune score that combines specific T-cell location and density may have prognostic value in patients with resected pancreatic adenocarcinoma, independently from current pathologic features.
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