"Gene expression profiling of mantle cell lymhoma in leukemic phase with oligonucleotide microarrays" / "Análise do perfil de expressão gênica do linfoma de células do manto em fase leucêmica com microarrays de oligonucleotídeos"
AUTOR(ES)
Edgar Gil Rizzatti
DATA DE PUBLICAÇÃO
2005
RESUMO
Mantle cell lymphoma is associated with the translocation t(11;14)(q13;32) and overexpression of cyclin D1. Mantle cell lymphoma is predominantly disseminated at diagnosis and a frank leukemic phase is detected in one third of patients. The pre-germinal-center naive B-cells, which populate the mantle zone of the secondary lymphoid follicles, are the cells of origin of mantle cell lymphoma. Overexpression of cyclin D1 is not sufficient by itself to cause lymphoma, and a better understanding of the additional molecular lesions may provide insights toward new therapeutic approaches. In this context, large scale gene expression studies may be useful in the investigation of such additional molecular lesions. However, the great majority of mantle cell lymphoma cases studied by these methods to date had the genetic material harvested from lymph nodes, which have a variable proportion of normal cells from the lymphoid stroma. It is therefore not known how many genes identified as differentially expressed in mantle cell lymphoma by tumor versus normal experiments are cell-autonomous rather than dependent on the tumor microenvironment. To address this issue, we compared the gene expression profile of mantle cell lymphoma cells and normal naive B-cells using oligonucleotide microarrays. Lymphoma cells and naive B-cells (IgD+CD38±CD27-) were highly purified, by magnetic activated cell sorting, from the peripheral blood of patients with mantle cell lymphoma in the leukemic phase and from tonsils of normal individuals, respectively (purity >95% in all samples). Three individuals were selected for each group and experiments were performed in replicates using the Amersham CodeLink Human UniSet I Bioarrays, with 10,000 genes. We identified 106 genes differentially expressed with a fold change of at least three-fold, 63 induced and 43 repressed in mantle cell lymphoma in comparison with naive B-cells. Ten genes were selected (six induced and four repressed in lymphoma cells) for quantification by real-time RT-PCR in non-purified peripheral blood samples from 21 patients with mantle cell lymphoma in the leukemic phase, as well as in 14 patients with other chronic lymphoproliferative diseases and seven normal individuals. Microarray results were confirmed by real-time RT-PCR for all selected genes and expression values of the TLR1 gene as quantified by this method showed significant correlation with patient survival in mantle cell lymphoma. In addition to the identification of several modulated genes in mantle cell lymphoma at cellular level, this study revealed that some genes functionally connected through apoptosis or the PI3K/AKT, WNT and TGFβ signaling pathways are aberrantly expressed in mantle cell lymphoma. These results add original data to the molecular pathogenesis of mantle cell lymphoma and point to specific molecular signaling pathways related to inhibition of apoptosis as potential targets for new therapeutic approaches.
ASSUNTO(S)
linfoma de células do manto linfoma não-hodgkin microarrays microarrays mantle cell lymphoma expressão gênica non-hodgkins lymphoma gene expression profiling
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