Comparative Genome-Scale Analysis of Gene Expression Profiles in T Cell Lymphoma Cells during Malignant Progression Using a Complementary DNA Microarray

Sy, Li; Ross, Douglas T.; Kadin, Marshall E.; Brown, Patrick O.; Wasik, Mariusz A.

doi:10.1016/s0002-9440(10)64073-4

Cited by 57 publications

(31 citation statements)

References 38 publications

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“…These cells are representative of the primary tumors and retain the features of the original lymphoma. 26 All 3 PCALCL cells highly expressed SATB1, and Mac-2A and -2B cells showed significantly higher expression ( Figure 1C), whereas the other CD30…”

Section: Statisticsmentioning

confidence: 96%

SATB1 overexpression promotes malignant T-cell proliferation in cutaneous CD30+ lymphoproliferative disease by repressing p21

Wei

Zhang

et al. 2014

Blood

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Section: Statisticsmentioning

confidence: 96%

SATB1 overexpression promotes malignant T-cell proliferation in cutaneous CD30+ lymphoproliferative disease by repressing p21

Wei

Zhang

et al. 2014

Blood

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“…Analysis of several B-NHLs series has led to the definition of molecular subgroups with specific outcomes (Alizadeh et al, 2000;Rosenwald et al, 2002;Shipp et al, 2002;Thieblemont et al, 2004). In contrast, only a limited number of T-cell neoplasms have been investigated using microarrays, including mycosis fungoides (Tracey et al, 2003), leukemic phase of cutaneous T-NHL (Kari et al, 2003), cell lines derived from T-cell malignancies (Li et al, 2001;Fillmore et al, 2002), or PTCL (Martinez-Delgado et al, 2004). A recent profiling analysis was focused on the comparison between PTCL and T-lymphoblastic lymphoma (T-LBL) types (Martinez-Delgado et al, 2004), but a molecular classification of PTCL entities has not yet been reported.…”

Section: Introductionmentioning

confidence: 99%

Gene expression profiling identifies molecular subgroups among nodal peripheral T-cell lymphomas

et al. 2005

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“…15,16 This approach has now been used successfully by a number of groups to identify distinct gene expression patterns in various tumors, tumor cell lines, and disease states. [17][18][19][20][21][22][23][24] In this study, we use cDNA microarrays to examine the global transcriptional profiles of four t(14;18)-positive lymphoma-derived cell lines and demonstrate that they can be readily distinguished from two t(11;14)-positive mantle-cell lymphoma cell lines on the basis of their respective expression profiles. We also demonstrate the utility of real-time quantitative fluorescence RT-PCR for validation of microarray expression data and show how this approach may be used to identify differentially expressed genes that could be involved in the development of t(14;18)-positive NHLs.…”

mentioning

confidence: 99%

Microarray Analysis of B-Cell Lymphoma Cell Lines with the t(14;18)

Robetorye

Bohling

Morgan

et al. 2002

The Journal of Molecular Diagnostics

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The t(14;18) is the most common genetic alteration in follicular lymphoma, and is detectable in a subset of diffuse large B-cell lymphomas (DLBCL), resulting in over-expression of the anti-apoptotic protein BCL-2. Although the t(14;18)-induced over-expression of BCL-2 is an important step in lymphomagenesis,The t(14;18) is a frequent chromosomal alteration in nonHodgkin's lymphomas (NHL), occurring in up to 90% of follicular lymphomas 1 and 20 to 30% of diffuse large B-cell lymphomas (DLBCL). 2,3 This translocation is acquired early in B-cell development and results in juxtaposition of the bcl-2 gene on chromosome 18 with the immunoglobulin heavy-chain locus on chromosome 14, resulting deregulated expression of a structurally intact BCL-2 protein. 4 -8 BCL-2 is located in the inner mitochondrial membrane and functions as an anti-apoptotic protein that inhibits programmed cell death, 9 resulting in accumulation of B-lymphocytes by virtue of increased cell survival. 9 -11 Although the t(14;18)-induced over-expression of bcl-2 is an important step in lymphomagenesis, this alteration alone is not sufficient to produce malignant lymphoma. This has been demonstrated in in vitro gene transfer experiments using cell lines and transgenic mice studies in which forced over-expression of bcl-2 was insufficient to cause lymphoma. 12,13 Indeed, low numbers of t(14; 18)-carrying cells can be detected in benign lymphoid tissues such as follicular hyperplasias and the hyperplastic tonsils of young children. 14 These studies indicate that cumulative genetic and cellular alterations superimposed on the t(14;18) are necessary for the development of lymphoma and underscore the need for further analysis of t(14;18)-containing DLBCLs to identify additional genes involved in lymphomagenesis and progression.cDNA microarray technology allows large scale parallel analyses of gene expression and permits simultaneous comparison of the relative gene expression levels of several thousand genes in different cell types. 15,16 This approach has now been used successfully by a number

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Comparative Genome-Scale Analysis of Gene Expression Profiles in T Cell Lymphoma Cells during Malignant Progression Using a Complementary DNA Microarray

Cited by 57 publications

References 38 publications

SATB1 overexpression promotes malignant T-cell proliferation in cutaneous CD30+ lymphoproliferative disease by repressing p21

SATB1 overexpression promotes malignant T-cell proliferation in cutaneous CD30+ lymphoproliferative disease by repressing p21

Gene expression profiling identifies molecular subgroups among nodal peripheral T-cell lymphomas

Microarray Analysis of B-Cell Lymphoma Cell Lines with the t(14;18)

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