Literature DB >> 7680404

Stroma-supported immunocytometric assay (SIA): a novel method for testing the sensitivity of acute lymphoblastic leukemia cells to cytotoxic drugs.

D Campana1, A Manabe, W E Evans.   

Abstract

The accuracy of drug-sensitivity assays for neoplastic cells depends on the ability to sustain cell survival in vitro, but cells in most cases of acute lymphoblastic leukemia (ALL) rapidly die by apoptosis in culture. We recently reported that allogeneic bone marrow stromal layers support long-term culture of ALL cells. We now describe the standardization of a novel drug-sensitivity assay for ALL lymphoblasts maintained on stromal layers, in which the viability of treated and untreated cells is compared using flow cytometry. Cultures were performed in U-bottomed 96-well plates: 2 x 10(4) stromal cells per well produced rapidly confluent layers which supported the survival of ALL blasts. In four ALL cases studied, 68.8-106% (median 94.8%) of the lymphoblasts originally seeded were recovered after 7 days of culture, in contrast to < 5% recovered in the absence of stroma. Sensitivity to five antileukemic drugs was tested at the indicated concentrations: vincristine (0.001-1 microgram/ml); dexamethasone (0.001-100 microM); 6-thioguanine (0.078-20 micrograms/ml); teniposide (0.001-10 microM); cytosine arabinoside (0.039-10 microM). After 4 days of culture, cells were labeled with CD19 monoclonal antibody and analyzed by flow cytometry. The concentration of each antileukemic agent producing 50% cytotoxicity (LC50) was determined for each patient by fitting a sigmoid model to the drug concentrations versus percentage viability data. Clinically relevant drug concentrations produced cytotoxic effects, and ALL blast sensitivity varied considerably among patients. We conclude that this is an informative method of systematically evaluating drug sensitivity in ALL patients.

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Year:  1993        PMID: 7680404

Source DB:  PubMed          Journal:  Leukemia        ISSN: 0887-6924            Impact factor:   11.528


  9 in total

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3.  A Dexamethasone-regulated Gene Signature Is Prognostic for Poor Survival in Glioblastoma Patients.

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4.  Mesenchymal cells regulate the response of acute lymphoblastic leukemia cells to asparaginase.

Authors:  Shotaro Iwamoto; Keichiro Mihara; James R Downing; Ching-Hon Pui; Dario Campana
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5.  Integrated analysis of CRLF2 signaling in acute lymphoblastic leukemia identifies Polo-like kinase 1 as a potential therapeutic target.

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6.  Stroma-supported culture in childhood B-lineage acute lymphoblastic leukemia cells predicts treatment outcome.

Authors:  M Kumagai; A Manabe; C H Pui; F G Behm; S C Raimondi; M L Hancock; H Mahmoud; W M Crist; D Campana
Journal:  J Clin Invest       Date:  1996-02-01       Impact factor: 14.808

7.  Ligation of CD38 suppresses human B lymphopoiesis.

Authors:  M Kumagai; E Coustan-Smith; D J Murray; O Silvennoinen; K G Murti; W E Evans; F Malavasi; D Campana
Journal:  J Exp Med       Date:  1995-03-01       Impact factor: 14.307

8.  Effect of Aplidin in acute lymphoblastic leukaemia cells.

Authors:  E Erba; M Serafini; G Gaipa; G Tognon; S Marchini; N Celli; D Rotilio; M Broggini; J Jimeno; G T Faircloth; A Biondi; M D'Incalci
Journal:  Br J Cancer       Date:  2003-08-18       Impact factor: 7.640

Review 9.  Proteomics-based discovery of biomarkers for paediatric acute lymphoblastic leukaemia: challenges and opportunities.

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  9 in total

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