Haematologica 2003 - Supplements

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terminal kinase (JNK) pathway which controls osteoclast proliferation. The important function of TRAF6 in signal transduction provides us an ideal target for enhancing the cell killing of MM cells and inhibiting bone turnover initiated by osteoclast activity. We have generated two human TRAF6 dsRNA by construction in vitro for Target 1 TRAF6 mRNA sequence 5’-AAACTGTGAAA ACAGCTGTGG-3’ and Target 2 TRAF6 mRNA Sequence 5’- AGTATGAATGCCCCATCTGC - 3’, The apoptosis and cell proliferation assays showed that Target-1 dsRNA inhibited MM cell proliferation in a dosedependent manner. The Target-2 dsRNA did not produce detectable inhibition of MM cell proliferation. Only the Target-1 dsRNA induced MM cell apoptosis. In contrast, the Target-2 dsRNA and the transfection reagent control vector did not induce cell apoptosis. We tested that whether silence Target-1 TRAF6 mRNA could inhibit NF-kB gene expression induced by IL-1. The 8226 MM cells were transduced of either 100nM TRAF6 or 100nM GAPDH dsRNA for 72 hours and then the cells were incubated with IL-1 for 0, 15, 30, and 60min. The cells were lysates and the total RNA or protein was detected by RT-PCR or western blot. The result showed that amount of NF-kB mRNA or activated NF-kB was significantly increased after 30 minute IL-1 stimulation while NF-kB dropped to normal level after 60 minutes. In contrast, in cells that received TRAF6 dsRNA, the amount of phosphor-NF-kB is no changed It has been clear that NF-kB specific response to TRAF6 knocked down by silence TRAF6 mRNA. We sought further to determine whether TRAF6 RNAi could inhibit NF-kB trigger function on luciferase activity. Using luciferase vector to monitor the activation of NF-kB signal transduction pathway. PNF-kB-Luc is designed to measure the binding of NF-kB to k enhancer, providing a direct measurement of activation this pathway. PTAL-Luc is ideal for use as a negative control vector. In view of the results showed that IL-1 stimulation of the double transfected cells at 30 minute result in a significant induction of luciferase by NF-kB releasing. Furthermore, this induction was abolished when TRAF6 mRNA was silenced by dsRNA. Multiple nuclear cells (pre-osteoclast) were decreased after silence TRAF6 when monocytes stimulated with RANKL and m-SCF. For future studies, we would like to use SCID-hu murine models of human myeloma to further develop this therapeutic strategy in relevant pre-clinical in vivo models. The in vitro studies outlined in this proposal will certainly significantly advance the understanding of this adapter protein in the pathogenesis and give us more impetus to target this protein for future therapeutic manipulation for patients with multiple myeloma. 12. Vaccination strategies in multiple myeloma 402 NY-ESO-1 AND MAGE-A3 ARE HIGHLY EXPRESSED IN MYELOMA PATIENTS WITH ABNORMAL CYTOGENETICS AND/OR RELAPSE Sushil K. Gupta, Fenghuang Zhan, Pei Lin, Jan V. Droogenbroeck*, Ramesh B. Batchu, Friedel Nollet*, Susann M Szmania, Amberly Moreno, Nancy Rosen, Guilio Spagnoli†,Bart Barlogie, Guido Tricot, John Shaughnessy and Frits van Rhee Myeloma Institute for Research and Therapy, University of Arkansas for Medical Sciences, Little Rock, AR U.S.A. *AZ Sint Jan, Department of Hematology, Brugge, Belgium. †Department of Surgery, University of Basel, Switzerland. Despite recent successes with chemotherapy and tandem autologous PBSCT, myeloma remains largely incurable. This highlights the need for novel, synergistic therapies, such as immunotherapy, which may reduce myeloma relapse. Using micro-array and immunohistochemical (IHC) staining, we have examined the expression of two potential targets for immunotherapy, NY-ESO-1 and MAGE-3. Purified myeloma cells were studied by micro-array (n=335), micro-array and IHC on corresponding biopsy (n=20), or IHC alone (n=19, 35 biopsies). Micro-array analysis of 335 patients revealed that expression of NY-ESO-1 and MAGE-A3 is related to the stage of myeloma. The frequency of expression of NY-ESO-1 and MAGE-A3 in MGUS, smoldering myeloma and newly diagnosed myeloma patients eligible for Total Therapy II (TT II) was 4.5%, 5.9% and 20.5% (NY-ESO-1) and 9.1%, 11.8% and 26.2% respectively (MAGE-A3). The presence of abnormal cytogenetics influenced the expression of both antigens. Newly diagnosed TT II trial patients with abnormal cytogenetics were more likely to express NY-ESO-1 and MAGE-A3 cRNA (NY-ESO-1 60% vs. 30.9%, p=0.004; MAGE-A3 65.8% vs. 27.5%, p=1.16x10-6). The percentage NY-ESO-1/MAGE-3 positive plasma cells at the protein level (IHC) was similarly correlated with abnormal cytogenetics. Both antigens (micro-array) were expressed in >50% of relapsed patients (NY-ESO-1 50%, p=8.8x10-9 and MAGE-A3 58.3%, p= 4.5x10-9). Strikingly, 100% patients with abnormal cytogenetics at relapse expressed NY-ESO-1 and MAGE-A3 (p=6.09x10-6 & 3.25x10-6). All these biopsies also stained positive by IHC for NY-ESO-1 and MAGE-A3. 13 patients were studied at diagnosis and at relapse. All biopsies positive at diagnosis by IHC for NY-ESO-1 or MAGE-A3 were positive for both antigens at relapse. The percentage NY-ESO-1 and MAGE-A3 positive myeloma cells in the biopsies was high (>50-90% positive plasma cells; 89% biopsies for NY-ESO-1 and 87% MAGE-A3). Double staining experiments are in progress to test whether the same myeloma cells are positive for both NY- ESO-1 and MAGE-A3. Expression of NY-ESO-1 and MAGE-A3 could be upregulated in myeloma cell-lines by incubating with the hypomethylating agent, decitabine. There was a significant increase in expression of NY-ESO-1 and MAGE-A3 after incubation with decitabine of the NY-ESO-1 and MAGE-A3 negative myeloma cell line U-937 by real-time PCR. In conclusion, NY-ESO-1 and MAGE-A3 are highly expressed in myeloma with abnormal cytogenetics and relapsed myeloma. These antigens can therefore be used as immunotherapy for myeloma with abnormal cytogenetics. Alternatively, NY-ESO- S267
terminal kinase (JNK) pathway which controls osteoclast proliferation. The important function of TRAF6 in signal transduction provides us an ideal target for enhancing the cell killing of MM cells and inhibiting bone turnover initiated by osteoclast activity. We have generated two human TRAF6 dsRNA by construction in vitro for Target 1 TRAF6 mRNA sequence 5’-AAACTGTGAAA ACAGCTGTGG-3’ and Target 2 TRAF6 mRNA Sequence 5’- AGTATGAATGCCCCATCTGC - 3’, The apoptosis and cell proliferation assays showed that Target-1 dsRNA inhibited MM cell proliferation in a dosedependent manner. The Target-2 dsRNA did not produce detectable inhibition of MM cell proliferation. Only the Target-1 dsRNA induced MM cell apoptosis. In contrast, the Target-2 dsRNA and the transfection reagent control vector did not induce cell apoptosis. We tested that whether silence Target-1 TRAF6 mRNA could inhibit NF-kB gene expression induced by IL-1. The 8226 MM cells were transduced of either 100nM TRAF6 or 100nM GAPDH dsRNA for 72 hours and then the cells were incubated with IL-1 for 0, 15, 30, and 60min. The cells were lysates and the total RNA or protein was detected by RT-PCR or western blot. The result showed that amount of NF-kB mRNA or activated NF-kB was significantly increased after 30 minute IL-1 stimulation while NF-kB dropped to normal level after 60 minutes. In contrast, in cells that received TRAF6 dsRNA, the amount of phosphor-NF-kB is no changed It has been clear that NF-kB specific response to TRAF6 knocked down by silence TRAF6 mRNA. We sought further to determine whether TRAF6 RNAi could inhibit NF-kB trigger function on luciferase activity. Using luciferase vector to monitor the activation of NF-kB signal transduction pathway. PNF-kB-Luc is designed to measure the binding of NF-kB to k enhancer, providing a direct measurement of activation this pathway. PTAL-Luc is ideal for use as a negative control vector. In view of the results showed that IL-1 stimulation of the double transfected cells at 30 minute result in a significant induction of luciferase by NF-kB releasing. Furthermore, this induction was abolished when TRAF6 mRNA was silenced by dsRNA. Multiple nuclear cells (pre-osteoclast) were decreased after silence TRAF6 when monocytes stimulated with RANKL and m-SCF. For future studies, we would like to use SCID-hu murine models of human myeloma to further develop this therapeutic strategy in relevant pre-clinical in vivo models. The in vitro studies outlined in this proposal will certainly significantly advance the understanding of this adapter protein in the pathogenesis and give us more impetus to target this protein for future therapeutic manipulation for patients with multiple myeloma. 12. Vaccination strategies in multiple myeloma 402 NY-ESO-1 AND MAGE-A3 ARE HIGHLY EXPRESSED IN MYELOMA PATIENTS WITH ABNORMAL CYTOGENETICS AND/OR RELAPSE Sushil K. Gupta, Fenghuang Zhan, Pei Lin, Jan V. Droogenbroeck*, Ramesh B. Batchu, Friedel Nollet*, Susann M Szmania, Amberly Moreno, Nancy Rosen, Guilio Spagnoli†,Bart Barlogie, Guido Tricot, John Shaughnessy and Frits van Rhee Myeloma Institute for Research and Therapy, University of Arkansas for Medical Sciences, Little Rock, AR U.S.A. *AZ Sint Jan, Department of Hematology, Brugge, Belgium. †Department of Surgery, University of Basel, Switzerland. Despite recent successes with chemotherapy and tandem autologous PBSCT, myeloma remains largely incurable. This highlights the need for novel, synergistic therapies, such as immunotherapy, which may reduce myeloma relapse. Using micro-array and immunohistochemical (IHC) staining, we have examined the expression of two potential targets for immunotherapy, NY-ESO-1 and MAGE-3. Purified myeloma cells were studied by micro-array (n=335), micro-array and IHC on corresponding biopsy (n=20), or IHC alone (n=19, 35 biopsies). Micro-array analysis of 335 patients revealed that expression of NY-ESO-1 and MAGE-A3 is related to the stage of myeloma. The frequency of expression of NY-ESO-1 and MAGE-A3 in MGUS, smoldering myeloma and newly diagnosed myeloma patients eligible for Total Therapy II (TT II) was 4.5%, 5.9% and 20.5% (NY-ESO-1) and 9.1%, 11.8% and 26.2% respectively (MAGE-A3). The presence of abnormal cytogenetics influenced the expression of both antigens. Newly diagnosed TT II trial patients with abnormal cytogenetics were more likely to express NY-ESO-1 and MAGE-A3 cRNA (NY-ESO-1 60% vs. 30.9%, p=0.004; MAGE-A3 65.8% vs. 27.5%, p=1.16x10-6). The percentage NY-ESO-1/MAGE-3 positive plasma cells at the protein level (IHC) was similarly correlated with abnormal cytogenetics. Both antigens (micro-array) were expressed in >50% of relapsed patients (NY-ESO-1 50%, p=8.8x10-9 and MAGE-A3 58.3%, p= 4.5x10-9). Strikingly, 100% patients with abnormal cytogenetics at relapse expressed NY-ESO-1 and MAGE-A3 (p=6.09x10-6 & 3.25x10-6). All these biopsies also stained positive by IHC for NY-ESO-1 and MAGE-A3. 13 patients were studied at diagnosis and at relapse. All biopsies positive at diagnosis by IHC for NY-ESO-1 or MAGE-A3 were positive for both antigens at relapse. The percentage NY-ESO-1 and MAGE-A3 positive myeloma cells in the biopsies was high (>50-90% positive plasma cells; 89% biopsies for NY-ESO-1 and 87% MAGE-A3). Double staining experiments are in progress to test whether the same myeloma cells are positive for both NY- ESO-1 and MAGE-A3. Expression of NY-ESO-1 and MAGE-A3 could be upregulated in myeloma cell-lines by incubating with the hypomethylating agent, decitabine. There was a significant increase in expression of NY-ESO-1 and MAGE-A3 after incubation with decitabine of the NY-ESO-1 and MAGE-A3 negative myeloma cell line U-937 by real-time PCR. In conclusion, NY-ESO-1 and MAGE-A3 are highly expressed in myeloma with abnormal cytogenetics and relapsed myeloma. These antigens can therefore be used as immunotherapy for myeloma with abnormal cytogenetics. Alternatively, NY-ESO- S267
Page 1 and 2:
Focussed Symposia Arsenic trioxide
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assess whether such a program will
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The overall response rate was noted
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Figure 5A Table 1: VEL + THAL for R
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naturally occurring OPG. Present tr
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0.505). Finally, the multiple event
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CLINICOPATHOLOGICAL DEFINITION OF W
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Plenary Sessions 1. Development of
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clonotypic IgH VDJ signature confir
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can be considered as two entities,
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immunofluorescence staining for DKK
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P2.3 DEVELOPMENT OF A MULTIPLE MYEL
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P2.5 MOLECULAR CYTOGENETICS OF MYEL
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clear that the biggest challenge fo
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esponse and have demonstrated that
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variable region of the idiotypic im
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4. From MGUS to symptomatic MM Fig.
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(MRI); some have claimed that level
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P4.5 CYTOKINES IN MGUS: THERAPEUTIC
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preventing phosphorylation of p70S6
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transducing component of the interl
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survive initial drug exposure and a
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quiescent counterpart, the human um
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transcriptional activity of NF-êB;
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manifestations and anomalous protei
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P7.4 ROLE OF SERUM FREE LIGHT CHAIN
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P7.6 IMMUNOPHENOTYPIC INVESTIGATION
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presumably through the circulation,
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9. Chemotherapy, maintenance treatm
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stratified according to their antim
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explore higher doses of zoledronic
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initial therapy. However, the role
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P10.2.2 SINGLE VERSUS TANDEM HIGH D
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With a median follow-up of 38 month
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cells could be harvested following
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11. What is the role of allogeneic
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found that 75% of patients who were
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patients with responsive disease 3
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9. Giralt S, Estey E, Albitar M, et
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Badros A, Barlogie B, Siegel E, et
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Figure 3b. Event-free Survival 4-Ye
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improve patient outcome in MM. Impo
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myeloma and in 40% of previously un
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degrade OPG in the same way as myel
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P12.2.5 MONOCLONAL ANTIBODY THERAPY
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myeloma. Blood 2001; 98:210-216. 6.
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MHC molecules, in effectively prese
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mice demonstrate that class II-spec
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detected in 293 and NIH3T3 cells. S
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hypothesis that (1) CCND1 and FGFR3
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patient samples. In addition, the p
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016 NEUTRAL ENDOPEPTIDASE (CD10) KN
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2. Genetic heterogeneity in MM: imp
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evidence from two t(11;14) cases wh
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immunoglobulin heavy chain (IgH) lo
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034 Instability of Pericentromeric
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clusters were found, the first was
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MGUS but most likely not crucial fo
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Objective: To compare the impact on
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4 patients had MMSET/IgH but did no
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and clonal PC from MGUS, MM and PCL
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059 VEGF receptor expresion in Mult
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two HLA-A2+ myeloma patients with C
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molecules expressed on the surface
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Recognition of these antigens appea
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Diagnosis requires a single area of
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081 Incidence of solid tumors in co
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Growth Factor (VEGF), Hepatocyte Gr
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PC-AI levels of MGUS and SMM patien
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093 The predominant pathway of tran
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was associated with I.V. line, whil
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103 Vascular amyloidosis induces se
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5. Signal transduction pathways and
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integrin in IGF-1-triggered MM cell
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118 IL-6- Induced Phosphorylation o
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123 THE IGF/IGF-1R SYSTEM IS A MAJO
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human myeloma cell line (HMCL) to a
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ligation or dexamethasone (Georgii-
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6. Role of microenvironment 6.1 Cel
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141 Human myeloma cells adhere to f
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145 STUDY OF BONE MARROW ANGIOGENES
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patients, the growth of primary mye
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tibia (con=49.1±0.7mg/cm2 vs 5T2=4
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157 The Nitrogen-Containing Bisphos
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7. New prognostic criteria for clas
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atio of >3. This system has subdivi
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Patient 1 (IgG/κ);IgG - 16.5 days,
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176 Pro-inflammatory and angiogenic
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180 Clinical study on the bone lesi
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7.2 Imaging studies 185 99mTc-MIBI
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189 Factors Predicting Occult Spina
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vivo detected resonances was invest
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Support Unit (CTSU) with flexibilit
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(β2m) & C reactive protein (CRP).
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plasmids carrying the clonotypic in
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newly diagnosed multiple myeloma as
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216 Transgenic expression of Myc an
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221 Prolonged survival in the 5T2MM
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9. Chemotherapy, maintenance, treat
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229 EFFECTIVENESS OF STANDARD CHEMO
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234 Melphalan and Dexamethasone- Is
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Methods. We investigated the VECD p
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9.2 Renal complications. 243 MERIT
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cost of SRE-related care was $10,24
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those with Hb >13 g/dL. Analysis of
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sustained response, lasting from 52
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proportion of bone abnormality. IgD
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disease. The lack of response to in
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yielding a median of 3x106/kg CD34
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patients(pts) aged ≥60 yrs. We co
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PBSC mobilizing regimen utilizing C
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their leukocytes and platelets. No
Page 225 and 226: 25 Gy to marrow. The tracer dose wa
Page 227 and 228: non-CR after the first transplant a
Page 229 and 230: 296 PERIPHERAL BLOOD STEM CELL TRAN
Page 231 and 232: References Effect of dose-intensive
Page 233 and 234: with cyclosporine A and methotrexat
Page 235 and 236: 11.Role of novel therapies targetin
Page 237 and 238: 312 Thalidomide as Rescue of Relaps
Page 239 and 240: patients, light chain in 1 patients
Page 241 and 242: platelets of 207 (76-402), B2M of 3
Page 243 and 244: 325 Low Dose Thalidomide plus Dexam
Page 245 and 246: in 5 pts (11%), M protein decreased
Page 247 and 248: time from diagnosis was 3.7 years a
Page 249 and 250: 339 Thalidomide, Clarithromycin and
Page 251 and 252: 344 COMBINATION OF THALIDOMIDE, DEX
Page 253 and 254: experienced early death during the
Page 255 and 256: untreated patients with high tumor
Page 257 and 258: 357 Thalidomide protects endothelia
Page 259 and 260: 362 EOSINOPHILIA IS A VERY COMMON F
Page 261 and 262: 11.5 CC 4047, PS 341 and arsenic tr
Page 263 and 264: without chromosome 13. Mean IC50 fo
Page 265 and 266: myeloma patients. Phase I data indi
Page 267 and 268: 11.6 Other drugs 380 EFFECT OF STI5
Page 269 and 270: significant inhibition of cell prol
Page 271 and 272: which acts to prevent the synthesis
Page 273 and 274: of B and its metabolites, however,
Page 275: and 10 months after start of therap
Page 279 and 280: lymphocytes was tested by Ellispot.
Page 281 and 282: 411 Dendritic Cell-Based Idiotype V
Page 283 and 284: Author Index Abe M 74 160 Abelman W
Page 285 and 286: De La Serna J 291 De Laurenzi A P11
Page 287 and 288: Hull DR 338 Hullen C P10.2.1 Humes
Page 289 and 290: Morra E 249 280 359 Morris CM 226 M
Page 291 and 292: Siegel D 70 115 250 Sierra J 304 30
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