Long-term bone marrow cultured stromal cells regulate myeloma tumour growth in vitro:: studies with primary tumour cells and LTBMC-dependent cell lines

被引：29

作者：

Bloem, AC

Lamme, T

de Smet, M

Kok, H

Vooijs, W

Wijdenes, J

Boom, SE

Lokhorst, HM

机构：

[1] Univ Utrecht Hosp, Dept Immunol, NL-3584 CX Utrecht, Netherlands

[2] Univ Utrecht Hosp, Dept Haematol, NL-3584 CX Utrecht, Netherlands

[3] Univ Utrecht Hosp, Dept Immunohaematol, NL-3584 CX Utrecht, Netherlands

[4] Diaclone, Besancon, France

来源：

BRITISH JOURNAL OF HAEMATOLOGY | 1998年 / 100卷 / 01期

关键词：

plasma cell; myeloma; growth; stromal cells; IL-6;

D O I：

10.1046/j.1365-2141.1998.00517.x

中图分类号：

R5 [内科学];

学科分类号：

1002 ; 100201 ;

摘要：

Long-term bone marrow cultured stromal cells (LTBMC) produce IL-6 after contact with tumour cells from multiple myeloma patients. We found that LTBMC could substitute for exogenous IL-6 in the stimulation of bone marrow plasma cells from myeloma patients with active disease in short-term cultures. In addition, tumour cells of some patients with inactive disease, which were unresponsive to exogenous IL-6, were induced to IL-6-dependent growth after LTBMC co-culture. To study the role of LTBMC in myeloma tumour growth in vitro, plasma cell lines UM-2 and UM-3 were selected. UM-2 and UM-3 grew in contact with LTBMC and proliferation was blocked by antibodies against IL-6, IL-6 receptor (IL-6R, gp80, CD126) or the common signal transducing unit, gp130 (CD130). Culture with IL-6 alone or combined with GM-CSF resulted in cell death via apoptosis. The combination of IL-6 with soluble gp80, however, maintained in vitro proliferation of UM-2 and UM-3 cells. These data imply that LTBMC regulate myeloma growth in vitro via production of IL-6, possibly via induction of a functional IL-6 receptor on the tumour cells.

引用

页码：166 / 175

页数：10

共 46 条

[1] AHSMANN EJM, 1992, BLOOD, V79, P2068
[2] ANDERSON KC, 1989, BLOOD, V73, P1915
[3] BARILLE S, 1995, BLOOD, V86, P3151
[4] SERUM LEVELS OF INTERLEUKIN-6, A POTENT MYELOMA CELL-GROWTH FACTOR, AS A REFLECT OF DISEASE SEVERITY IN PLASMA-CELL DYSCRASIAS
BATAILLE, R
JOURDAN, M
ZHANG, XG
KLEIN, B
[J]. JOURNAL OF CLINICAL INVESTIGATION, 1989, 84 (06) : 2008 - 2011
[5] PHENOTYPICAL AND FUNCTIONAL-CHARACTERIZATION OF THE IDIOTYPE-POSITIVE BLOOD B-CELLS IN MULTIPLE-MYELOMA
BLOEM, AC
CHAND, MA
VANCAMP, B
BAST, EJEG
BALLIEUX, RE
[J]. SCANDINAVIAN JOURNAL OF IMMUNOLOGY, 1988, 28 (06) : 791 - 799
[6] CONFORMATIONS OF IMMUNOGLOBULIN HYPERVARIABLE REGIONS
CHOTHIA, C
LESK, AM
TRAMONTANO, A
LEVITT, M
SMITHGILL, SJ
AIR, G
SHERIFF, S
PADLAN, EA
DAVIES, D
TULIP, WR
COLMAN, PM
SPINELLI, S
ALZARI, PM
POLJAK, RJ
[J]. NATURE, 1989, 342 (6252) : 877 - 883
[7] CLEMENT C, 1995, LEUCOCYTE TYPING 5, V1, P714
[8] INVITRO CULTURE OF PRIMARY PLASMACYTOMAS REQUIRES STROMAL CELL FEEDER LAYERS
DEGRASSI, A
HILBERT, DM
RUDIKOFF, S
ANDERSON, AO
POTTER, M
COON, HG
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1993, 90 (05) : 2060 - 2064
[9] CELLULAR AND MOLECULAR GENETIC FEATURES OF MYELOMA AND RELATED DISORDERS
DURIE, BGM
[J]. HEMATOLOGY-ONCOLOGY CLINICS OF NORTH AMERICA, 1992, 6 (02) : 463 - 477
[10] DURIE BGM, 1975, CANCER, V36, P842, DOI 10.1002/1097-0142(197509)36:3<842::AID-CNCR2820360303>3.0.CO

← 1 2 3 4 5 →