INTERACTIONS OF DIMETHYL-SULFOXIDE AND GRANULOCYTE-MACROPHAGE COLONY-STIMULATING FACTOR ON THE CELL-CYCLE KINETICS AND PHOSPHOPROTEINS OF G1-ENRICHED HL-60 CELLS - EVIDENCE OF EARLY EFFECTS ON LAMIN-B PHOSPHORYLATION

被引:15
作者
BRENNAN, JK [1 ]
LEE, KS [1 ]
FRAZEL, MA [1 ]
KENG, PC [1 ]
YOUNG, DA [1 ]
机构
[1] UNIV ROCHESTER,SCH MED & DENT,DEPT RADIAT ONCOL,ROCHESTER,NY 14642
关键词
D O I
10.1002/jcp.1041460313
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
We have found that GM-CSF and DMSO have antagonistic effects on the proliferation but not maturation of asynchronously growing HL-60 cells such that growth in the presence of both more closely resembles normal hematopoiesis (Brennan et al., J. Cell Physiol. 132:246, 1987). Studies were undertaken to determine whether or not the agents affected the same mitogenic pathway and locus in the cell cycle. HL-60 populations containing at least 90% G1 cells were obtained by centrifugal elutriation, exposed to 100-mu/ml recombinant human GM-CSF and/or 0-1.25% DMSO, and phosphoprotein changes quantified on autoradiograms of [P-32]-orthophosphate-labeled cell proteins separated by giant 2-D gel electrophoresis. Results were correlated with 1) intracellular pH, determined by measurement of BCECF fluorescence; 2) [P-32]-orthophosphate uptake; 3) cell cycle progression, determined by flow quantitation of DNA content in mithramycin or propidium iodide-stained cells; and 4) growth, determined by cell volume and concentration. GM-CSF stimulated and DMSO inhibited the GM-CSF-stimulated phosphorylation of 1 protein (approximately 65 kDa, p.i. 5.6) within 2 min of exposure. These effects were sustained through G1, not associated with changes in intracellular pH, and preceded similar antagonistic effects on phosphate uptake (15-30 minutes), cell volume change (16-24 hr), and cell concentration increase (28-32 hr). GM-CSF accelerated and DMSO inhibited G1 to S transit with the most marked antagonism observed in the second cycle following synchronization (28 to 40 hrs). Cell maturation (morphology, NBT reduction) was dominated by DMSO and not antagonized by GM-CSF. We have identified p65 as the nuclear intermediate filament protein, lamin B, on the basis of its locus on gels and its binding of a monoclonal antibody to intermediate filaments and antiserum to human lamin B on immunoblots. These studies suggest that at least part of the GM-CSF-DMSO antagonism is exerted through the same mitogenic pathway, that a major locus of cytokinetic effect is on G1 to S transit, and that nuclear envelope protein phosphorylation is an important early event.
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页码:425 / 434
页数:10
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