Interactions of dimethyl sulfoxide and granulocyte‐macrophage colony‐stimulating factors on the growth and maturation of HL‐60 cells

Brennan, James K.; Lee, K S; Abboud, Camille N.; Erickson‐Miller, Connie L.; Keng, Peter C.

doi:10.1002/jcp.1041320208

Cited by 11 publications

(7 citation statements)

References 38 publications

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“…The ter stationary phase (Sollner-Webb and Tower, 1986; cellular changes that eventually lead to growth arrest Grummt et al, 1977;Grummt et al, 1976; Cavanaugh begin early in the differentiation program (Fibach et al, et al, 1984). Changes in rRNA transcription appear to 1982; von Melchner and Hoffken, 1985) and are partially be more closely related to the cell growth cycle than to reversible by the growth factor GM-CSF (Schwartz and the synthesis of DNA or the immediate entry of cells Maher, 1988;Brennan et al, 1987). into S phase (Sollner-Webb and Tower, 1986).…”

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Multiple mechanisms for the inhibition of rRNA synthesis during HL‐60 leukemia cell differentiation

Schwartz

Nilson

1988

Journal Cellular Physiology

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Treatment of HL-60 human promyelocytic leukemia cells with inducers of granulocytic differentiation produces a depletion of cellular rRNA, with the anthracycline antibiotics aclacinomycin A (ACM) and marcellomycin (MCM) causing a more rapid loss than dimethylsulfoxide (DMSO). This action is associated with a large reduction in RNA synthesis, which precedes any decreases in protein or DNA synthesis, and is specific for rRNA relative to total polyadenylated RNA synthesis. A 70% reduction in rRNA synthesis occurs within 20 minutes of ACM treatment and by 30 hours of DMSO exposure. Relative to the amount of 28S and 18S rRNA in the cells, there is a nearly complete depletion of the amount of 45S rRNA and other large rRNA precursors in cells treated with ACM, MCM, and the intercalating agent actinomycin D. In contrast, DMSO treatment produces a more coordinated decrease in 18S and 28S rRNA and rRNA precursors. The anthracycline antibiotics inhibited the synthesis of 5' proximal and 3' distal regions of the pre-rRNA transcript, while actinomycin D had a relatively sparing effect on the transcription of the 5' external transcribed spacer region of the gene relative to depletion of 3' transcripts. These studies demonstrate that different inducers of HL-60 differentiation have varying sites of action on rRNA synthesis and/or processing, with depletion of cellular rRNA as a common consequence.

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confidence: 99%

Multiple mechanisms for the inhibition of rRNA synthesis during HL‐60 leukemia cell differentiation

Schwartz

Nilson

1988

Journal Cellular Physiology

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“…Two HL-60 populations were used in these studies: the highly passaged line, HL-60 UR, has been in continuous culture in this laboratory for 10 years, whereas HL-60 passage 76 cells were thawed from frozen stocks and used from passages 76-100. Both were maintained in McCoy's 5A Medium (GIBCO) with 10% fetal bovine serum (Hyclone) ("standard medium") and passaged twice weekly as previously described (Brennan et al, 1987). Cells from the late exponentialearly plateau phase of growth (-1 x lo6 cells/ml for passage 76 and -2 x 106 cells/ml for UR) were washed in buffer and resuspended in standard medium (growth studies), 3% serum-medium (elutriation), or phosphatefree, serum-free medium ([32Pl-orthophosphate labeling).…”

Section: Materials and Methods Hl-60 Cells And Their Maintenancementioning

confidence: 99%

“…HL-60 cell proliferation and maturation 1 X lo5 cells/ml were cultured at 37°C in 25 cm2 tissue culture flasks containing standard medium, 0-100 uiml recombinant human GM-CSF (RH-CSF, Genzyme, specific activity 5 x lo7 CFU-GM/mg protein), and 0-1.5% DMSO (Fisher Scientific) for 7 days. Cell viability was assessed by trypan blue exclusion; cell concentrations and volume distributions were quantified with an electronic particle counter-sizer (Coulter), and maturation was assessed by nitroblue tetrazolium (NBT) reduction, as previously described (Brennan et al, 1987).…”

Section: Materials and Methods Hl-60 Cells And Their Maintenancementioning

confidence: 99%

“…We have previouslv reported that DMSO inhibits the autonomous growth" of -unsynchronized, highly passaged HL-60 myeloid leukemia cells and that this growth inhibition is reversed by addition of recombi-nant human GM-CSF to cultures (Brennan et al, 1987). Since DMSO-induced granulocytic differentiation (NBT reduction) is not antagonized by GM-CSF, their conjoint presence in cultures produces a facsimile of normal development where renewal and differentiation are balanced.…”

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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

Brennan

Lee

Frazel

et al. 1991

Journal Cellular Physiology

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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 u/ml recombinant human GM-CSF and/or 0-1.25% DMSO, and phosphoprotein changes quantified on autoradiograms of [32P]-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) [32P]-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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“…HL-60 cells are cytokine-dependent myelomonocytic precursor cells [31,32] that retain their bipotent ability to differentiate along either the myeloid or the monocytic lineages when treated with all-trans retinoic acid (atRA) or 1,25-dihydroxyvitamin D3(VD3), respectively [33][34][35]. They express an ensemble of atRA-or VD3-induced or regulated cell surface receptors such as the insulin receptor [36,37] and c-FMS receptor tyrosine kinases [38,39], FcgRIIA [40], BLR1 [41], and CD38 [42,43].…”

Section: Introductionmentioning

confidence: 99%

All-trans retinoic acid induces p62DOK1 and p56DOK2 expression which enhances induced differentiation and G0 arrest of HL-60 leukemia cells

2006

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p62 DOK1 (DOK1) and p56 DOK2 (DOK2) are sequence homologs that act as docking proteins downstream of receptor or nonreceptor tyrosine kinases. Originally identified in chronic myelogenous leukemia cells as a highly phosphorylated substrate for the chimeric p210 bcr-abl protein, DOK1 was suspected to play a role in leukemogenesis. However, p62 DOK1À/À fibroblast knockout cells were found to have enhanced MAPK signaling and proliferation due to growth factors, suggesting negative regulatory capabilities for DOK1. The role of DOK1 and DOK2 in leukemogeneis thus is enigmatic. The data in this report show that both the DOK1 and the DOK2 adaptor proteins are constitutively expressed in the myelomonoblastic leukemia cell line, HL-60, and that expression of both proteins is induced by the chemotherapeutic differentiation causing agents, all-trans retinoic acid (atRA) and 1,25-dihydroxyvitamin D3 (VD3). Ectopic expression of either protein enhances atRA-or VD3-induced growth arrest, differentiation, and G 0 /G 1 cell cycle arrest and results in increased ERK1/2 phosphorylation. DOK1 and DOK2 are similarly effective in these capabilities. The data provide evidence that DOK1 and DOK2 proteins have a similar role in regulating cell proliferation and differentiation and are positive regulators of the MAPK signaling pathway in this context. Am. J. Hematol. 81:603-615, 2006. V V C

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Interactions of dimethyl sulfoxide and granulocyte‐macrophage colony‐stimulating factors on the growth and maturation of HL‐60 cells

Cited by 11 publications

References 38 publications

Multiple mechanisms for the inhibition of rRNA synthesis during HL‐60 leukemia cell differentiation

Multiple mechanisms for the inhibition of rRNA synthesis during HL‐60 leukemia cell differentiation

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

All-trans retinoic acid induces p62DOK1 and p56DOK2 expression which enhances induced differentiation and G0 arrest of HL-60 leukemia cells

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Interactions of dimethyl sulfoxide and granulocyte‐macrophage colony‐stimulating factors on the growth and maturation of HL‐60 cells

Cited by 11 publications

References 38 publications

Multiple mechanisms for the inhibition of rRNA synthesis during HL‐60 leukemia cell differentiation

Multiple mechanisms for the inhibition of rRNA synthesis during HL‐60 leukemia cell differentiation

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

All-trans retinoic acid induces p62DOK1 and p56DOK2 expression which enhances induced differentiation and G0 arrest of HL-60 leukemia cells

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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