Mechanisms of serum potentiation of GM-CSF production by human airway smooth muscle cells

doi:10.1152/ajplung.00126.2004

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Am J Physiol Lung Cell Mol Physiol 287: L1007-L1016, 2004; doi:10.1152/ajplung.00126.2004
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Mechanisms of serum potentiation of GM-CSF production by human airway smooth muscle cells

D. J. Lalor ,¹^,* B. Truong,¹^,* S. Henness,¹ A. E. Blake,¹ Q. Ge,² A. J. Ammit,¹ C. L. Armour,¹ and J. M. Hughes¹

¹Respiratory Research Group, Faculty of Pharmacy and ²Department of Pharmacology, University of Sydney, New South Wales 2006, Australia

Submitted 5 April 2004 ; accepted in final form 25 June 2004

Inflammation and vascular leakage are prevalent in asthma. Thisstudy aimed to elucidate the mechanisms involved in serum potentiationof cytokine-induced granulocyte macrophage colony stimulatingfactor (GM-CSF) production by human airway smooth muscle cellsand to identify possible factors responsible. Serum-deprivedcells at low density were stimulated with TNF- ${alpha}$ and IL-1 ${beta}$ for24 h. Human AB serum (10%), inhibitors of RNA and protein synthesisor specific signaling molecules, or known smooth muscle mitogenswere then added for 24 h. Culture supernatants were analyzedfor GM-CSF levels, and cells were harvested to assess viability,cell cycle progression, GM-CSF-specific mRNA content, and p38phosphorylation. Serum potentiated GM-CSF release when addedbefore, together with (maximal), or after the cytokines. Thepotentiation involved both new GM-CSF-specific mRNA productionand protein synthesis. The mitogens IGF, PDGF, and thrombinall potentiated GM-CSF release, and neutralizing antibodiesfor EGF, IGF, and PDGF reduced the serum potentiation. Inhibitorstudies ruled as unlikely the involvement of p70^S6kinase andthe MAPK p42/p44, two signaling pathways implicated in proliferation,and the involvement of the MAPK JNK, while establishing rolesfor p38 MAPK and NF- ${kappa}$ B in the potentiation of GM-CSF release.Detection of significant p38 phosphorylation in response toserum stimulation, through Western blotting, further demonstratedthe involvement of p38. These studies have provided evidenceto support p38 being targeted to interrupt the cycle of inflammation,vascular leakage and cytokine production in asthma.

granulocyte macrophage colony stimulating factor; serum; p38 mitogen-activated protein kinase; NF- ${kappa}$ B

Address for reprint requests and other correspondence: J. M. Hughes, Faculty of Pharmacy A15, Univ. of Sydney, NSW 2006 Australia (E-mail: margh{at}pharm.usyd.edu.au)