Differential Tumor Necrosis Factor Alpha Expression and Release from Peritoneal Mouse Macrophages In Vitro in Response to Proliferating Gram-Positive versus Gram-Negative Bacteria

doi:10.1128/IAI.68.8.4422-4429.2000

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Infection and Immunity, August 2000, p. 4422-4429, Vol. 68, No. 8
0019-9567/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Differential Tumor Necrosis Factor Alpha Expression and Release from Peritoneal Mouse Macrophages In Vitro in Response to Proliferating Gram-Positive versus Gram-Negative Bacteria

Wei Cui,¹ David C. Morrison,¹^,²^,³ and Richard Silverstein⁴^,^*

Departments of Basic Medical Science¹ and Anesthesiology,² School of Medicine, University of Missouri at Kansas City, Kansas City, Missouri 64108; Office of Research Administration, Saint Luke's Hospital, Kansas City, Missouri 64111³; and Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, Kansas 66160⁴

Received 9 February 2000/Returned for modification 22 March 2000/Accepted 3 May 2000

Viable Escherichia coli and Staphylococcus aureus bacteria elicited markedly different in vitro tumor necrosis factor alpha(TNF- $alpha$ ) responses when placed in coculture with peritoneal murinemacrophages. These include quantitative differences in TNF- $alpha$ mRNAexpression and corresponding protein product secretion as wellas kinetic differences in the profiles of the TNF- $alpha$ responses.Further, lipopolysaccharide (from E. coli) is a major contributingfactor to these differences, as revealed by comparative experimentswith endotoxin-responsive (C3Heb/FeJ) and endotoxin-hyporesponsive(C3H/HeJ) macrophages. Nevertheless, the eventual overall magnitudeof the TNF- $alpha$ secretion of macrophages in response to S. aureuswas at least equivalent to that observed with E. coli, while appearingat time periods hours later than the E. coli-elicited TNF- $alpha$ response.Both the magnitude and kinetic profile of the TNF- $alpha$ responseswere found to be relatively independent of the rate of bacterialproliferation, at least to the extent that similar results wereobserved with both viable and paraformaldehyde-killed microbes.Nevertheless, S. aureus treated in culture with the carbapenemantibiotic imipenem manifests markedly altered profiles of TNF- $alpha$ response, with the appearance of an early TNF- $alpha$ peak not seenwith viable organisms, a finding strikingly similar to that recentlyreported by our laboratory from in vivo studies (R. Silverstein,J. G. Wood, Q. Xue, M. Norimatsu, D. L. Horn, and D. C. Morrison,Infect. Immun. 68:2301-2308, 2000). In contrast, imipenem treatmentof E. coli-cocultured macrophages does not significantly alterthe observed TNF- $alpha$ response either in vitro or in vivo. In conclusion,our data support the concept that the host inflammatory responseof cultured mouse macrophages in response to viable gram-positiveversus gram-negative microbes exhibits distinctive characteristicsand that these distinctions are, under some conditions, alteredon subsequent bacterial killing, depending on the mode of killing.Of potential importance, these distinctive in vitro TNF- $alpha$ profilesfaithfully reflect circulating levels of TNF- $alpha$ in infected mice.These results suggest that coculture of peritoneal macrophageswith viable versus antibiotic-killed bacteria and subsequent assessmentof cytokine response (TNF- $alpha$ ) may be of value in clarifying, andultimately controlling, related host inflammatory responses insepticpatients.

^* Corresponding author. Mailing address: Department of Biochemistry and Molecular Biology, University of Kansas Medical Center,Kansas City, KS 66160. Phone: (913) 588-6954. Fax: (913) 588-7440.E-mail: rsilvers{at}kumc.edu.

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