Elucidation of signaling molecules involved in macrophage activation by bacterial lipopolysaccharide

2002 Fiscal Year Final Research Report Summary

• Project/Area Number: 13670281
• Research Category: Grant-in-Aid for Scientific Research (C)
• Allocation Type: Single-year Grants
• Section: 一般
• Research Field: Bacteriology (including Mycology)
• Research Institution: Jichi Medical School
• Principal Investigator: SAITO Shinji Jichi Medical School, School of Medicine, Research Associate, 医学部, 助手 (50195989)
• Project Period (FY): 2001 – 2002
• Keywords: macrophage / lipopolysaccharide / IL-12 / MAPK / ERK

Research Abstract

In response to IPS, murine peritoneal macrophages produced IL-12 (heterodimer of p35 and p40 subunits) but marine macrophage line cells of RAW264.7 did not RAW264.7 produced no IL-12p35 and a small amount of IL-12p40 upon LPS stimulation. Subcloning of RAW264.7 was carried out and isolated high producer clones of IL-12p40 (clone Hi). To understand the underlying mechanisms of LPS-induced IL-12 production, clone Hi was investigated its LPS responsive features in comparison to those of its parent RAW264.7, low producer clone (clone Lw), and another IL-12p40 high producer cell line, J774.1. In LPS-induced productions of TNF, IL-1, IL-6, and NO, or in expressions of their mRNA, no significant differences between the two clones were found mRNA expression of IL-12p40 was detected in clone Lw and the parent RAW264.7 by stimulation with BCG but not with LPS. These results indicated that low production of IL-12p40 by LPS stimulated RAW264.7 and clone Lw was not due to the defect or mutation on IL-12p40 gene. Presence of some specific signaling processes for LPS-induced IL-12p40 production was suggested. There was no significant difference between clone Hi and Lw in LPS-induced phosphorylations of MAP kinases, ERK1/2, p38MAPK, and SAPK/JNK. However, ERK1/2 phosphorylation in J774.1 in response to LPS was remarkably lower than that in RAW264.7 and its subclones. Strong mRNA expression of IL-12p40 in response to LPS was defected in RAW264.7 and clone Lw pretreated with an inhibitor of MEK1/2. These results suggest that over activation of ERK1/2 induce some suppressive signals on IL-12p40 expression. In clone Hi, expression of IL-12p40 mRNA in response to LPS was detected without the MEK1/2 inhibitor pretreatment, although weaker than that of J774.1. Pretreatment of cycloheximide suppressed all of LPS-induced mRNA expressions tested except for TNF. These results suggest that these gene expressions require de novo protein synthesis.

Research Products

• [Publications] Shimomura, H.: "Lipopolysaccharide of Burkholderia cepacia and its unique character to stimulate murine macrophages with relative lack of interleukin-1β-inclucing ability"Infection and Immunity. 69・6. 3663-3669 (2001)
  • Description: 「研究成果報告書概要(和文)」より
• [Publications] Shimomura,H.: "Lipopolysaccharide of Burkholderia cepacia and its unique character to stimulate murine macrophages with relative lack of interleukin-1β-inducing ability"Infection and Immunity. 69(6). 3663-3669 (2001)
  • Description: 「研究成果報告書概要(欧文)」より