4.6 Article

Changes in circulating lymphocyte subpopulations and mitogen-stimulated response in a rat infusion model of intra-abdominal infection

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CRITICAL CARE MEDICINE
卷 28, 期 7, 页码 2515-2521

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LIPPINCOTT WILLIAMS & WILKINS
DOI: 10.1097/00003246-200007000-00054

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sepsis; animal model; bacterial infection; interleukin-2; immunosuppression; flow cytometry; Escherichia coli

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Objective: To describe the alterations in circulating concentrations of immune cells as well as in in vitro mitogen-stimulated response In a recently developed rat model of intra-abdominal infection. Design: Randomized, controlled study. Setting: Government research facility. Subjects: Male Sprague-Dawley rats. Interventions: Infected animals received an intraperitoneal infusion of 6.0 x 10(8) colony forming units of Escherichia coli during 12 hrs, whereas control rats received a sterile inoculum, All experimental animals underwent laparotomy and peritoneal lavage at the end of the infusion period. Blood samples were obtained 12 hrs, 36 hrs, or 7 days after the onset of infusion. Splenocytes were concomitantly harvested and assayed for response to the mitogens phytohemagglutinin (PHA), concanavalin A (Con A), and lipopolysaccharides, as well as for production of interleukin (IL)-2. Measurements and Main Results: Infected rats showed a marked leukopenia (-82% for 36 hrs), with leukocyte counts returning to normal at 7 days. They also developed a marked lymphocytopenia throughout the study; this was achieved through comparable reductions in circulating T and B cells. Con A responses in both groups were similar for 7 days. In contrast, splenocytes from infected animals showed reduced responses to lipopolysaccharides (-64%) and PHA (-30%) for 36 hrs compared with control splenocytes. IL-2 production from mitogen-stimulated splenocytes was suppressed in infected rats to 66% of that of control rats for 7 days. Suppressed PHA responses were not restored to control values in the presence of IL-2. For all of the parameters assessed, control animals showed either no significant changes or relatively fewer changes than infected rats. Conclusions: This model of intra-abdominal infection is associated with changes in circulating concentrations of immune cells as well as with temporary functional defects in B acid T cells, consistent with those often observed in patients with peritonitis. However, the role of IL-2 in limiting the adverse effects of infection in this experimental model seems to be limited. This model may be a useful tool in furthering our understanding of the pathophysiology of intra-abdominal infections and in assessing the efficacy of new therapeutic modalities.

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