Role of macrophage inflammatory protein-2 in aspiration-induced lung injury

Objective: To determine the role of the chemokine, macrophage inflammatory protein (MIP)-2, in the pathogenesis of aspiration-induced lung injury in the rat. Design: Prospective, randomized, controlled animal study, Setting: University research laboratories, Subjects: Adult, male Long-Evans rats. Interventions: Anesthetized rats underwent induction of lung injury by well-described models of aspiration triggered by intratracheal delivery of acid alone, gastric particles alone, or the combination. After injury, induction of MIP-2 messenger RNA in whole lungs and immunoreactive MIP-2 in bronchoalveolar lavage (BAL) fluids was determined, The contribution of MIP-2 to BAL fluid chemotactic activity was defined by using an in vitro chemotaxis assay, The in vivo effect of blocking MIP-2 on pulmonary vascular leak, BAL fluid neutrophils, Pao(2)/F10(2), ratio, and alveolar-arterial oxygen tension gradient in acid-induced lung injury was determined. Measurements and Main Results: Induction of MIP-2 messenger RNA and protein over time was observed in response to all three stimuli. A significant portion (25% to 41%) of the chemotactic activity in BAL fluids from injured rats was inhibited by anti-MIP-2 antibody, After acid injury, blocking of MIP-2 was associated with a 53% decrease in BAL fluid neutrophils and a 33% decrease in pulmonary vascular leak. Although acid injury both impaired oxygenation and increased venous admixture, in ville blocking of MIP-5 was associated with improved oxygenation as well as decreased venous admixture, Conclusions: MIP-2 was up-regulated during the development of aspiration-induced lung injury in rats. MIP-2 contributed to lung accumulation of neutrophils via a chemotactic mechanism. Although oxygenation and venous admixture are worsened by acid-induced lung injury in vivo, blocking of MIP-2 at the onset of injury improved these physiologic alterations. Because the aspiration event often is witnessed, chemokines may be valid therapeutic targets for inhibiting the subsequent inflammatory response.