RABBIT MACROPHAGE INTERFERONS: I. CONDITIONS FOR BIOSYNTHESIS BY VIRUS-INFECTED AND UNINFECTED CELLS

doi:10.1084/jem.125.4.559

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ARTICLE

RABBIT MACROPHAGE INTERFERONS : I. CONDITIONS FOR BIOSYNTHESIS BY VIRUS-INFECTED AND UNINFECTED CELLS

Thomas J. Smith M.D.¹ and Robert R. Wagner M.D.¹

¹ From the Department of Microbiology, The Johns Hopkins University School of Medicine, Baltimore, Maryland

Interferon is produced in cultures of rabbit leukocytes inresponse to infection with Newcastle disease virus or in theabsence of known viral infection. The macrophage appears tobe the responsible producing cell. Cultures prepared from sterileperitoneal exudates, which contained about 90% macrophages,are at least as efficient as cultures of rabbit kidney (RK)cells in their capacity to synthesize NDV-induced interferon.Interferon can be detected in the medium by 2 hr after viralinfection and the titers usually reach a peak of 10,000 PDD₅₀/mlby 4–6 hr. Exposure to actinomycin prior to or shortlyafter viral induction effectively blocks interferon synthesisby cells of both types. However, macrophages become refractoryto actinomycin by 30–60 min compared with 607–120min for RK cells, a finding which suggests earlier and morerapid transcription of interferon-specific messenger RNA inmacrophages. Macrophages harvested from the peritioneal cavityof rabbits injected intravenously with NDV 48 hr previouslyalso exhibit slightly reduced capacity to synthesize interferon,but this tolerant state is less marked than is tolerance toproduction of circulating interferon in intact rabbits.

Interferonis also synthesized by rabbit macrophages not infected withvirus but simply incubated at 37°C in medium with or withoutadded bacterial endotoxin. Uninfected polymorphonuclear leukocytes,rabbit kidney and spleen cells produced no detectable interferonunder similar conditions of cultivation. No interferon was releasedby intact macrophages incubated at 4°C or by ultrasonicallydisrupted macrophages incubated at 37°C. Although interferontiters were found to be higher when uninfected cultures wereexposed to 10–100 µg/ml of E. coli lipopolysaccharide,unavailability of suitable pyrogen-free maintenance media precludedanswering the question whether macrophages can continually synthesizeand release interferon spontaneously. Interferon yields fromuninfected macrophages were only 1% or less of the yields fromNDV-infected macrophages, but the rates of synthesis were similarunder both conditions. Studies with actinomycin and puromycinrevealed that sequential transcriptive and translational eventsare required for de novo interferon synthesis by uninfectedcells in a manner similar to virus-induced interferon synthesis.

Thephysical properties and molecular weights of these rabbit interferonsare discussed in the following report (12).

Submitted on October 28, 1966

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