Steinbeck M J, Khan A U, Karnovsky M J
Department of Pathology, Harvard Medical School, Boston, Massachusetts 02115.
J Biol Chem. 1993 Jul 25;268(21):15649-54.
The extracellular production of singlet oxygen (O2(1 delta g)) by stimulated macrophages was measured using a modification of our quantitative method initially developed to measure the intracellular production of O2(1 delta g) by neutrophils (Steinbeck, M. J., Khan, A. U., and Karnovsky, M. J. (1992) J. Biol. Chem. 267, 13425-13433). Glass coverslips were coated with the specific chemical trap for O2(1 delta g), 9,10-diphenylanthracene (DPA) and perylene, which is an internal standard, in a methylene chloride solution containing 0.3 mg/ml polystyrene. On evaporation, the polystyrene formed an even coating of DPA and perylene over the surface of a glass coverslip (PDP film). Unstimulated macrophages or macrophages stimulated with 4 beta-phorbol 12-myristate 13-acetate (PMA) or formyl-methionyl-leucyl-phenylalanine (fMLP) were then added to the PDP film in a darkened room and incubated at 37 degrees C for 30 min in a humidified 5% CO2 atmosphere. Both unstimulated and stimulated cells adhered to the PDP film in approximately equivalent numbers. Only stimulated cells produced measurable amounts of O2(1 delta g) in a dose-dependent response to either PMA or fMLP. The production of O2(1 delta g) by macrophages stimulated with PMA was maximal in response to 25 ng, 17.8 +/- 1.3 nmol of O2(1 delta g)/approximately 1.00 x 10(6) cells. The maximal response for fMLP was at a concentration of 1 microM, 18.4 +/- 1.0 nmol of O2(1 delta g)/approximately 1.00 x 10(6) cells. The specific detection of O2(1 delta g) by this method was confirmed by thermally releasing O2(1 delta g) from the DPA-O2(1 delta g) reaction product, DPA-endoperoxide, regenerating the original DPA compound. Production of O2(1 delta g) by the stimulated cells was inhibited 80-89% by the addition of 60-120 micrograms of superoxide dismutase, an enzyme that converts superoxide to hydrogen peroxide and ground state molecular oxygen or 79-84% with the addition of 2 mM histidine, an avid quencher of O2(1 delta g). Neither of these additions interfered with adhesion of the cells to the PDP film. The ability of superoxide dismutase to inhibit the production of O2(1 delta g) suggested that O2(1 delta g) was produced via a superoxide-dependent route. The ability of an oxidase to produce O2(1 delta g) secondary to superoxide production was substantiated further using a xanthine oxidase-acetaldehyde system. Purified xanthine oxidase produced both superoxide and O2(1 delta g), and their production was inhibited by the addition of superoxide dismutase.(ABSTRACT TRUNCATED AT 400 WORDS)
采用一种改良的定量方法,测定了受刺激巨噬细胞胞外单线态氧(O₂(¹Δg))的生成情况。该方法最初是为测量中性粒细胞胞内O₂(¹Δg)的生成而开发的(斯坦贝克,M. J.,汗,A. U.,和卡诺夫斯基,M. J.(1992年)《生物化学杂志》267卷,第13425 - 13433页)。用9,10 - 二苯基蒽(DPA)和作为内标的苝,在含有0.3 mg/ml聚苯乙烯的二氯甲烷溶液中,对玻璃盖玻片进行O₂(¹Δg)的特异性化学捕获物包被。蒸发后,聚苯乙烯在玻璃盖玻片表面形成DPA和苝的均匀涂层(PDP膜)。然后在暗室中将未受刺激的巨噬细胞或用4β - 佛波醇12 - 肉豆蔻酸酯13 - 乙酸酯(PMA)或甲酰 - 甲硫氨酰 - 亮氨酰 - 苯丙氨酸(fMLP)刺激的巨噬细胞添加到PDP膜上,并在37℃、5%二氧化碳饱和湿度的环境中孵育30分钟。未受刺激和受刺激的细胞以大致相等的数量附着在PDP膜上。只有受刺激的细胞对PMA或fMLP产生剂量依赖性的可测量量的O₂(¹Δg)。用PMA刺激的巨噬细胞产生O₂(¹Δg)的最大值出现在25 ng时,为17.8±1.3 nmol O₂(¹Δg)/约1.00×10⁶个细胞。fMLP的最大反应浓度为1 μM,为18.4±1.0 nmol O₂(¹Δg)/约1.00×10⁶个细胞。通过从DPA - O₂(¹Δg)反应产物DPA - 内过氧化物热释放O₂(¹Δg),使原始DPA化合物再生,证实了该方法对O₂(¹Δg)的特异性检测。添加60 - 120微克超氧化物歧化酶(一种将超氧化物转化为过氧化氢和基态分子氧的酶)或添加2 mM组氨酸(一种O₂(¹Δg)的强力猝灭剂)后,受刺激细胞产生O₂(¹Δg)的量被抑制80 - 89%或79 - 84%。这两种添加物均不影响细胞与PDP膜的附着。超氧化物歧化酶抑制O₂(¹Δg)生成的能力表明O₂(¹Δg)是通过超氧化物依赖性途径产生的。使用黄嘌呤氧化酶 - 乙醛系统进一步证实了氧化酶在产生超氧化物后产生O₂(¹Δg)的能力。纯化的黄嘌呤氧化酶同时产生超氧化物和O₂(¹Δg),添加超氧化物歧化酶可抑制它们的产生。(摘要截短至400字)
