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巨噬细胞失活因子的纯化

Purification of macrophage deactivating factor.

作者信息

Srimal S, Nathan C

机构信息

Beatrice and Samuel A. Seaver Laboratory, Department of Medicine, Cornell University Medical College, New York, New York 10021.

出版信息

J Exp Med. 1990 Apr 1;171(4):1347-61. doi: 10.1084/jem.171.4.1347.

Abstract

Macrophage deactivation factor (MDF) in P815 tumor cell-conditioned medium was assayed by its suppression of the ability of activated mouse peritoneal macrophages to release hydrogen peroxide. MDF displayed properties of a soluble protein(s) associated with both low (8-25,000) and high (greater than 450,000) Mr fractions. MDF was purified 6,140-fold by a seven-step procedure: extraction with acid-ethanol; precipitation with ether; and fractionation on gel filtration, anion-exchange, diphenyl reversed-phase and C4 reversed-phase HPLC columns, the last column twice. The final preparation contained two species: (a) a approximately 13,000 Mr band on reducing or nonreducing SDS-PAGE and on autoradiograms after radioiodination with chloramine T, and (b) a 66,000 Mr species ranging from approximately 5% to approximately 50% of the protein detectable by silver strain. The 66,000 Mr species was identified as albumin from its NH2-terminal amino acid sequence. However, no amino acid sequence could be obtained for the approximately 13,000 Mr species, either in fluid phase or after electroelution of the corresponding SDS-PAGE band. Thus, approximately 13,000 Mr MDF associates tightly with albumin through a variety of separation techniques, and may have a blocked NH2 terminus. Purified MDF afforded 50% inhibition of activated macrophage H2O2 releasing capacity at a concentration of 1-10 nM. Separation of MDF from most higher Mr moieties was associated with disproportionately small increases in specific activity, suggesting MDF might be partially inactivated by purification. As purified, MDF was approximately 1,000-fold less potent at deactivating macrophages than TGF-beta. Antibodies that neutralized the macrophage-deactivating effect of TGF-beta did not inhibit deactivation by MDF.

摘要

通过检测P815肿瘤细胞条件培养基中的巨噬细胞失活因子(MDF)对活化的小鼠腹腔巨噬细胞释放过氧化氢能力的抑制作用来进行分析。MDF表现出与低分子量(8 - 25,000)和高分子量(大于450,000)组分相关的可溶性蛋白质的特性。通过七步程序将MDF纯化了6,140倍:用酸乙醇提取;用乙醚沉淀;并在凝胶过滤、阴离子交换、二苯基反相和C4反相HPLC柱上进行分级分离,最后一个柱进行两次分离。最终制剂包含两种成分:(a)在还原或非还原SDS - PAGE上以及用氯胺T进行放射性碘化后的放射自显影片上呈现约13,000分子量条带,以及(b)一种66,000分子量的成分,其在银染可检测到的蛋白质中占约5%至约50%。根据其氨基末端氨基酸序列,将66,000分子量的成分鉴定为白蛋白。然而,无论是在液相中还是在相应SDS - PAGE条带电洗脱后,都无法获得约13,000分子量成分的氨基酸序列。因此,约13,000分子量的MDF通过多种分离技术与白蛋白紧密结合,并且可能具有封闭的氨基末端。纯化的MDF在浓度为1 - 10 nM时对活化巨噬细胞的H2O2释放能力有50%的抑制作用。将MDF与大多数较高分子量部分分离时,其比活性的增加不成比例地小,这表明MDF可能在纯化过程中部分失活。纯化后的MDF在使巨噬细胞失活方面的效力比TGF - β低约1,000倍。中和TGF - β巨噬细胞失活作用的抗体不抑制MDF的失活作用。

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