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人外周血单核细胞衍生的巨噬细胞在体外产生具有溶血活性的C3。

Human peripheral blood monocyte-derived macrophages produce haemolytically active C3 in vitro.

作者信息

Strunk R C, Kunke K S, Giclas P C

出版信息

Immunology. 1983 May;49(1):169-74.

Abstract

The third component of complement (C3) synthesized by human monocyte-derived macrophages has been shown to have the same size and sub-unit structure as serum C3, but haemolytic activity has not been demonstrated. Human monocyte-derived macrophages were cultured from days 4 to 7 in medium without serum, and the conditioned medium was dialysed to remove inhibitors of the C3 assay and concentrated to enhance detection of low amounts of C3. Using these techniques C3 activity was detected routinely. The amount of C3 was 3.4 x 10(7) effective C3 molecules/ml of concentrated tissue culture medium (range 1.0-7.5 x 10(7)), and the number of C3 molecules synthesized by each cell was 4.4 x 10(5), assuming that each cell synthesized C3. The specific activity of the C3 synthesized by the monocytes was the same as the specific activity of C3 that had been purified from serum and then incubated with the cells and processed in the same manner as the monocyte media. Synthesis as the basis for the presence of the C3 activity in the medium was indicated by an inhibition of production of the C3 activity of 66 +/- 16% by cycloheximide, 2 micrograms/ml. Thus, human blood monocytes that migrate into areas of inflammation can mature into cells capable of producing C3 which can participate in the complement sequence and thus potentiate inflammation.

摘要

人单核细胞衍生的巨噬细胞合成的补体第三成分(C3),其大小和亚基结构已被证明与血清C3相同,但尚未证实其溶血活性。人单核细胞衍生的巨噬细胞在无血清培养基中培养4至7天,将条件培养基透析以去除C3检测的抑制剂,并进行浓缩以增强对少量C3的检测。使用这些技术可常规检测到C3活性。C3的量为3.4×10⁷个有效C3分子/毫升浓缩组织培养基(范围为1.0 - 7.5×10⁷),假设每个细胞都合成C3,则每个细胞合成的C3分子数为4.4×10⁵。单核细胞合成的C3的比活性与从血清中纯化后与细胞一起孵育并以与单核细胞培养基相同方式处理的C3的比活性相同。2微克/毫升放线菌酮对C3活性产生的抑制作用为66±16%,这表明合成是培养基中C3活性存在的基础。因此,迁移到炎症区域的人血单核细胞可以成熟为能够产生C3的细胞,C3可参与补体序列,从而增强炎症反应。

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本文引用的文献

7
Biosynthesis of complement by human monocytes.人单核细胞补体的生物合成。
Clin Immunol Immunopathol. 1981 Mar;18(3):334-43. doi: 10.1016/0090-1229(81)90126-4.

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