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巨噬细胞分泌分子对淋巴细胞功能的调节。I. 描述与部分生化分析。

The modulation of lymphocyte functions by molecules secreted by macrophages. I. Description and partial biochemical analysis.

作者信息

Calderon J, Kiely J M, Lefko J L, Unanue E R

出版信息

J Exp Med. 1975 Jul 1;142(1):151-64. doi: 10.1084/jem.142.1.151.

Abstract

Culture fluids of peritoneal exudate cells rich in macrophages stimulated DNA synthesis of thymocytes and, to lesser extent, of spleen cells. We also investigated the effects of culture fluids from macrophages on the in vitro response to a hapten-carrier protein (fluorescein-menocyanin) using spleen cells from immune mice. Macrophage culture fluids contained an activity that increased the plaque-forming cell response of both IgG and IgM class. This increase was observed in the absence of any added hapten protein to the culture. The helper function of T lymphocytes (as evidenced by challenging with the hapten on the homologous carrier) was also increased by the macrophage culture fluid. However, this enhancement was best observed in conditions of relatively low T-cell activity. Also, the macrophage fluid allowed spleen cells of nude athymic mice to make a plaque-forming cell response to sheep red blood cells of both the IgM and IgG class. The macrophage was the cell source of the stimulatory molecule since it was generated only in cultures of macrophages devoid of significant number of lymphocytes. Stimulatory activity was not found in cultures of lymphocytes, mouse embryo cells, or 3T3 cells. The thymocyte stimulatory molecule did not contain H-2 antigens, was resistant to diisopropylfluorophosphate treatment, eluted from Sephadex with a size ranging from 15,000 to 21,000 daltons, and was sensitive to chymotrypsin and pepsin.

摘要

富含巨噬细胞的腹腔渗出液细胞培养液可刺激胸腺细胞的DNA合成,对脾细胞的刺激作用较弱。我们还使用免疫小鼠的脾细胞,研究了巨噬细胞培养液对体外对半抗原-载体蛋白(荧光素-钥孔戚血蓝蛋白)反应的影响。巨噬细胞培养液含有一种活性物质,可增强IgG和IgM类的噬斑形成细胞反应。在培养液中未添加任何半抗原蛋白的情况下观察到了这种增强。巨噬细胞培养液还增强了T淋巴细胞的辅助功能(通过用同源载体上的半抗原进行激发来证明)。然而,在T细胞活性相对较低的条件下,这种增强作用最为明显。此外,巨噬细胞培养液使无胸腺裸鼠的脾细胞对绵羊红细胞产生IgM和IgG类的噬斑形成细胞反应。巨噬细胞是刺激分子的细胞来源,因为它仅在不含大量淋巴细胞的巨噬细胞培养物中产生。在淋巴细胞、小鼠胚胎细胞或3T3细胞的培养物中未发现刺激活性。胸腺细胞刺激分子不含H-2抗原,对二异丙基氟磷酸处理有抗性,从葡聚糖凝胶上洗脱时大小范围为15,000至21,000道尔顿,对胰凝乳蛋白酶和胃蛋白酶敏感。

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