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短小棒状杆菌在腹膜巨噬细胞激活中的作用。II. 巨噬细胞亚群对不同抗肿瘤活性的识别

Role of Corynebacterium parvum in the activation of peritoneal macrophages. II. Identification of distinguishable anti-tumor activities by macrophage subpopulations.

作者信息

Chapes S K, Haskill S

出版信息

Cell Immunol. 1983 Feb 15;76(1):49-57. doi: 10.1016/0008-8749(83)90347-7.

Abstract

Two different mechanisms of murine macrophage (MP) antitumor activity are described in this report. C. parvum-activated peritoneal MPs were tested for cytotoxic and cytostatic activity 4 days after ip immunization. Cytotoxic activity could be distinguished from cytostatic activity using two different assay protocols. When MPs were separated by 1g velocity sedimentation, cytotoxic MPs were confined to high velocity fractions. In contrast, cytostatic MPs were found in cell fractions with velocities as low as 5.2 mm/hr. These two MP activities were also distinguishable by culturing at 37 degrees C for 24 hr. Cytotoxicity was abrogated when MPs were incubated in MEM, or MEM supplemented with lymphokine (LK) or indomethacin. In contrast, cytostasis remained at high levels when the cells were incubated with LK or indomethacin. Cytotoxicity was not retained after overnight culture even if LPS was present, or if various spleen or non-adherent peritoneal exudate cells were cocultured with the cytotoxic effector cells. Assays done to determine the presence of suppressor cells failed to find any inhibitory cell type. The phagocytic index, acid phosphatase activity, and H2O2 secretion were also measured before and after overnight culture. Acid phosphatase and phagocytic activities did not decline whereas H2O2 secretion declined significantly. These data indicate that in response to C. parvum, at least two different effector cell types with distinct antitumor activities are generated. Cytotoxicity, like the ability of cells to secrete H2O2, is found to be a short-lived function of CP stimulated MPs. In contrast, cytostasis is a function retained longer by MPs in culture.

摘要

本报告描述了小鼠巨噬细胞(MP)抗肿瘤活性的两种不同机制。腹腔注射免疫4天后,检测微小隐孢子虫激活的腹腔MP的细胞毒性和细胞生长抑制活性。使用两种不同的检测方案可区分细胞毒性活性和细胞生长抑制活性。当通过1g速度沉降分离MP时,细胞毒性MP局限于高速部分。相比之下,在速度低至5.2毫米/小时的细胞部分中发现了细胞生长抑制MP。通过在37℃培养24小时,这两种MP活性也可区分。当MP在MEM或补充有淋巴因子(LK)或消炎痛的MEM中孵育时,细胞毒性被消除。相比之下,当细胞与LK或消炎痛孵育时,细胞生长抑制仍保持在高水平。即使存在LPS,或者将各种脾脏或非贴壁腹腔渗出细胞与细胞毒性效应细胞共培养,过夜培养后细胞毒性也不会保留。为确定抑制细胞的存在而进行的检测未能发现任何抑制细胞类型。还在过夜培养前后测量了吞噬指数、酸性磷酸酶活性和H2O2分泌。酸性磷酸酶和吞噬活性没有下降,而H2O2分泌显著下降。这些数据表明,对微小隐孢子虫的反应会产生至少两种具有不同抗肿瘤活性的效应细胞类型。细胞毒性,如细胞分泌H2O2的能力,被发现是CP刺激的MP的一种短暂功能。相比之下,细胞生长抑制是MP在培养中保留时间更长的一种功能。

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