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巨噬细胞上清液对系膜细胞增殖具有刺激和抑制双重作用。

Macrophage supernatants have both stimulatory and suppressive effects on mesangial cell proliferation.

作者信息

Mattana J, Singhal P C

机构信息

Department of Medicine, Long Island Jewish Medical Center, New Hyde Park, NY 11042.

出版信息

J Cell Physiol. 1993 Feb;154(2):289-93. doi: 10.1002/jcp.1041540211.

Abstract

Macrophages may modulate mesangial expansion following renal injury via secretory products. We undertook the present study to determine the effects of macrophage supernatants on mesangial cell proliferation. Macrophage supernatants collected in serum-free media after 24 hours caused significantly enhanced mesangial cell proliferation in long-term culture at concentrations up to 50% but caused suppression at higher concentrations (control, 122,000 +/- 14,000 cells/well; 50% supernatant, 188,000 +/- 15,100 cells/well, P < 0.02 compared to control, n = 4; 80% supernatant, 52,000 +/- 3,500 cells/well, P < 0.01 compared to control, n = 4). In short-term culture [3H]thymidine incorporation, a measure of DNA synthesis, was significantly enhanced compared to control at supernatant concentrations up to 30% (30% supernatant, 4,120 +/- 310 cpm/well; control, 3,210 +/- 97 cpm/well, P < 0.5, n = 4), but uptake was reduced at high concentration (80% supernatant, 2,900 +/- 74 cpm/well; control, 3,210 +/- 97 cpm/well, P < 0.05, n = 4). When macrophage supernatants were collected after 48 hours incubation and incubated with mesangial cells, mesangial cell thymidine uptake was significantly suppressed compared to control (48-hour supernatant, 4,060 +/- 260 cpm/well; control, 5,890 +/- 270 cpm/well, P < 0.01, n = 4) and compared to 24-hour supernatants, which enhanced uptake (24-hour supernatant, 8,080 +/- 340 cpm/well; control, 5,890 +/- 270 cpm/well, P < 0.01, n = 4). Our results suggest that macrophage supernatants can directly enhance mesangial cell proliferation in vitro in both short-term and long-term culture, though this effect is lost at high concentrations of supernatant. These data lend support to the potential role of the macrophage in mediating mesangial expansion following renal injury.

摘要

巨噬细胞可能通过分泌产物调节肾损伤后的系膜扩张。我们进行本研究以确定巨噬细胞上清液对系膜细胞增殖的影响。在无血清培养基中培养24小时后收集的巨噬细胞上清液,在浓度高达50%时可显著增强长期培养中的系膜细胞增殖,但在更高浓度时则导致抑制(对照组,122,000±14,000个细胞/孔;50%上清液组,188,000±15,100个细胞/孔,与对照组相比P<0.02,n = 4;80%上清液组,52,000±3,500个细胞/孔,与对照组相比P<0.01,n = 4)。在短期培养中,作为DNA合成指标的[3H]胸腺嘧啶核苷掺入量,在高达30%的上清液浓度下与对照组相比显著增强(30%上清液组,4,120±310 cpm/孔;对照组,3,210±97 cpm/孔,P<0.5,n = 4),但在高浓度时摄取减少(80%上清液组,2,900±74 cpm/孔;对照组,3,210±97 cpm/孔,P<0.05,n = 4)。当在孵育48小时后收集巨噬细胞上清液并与系膜细胞一起孵育时,与对照组相比,系膜细胞胸腺嘧啶核苷摄取显著受到抑制(48小时上清液组,4,060±260 cpm/孔;对照组,5,890±270 cpm/孔,P<0.01,n = 4),并且与增强摄取的24小时上清液相比也受到抑制(24小时上清液组,8,080±340 cpm/孔;对照组,5,890±270 cpm/孔,P<0.01,n = 4)。我们的结果表明,巨噬细胞上清液在短期和长期培养中均可在体外直接增强系膜细胞增殖,尽管在高浓度上清液时这种作用会丧失。这些数据支持了巨噬细胞在介导肾损伤后系膜扩张中的潜在作用。

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