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正常肝脏和受损肝脏的库普弗细胞分泌产物可刺激储脂细胞的增殖。

Proliferation of fat-storing cells is stimulated by secretions of Kupffer cells from normal and injured liver.

作者信息

Zerbe O, Gressner A M

机构信息

Department of Clinical Chemistry, Philipps University, Marburg, Federal Republic of Germany.

出版信息

Exp Mol Pathol. 1988 Aug;49(1):87-101. doi: 10.1016/0014-4800(88)90023-8.

Abstract

The influence of Kupffer cells (KC) from normal, D-galactosamine- and thioacetamide-injured liver on the growth of rat liver fat-storing cells (FSC) in culture was studied. The supplementation of FSC incubation medium with normal and galactosamine-KC-conditioned media for 4 days caused 1.5- and 1.9-fold increase (P less than 0.005), respectively, in the DNA contents of FSC on the fifth day of culture. The stimulant effect reached a maximum at a 1:2 dilution of the conditioned medium with FSC incubation medium. The population doubling time of FSC grown in the absence of conditioned medium was calculated to be 41.5 +/- 3 hr; it was greatly shortened by KC-conditioned medium from galactosamine-treated rats (24 +/- 2 hr), by normal KC-conditioned medium (28 +/- 4 hr), and by KC medium from thioacetamide-injured rats (33 +/- 5 hr). Similarly KC-conditioned media of either source stimulated significantly the rate of [3H]thymidine incorporation into DNA of FSC even during short-term exposures of FSC with KC medium. The growth-promoting effect of normal KC-conditioned medium could be enhanced if the Kupffer cells were challenged with zymosan and phorbol esters, respectively, but not with lipopolysaccharide. The light microscopic appearance of FSC grown in the presence of KC-conditioned media was greatly changed: the cultures became more dense; the cells spread and developed long extensions. The size and number of lipid droplets decreased more rapidly than in control cultures maintained without addition of KC-conditioned media. The protein DNA ratio of FSC exposed with KC-conditioned media was reduced due to a strong increase in DNA, which is not followed by a similar increase in cellular protein. If referred to the DNA content of the culture, the incorporation of [3H]valine into the protein of the medium was not changed, that into cellular protein was strongly reduced under the influence of normal KC-conditioned medium. Secretions of Kupffer cells obviously stimulate significantly the proliferation of FSC in culture.

摘要

研究了来自正常肝脏、经D-半乳糖胺和硫代乙酰胺损伤的肝脏的库普弗细胞(KC)对培养的大鼠肝脏贮脂细胞(FSC)生长的影响。用正常和半乳糖胺-KC条件培养基补充FSC培养液4天,分别使培养第5天FSC的DNA含量增加了1.5倍和1.9倍(P<0.005)。条件培养基与FSC培养液按1:2稀释时,刺激作用达到最大。未添加条件培养基时FSC的群体倍增时间计算为41.5±3小时;经半乳糖胺处理大鼠的KC条件培养基(24±2小时)、正常KC条件培养基(28±4小时)和硫代乙酰胺损伤大鼠的KC培养基(33±5小时)可使其大大缩短。同样,任何一种来源的KC条件培养基即使在FSC与KC培养基短期接触期间,也能显著刺激[3H]胸腺嘧啶核苷掺入FSC的DNA速率。如果分别用酵母聚糖和佛波酯刺激库普弗细胞,而不用脂多糖刺激,则正常KC条件培养基的促生长作用会增强。在KC条件培养基存在下生长的FSC的光学显微镜外观发生了很大变化:培养物变得更密集;细胞铺展并长出长的突起。脂质小滴的大小和数量比未添加KC条件培养基的对照培养物下降得更快。由于DNA强烈增加,而细胞蛋白质没有类似增加,暴露于KC条件培养基的FSC的蛋白质/DNA比值降低。如果参照培养物的DNA含量,[3H]缬氨酸掺入培养基蛋白质的量没有变化,在正常KC条件培养基的影响下,掺入细胞蛋白质的量则大大减少。库普弗细胞的分泌物明显显著刺激培养中的FSC增殖。

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