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大鼠血小板相关物质对成年大鼠肝细胞原代培养物中DNA合成的刺激作用。

Stimulation of DNA synthesis in primary cultures of adult rat hepatocytes by rat platelet-associated substance(s).

作者信息

Strain A J, McGowan J A, Bucher N L

出版信息

In Vitro. 1982 Feb;18(2):108-16. doi: 10.1007/BF02796402.

DOI:10.1007/BF02796402
PMID:7044955
Abstract

Experiments in whole animals have shown that normally quiescent adult rat hepatocytes are induced to proliferate by blood borne substances, which we are now probing in primary monolayer cultures. Under our conditions, freshly isolated adult hepatocytes do not proliferate actively in a defined medium, but are stimulated to synthesize DNA--an essential first step--by either serum or an EGF-hormone combination. Stimulation of [3H]thymidine incorporation into hepatocyte DNA by addition of dialyzed mouse, human, horse, or bovine (fetal, newborn, or calf) serum, whose activities are all similar, is regularly surpassed by an EGF-insulin mixture without serum. This, in turn, is exceeded by dialyzed normal rat serum, which is several times more potent than the other sera tested. Removal of blood platelets reduces the activity of normal rat serum by over 50%. Heat inactivation (56 degrees C) causes a similar loss, but heat treatment of platelet-poor serum fails to cause further reduction. The activity of mouse and human serum is not reduced by platelet removal. Serum from partially hepatectomized rats is not significantly more stimulatory than normal rat serum, and its activity is depressed in the same way by platelet deprivation and heat inactivation. Lack of enhancement by partial hepatectomy is not consonant with whole animal studies and requires further investigation. The heat-labile portion of the DNA synthesis-stimulating activity of rat serum appears to derive from platelets. This activity differs from the well-characterized heat-stable human PDGF. Its relation to other reported platelet-associated growth factors is still undetermined.

摘要

对整体动物进行的实验表明,正常情况下处于静止状态的成年大鼠肝细胞会被血液中的物质诱导增殖,我们目前正在原代单层培养物中对此进行探究。在我们的实验条件下,新鲜分离的成年肝细胞在特定培养基中不会积极增殖,但会被血清或表皮生长因子(EGF)与胰岛素的组合刺激而合成DNA,这是必不可少的第一步。添加经透析的小鼠、人、马或牛(胎儿、新生或小牛)血清(其活性均相似)可刺激[3H]胸腺嘧啶核苷掺入肝细胞DNA,但无血清的EGF-胰岛素混合物的刺激作用通常超过血清。反过来,经透析的正常大鼠血清的刺激作用又超过了EGF-胰岛素混合物,其效力比其他测试血清高几倍。去除血小板会使正常大鼠血清的活性降低超过50%。热灭活(56℃)会导致类似程度的活性丧失,但对贫血小板血清进行热处理不会导致进一步降低。去除血小板不会降低小鼠和人血清的活性。部分肝切除大鼠的血清刺激作用并不比正常大鼠血清显著增强,并且其活性也会因血小板缺乏和热灭活而以相同方式降低。部分肝切除未能增强血清刺激作用这一现象与整体动物研究结果不一致,需要进一步研究。大鼠血清中刺激DNA合成的活性的热不稳定部分似乎来自血小板。这种活性不同于已被充分表征的热稳定的人血小板衍生生长因子(PDGF)。它与其他报道的血小板相关生长因子的关系仍未确定。

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