鸡肝实质精细结构的实验研究,特别参考了窦外巨噬细胞和窦内血细胞。第1部分。正常和墨汁灌注肝脏中的窦细胞和巨噬细胞。

M Ohata, T Ito
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引用次数: 13

摘要

用电镜观察了正常情况下和静脉灌注墨汁后的鸡肝脏。Kupffer细胞和窦状内皮细胞在灌注后最早阶段(15min)开始内吞墨汁颗粒。颗粒与细胞表面的附着仅发生在Kupffer细胞中,Kupffer细胞主动地吸收了被包裹的小泡颗粒。在内皮细胞中,颗粒通过核周的胞饮作用被摄取并沉积在Wisse的大胞饮液泡中。在Kupffer细胞和内皮细胞中,颗粒分别在灌注后30分钟和4小时储存最多。48h时,含有颗粒的液泡数量和大小减少,Kupffer细胞中出现有丝分裂现象。Ito细胞在后期(4和48小时)偶尔摄入少量碳颗粒;它们没有发生有丝分裂。弥散于薄壁的窦外巨噬细胞和淋巴组织中的吞噬网状细胞(巨噬细胞)仅在晚期(1-4小时)才表现出吞噬活性。灌注后48小时,两个细胞开始在其液泡中储存大量颗粒。这种延迟的吞噬活性可能归因于内皮细胞与窦状动脉分离的位置。一些孤立的巨噬细胞向正弦波内投射一个长过程,在早期阶段吞噬颗粒。48小时时,淋巴组织吞噬网状细胞发生有丝分裂,而薄壁内的孤立巨噬细胞未见有丝分裂。墨水灌注后,孤立巨噬细胞向窦状窦的迁移加快,频繁检测到巨噬细胞向库普弗细胞转化的图像。由此可见,库普弗细胞维持其所需数量不仅依靠自身的增殖,而且还依赖于分散在肝实质的窦外孤立巨噬细胞的补充,而这些巨噬细胞又来自于具有有丝分裂增殖能力的淋巴组织中的吞噬网状细胞。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Experimental study on the fine structure of chicken liver parenchyme with special references to extrasinusoidal macrophages and sinusoidal blood cells. Part 1. Sinusoidal cells and macrophages in the normal and India ink-perfused livers.

The chicken livers were electron microscopically observed under a normal condition and after an intravenous India ink perfusion. Kupffer cells and sinusoidal endothelial cells commenced to endocytose India ink particles in the earliest stages (15 min) after perfusion. The attachment of the particles to the cell surface occurred only in the Kupffer cells, which actively took up the particles with coated caveolae. In the endothelial cells the particles were ingested by pinocytosis in the perikaryon and deposited in the macropinocytic vacuoles of Wisse. In Kupffer and endothelial cells, the particles were stored most abundantly at 30 min and 4 hr after perfusion, respectively. At 48 hr, the vacuoles containing the particles were decreased in number and size, while mitotic figures were revealed in the Kupffer cells. Ito cells occasionally ingested in later stages (4 and 48 hr) a few carbon particles; they underwent no mitotic division. Extrasinusoidal macrophages scattered in the parenchyme and phagocytic reticular cells (macrophages) in the lymphoid tissues exhibited phagocytic activity only in later stages (1-4 hr). In 48 hr after the perfusion both cells began to store amounts of the particles in their vacuoles. This delayed phagocytic activity may be ascribed to the location of the cells separated from the sinusoid by the endothelium. Some solitary macrophages projecting a long process into the sinusoid took up the particles at earlier stages. At 48 hr, several mitotic divisions took place in the phagocytic reticular cells of the lymphoid tissue, while no mitotic divisions were found in the solitary macrophages in the parenchyme. After the ink perfusion, migration of solitary macrophages into the sinusoid was accelerated and images indicating their transformation into Kupffer cells were frequently detected. It was concluded that the Kupffer cells maintain their necessary number not only by their self-proliferation but also by replenishment from the extrasinusoidal solitary macrophages scattered in the hepatic parenchyme, which in turn are replenished from the phagocytic reticular cells in the lymphoid tissue capable of mitotic proliferation.

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