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三维多孔藻酸盐支架内的肝细胞行为。

Hepatocyte behavior within three-dimensional porous alginate scaffolds.

作者信息

Glicklis R, Shapiro L, Agbaria R, Merchuk J C, Cohen S

机构信息

Unit Biotechnology, Faculty of Engineering Sciences, Beer-Sheva, Israel.

出版信息

Biotechnol Bioeng. 2000 Feb 5;67(3):344-53. doi: 10.1002/(sici)1097-0290(20000205)67:3<344::aid-bit11>3.0.co;2-2.

Abstract

A potential approach to facilitate the performance of implanted hepatocytes is to enable their aggregation and re-expression of their differentiated function prior to implantation. Here we examined the behavior of freshly isolated rat adult hepatocytes seeded within a novel three-dimensional (3-D) scaffold based on alginate. The attractive features of this scaffold include a highly porous structure (sponge-like) with interconnecting pores, and pore sizes with diameters of 100-150 microm. Due to their hydrophilic nature, seeding hepatocytes onto the alginate sponges was efficient. DNA measurements showed that the total cell number within the sponges did not change over 2 weeks, indicating that hepatocytes do not proliferate under these culture conditions. Nearly all seeded cells maintained viability, according to the MTT assay. Within 24 h post-seeding, small clusters of viable cells, were seen scattered within the sponge. More than 90% of the seeded cells participated in the aggregation; the high efficiency is attributed to the non-adherent nature of alginate. The spheroids had smooth boundaries and by day 4 in culture reached an average diameter of 100 microm, which is at the same magnitude of the sponge pore size. The cells appeared to synthesize fibronectin which was deposited on the spheroids. No laminin or collagen type IV were detected in the deposit. The 3-D arrangement of hepatocytes within the alginate sponges promoted their functional expression; within a week the cells secreted the maximal albumin secretion rate of 60 microg albumin/10(6) cells/day. Urea secretion rate did not depend on cell aggregation and was similar to that obtained when hepatocytes were cultured on collagen type I coated dishes (100 microg/10(6) cells/day). Our studies show that alginate sponges can provide a conducive environment to facilitate the performance of cultured hepatocytes by enhancing their aggregation.

摘要

促进植入肝细胞发挥功能的一种潜在方法是,在植入前使其聚集并重新表达分化功能。在此,我们研究了将新鲜分离的成年大鼠肝细胞接种到基于藻酸盐的新型三维(3-D)支架内后的行为。该支架的吸引人之处包括具有相互连通孔隙的高度多孔结构(海绵状),以及直径为100 - 150微米的孔径。由于其亲水性,将肝细胞接种到藻酸盐海绵上很高效。DNA测量显示,海绵内的细胞总数在2周内没有变化,这表明肝细胞在这些培养条件下不会增殖。根据MTT测定,几乎所有接种的细胞都保持了活力。接种后24小时内,可见小的活细胞簇散布在海绵内。超过90%的接种细胞参与了聚集;这种高效率归因于藻酸盐的非粘附性质。这些球体边界光滑,培养4天时平均直径达到100微米,与海绵孔径大小相同。细胞似乎合成了沉积在球体上的纤连蛋白。在沉积物中未检测到层粘连蛋白或IV型胶原。藻酸盐海绵内肝细胞的三维排列促进了它们的功能表达;一周内细胞分泌白蛋白的最大速率达到60微克白蛋白/10⁶细胞/天。尿素分泌速率不依赖于细胞聚集,并与肝细胞在I型胶原包被培养皿上培养时的分泌速率相似(100微克/10⁶细胞/天)。我们的研究表明,藻酸盐海绵可以提供一个有利的环境,通过增强肝细胞聚集来促进培养肝细胞发挥功能。

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