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采用异种肝细胞构建生物人工肝。

Development of a bioartificial liver employing xenogeneic hepatocytes.

机构信息

Departments of Chemical Engineering and Materials Science, University of Minnesota, Minneapolis, MN, 55455-0132.

出版信息

Cytotechnology. 1997 Jan;23(1-3):29-38. doi: 10.1023/A:1007906512616.

Abstract

Liver failure is a major cause of mortality. A bioartificial liver (BAL) employing isolated hepatocytes can potentially provide temporary support for liver failure patients. We have developed a bioartificial liver by entrapping hepatocytes in collagen loaded in the luminal side of a hollow fiber bioreactor. In the first phase of development, liver-specific metabolic activities of biosynthesis, biotransformation and conjugation were demonstrated. Subsequently anhepatic rabbits were used to show that rat hepatocytes continued to function after the BAL was linked to the test animal. For scale-up studies, a canine liver failure model was developed using D-galactosamine overdose. In order to secure a sufficient number of hepatocytes for large animal treatment, a collagenase perfusion protocol was established for harvesting porcine hepatocytes at high yield and viability. An instrumented bioreactor system, which included dissolved oxygen measurement, pH control, flow rate control, an oxygenator and two hollow fiber bioreactors in series, was used for these studies. An improved survival of dogs treated with the BAL was shown over the controls. In anticipated clinical applications, it is desirable to have the liver-specific activities in the BAL as high as possible. To that end, the possibility of employing hepatocyte spheroids was explored. These self-assembled spheroids formed from monolayer culture exhibited higher liver-specific functions and remained viable longer than hepatocytes in a monolayer. To ease the surface requirement for large-scale preparation of hepatocyte spheroids, we succeeded in inducing spheroid formation in stirred tank bioreactors for both rat and porcine hepatocytes. These spheroids formed in stirred tanks were shown to be morphologically and functionally indistinguishable from those formed from a monolayer. Collagen entrapment of these spheroids resulted in sustaining their liver-specific functions at higher levels even longer than those of spheroids maintained in suspension. For use in the BAL, a mixture of spheroids and dispersed hepatocytes was used to ensure a proper degree of collagen gel contraction. This mixture of spheroids and dispersed cells entrapped in the BAL was shown to sustain the high level of liver-specific functions. The possibility of employing such a BAL for improved clinical performance warrants further investigations.

摘要

肝衰竭是主要的死亡原因之一。采用分离的肝细胞的生物人工肝脏(BAL)可能为肝衰竭患者提供暂时的支持。我们已经开发了一种生物人工肝脏,方法是将肝细胞包埋在装载在中空纤维生物反应器内腔侧的胶原中。在开发的第一阶段,证明了生物合成、生物转化和结合的肝脏特异性代谢活性。随后,使用无肝兔表明,大鼠肝细胞在 BAL 与受试动物连接后继续发挥功能。为了进行放大研究,使用 D-半乳糖胺过量建立了犬肝衰竭模型。为了确保为大型动物治疗获得足够数量的肝细胞,建立了胶原酶灌注方案,以高产率和高活力收获猪肝细胞。使用仪器化生物反应器系统进行这些研究,该系统包括溶解氧测量、pH 控制、流速控制、氧合器和两个串联的中空纤维生物反应器。与对照组相比,用 BAL 治疗的狗的存活率得到了提高。在预期的临床应用中,希望 BAL 中的肝脏特异性活性尽可能高。为此,探索了使用肝细胞球体的可能性。这些自组装的球体由单层培养形成,表现出更高的肝脏特异性功能,并且比单层培养中的肝细胞更具活力。为了简化大规模制备肝细胞球体的表面要求,我们成功地在搅拌罐生物反应器中诱导了大鼠和猪肝细胞的球体形成。在搅拌罐中形成的这些球体在形态和功能上与从单层形成的球体没有区别。胶原包埋这些球体可使它们的肝脏特异性功能维持在更高水平,时间甚至比悬浮培养的球体更长。为了在 BAL 中使用,将球体和分散的肝细胞混合使用,以确保胶原凝胶收缩达到适当的程度。BAL 中包埋的这种球体和分散细胞的混合物被证明可以维持高水平的肝脏特异性功能。为了提高临床性能,使用这种 BAL 的可能性需要进一步研究。

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