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肝细胞的低温保存。II. 钙离子和氨基酸的重要性。

Hypothermic preservation of hepatocytes. II. Importance of Ca2 and amino acids.

作者信息

Marsh D C, Belzer F O, Southard J H

机构信息

Department of Surgery, University of Wisconsin Hospital, Madison 53792.

出版信息

Cryobiology. 1990 Feb;27(1):1-8. doi: 10.1016/0011-2240(90)90047-8.

Abstract

The importance of the components of a tissue culture media, Leibovitz-15 (L-15), for maintaining viability of hypothermically preserved hepatocytes was analyzed. Hepatocytes isolated from rat livers were incubated at 5 degrees C in an oxygenated environment with continuous shaking (to simulate organ perfusion preservation). L-15 + 5 g% polyethylene glycol (PEG) or variants of this solution were used as the preservation media. After 48 hr of storage, hepatocyte viability was assessed by measuring the release of LDH into the incubation medium and cell volumes were determined. Following 90 min of normothermic incubation (to simulate organ reperfusion), mitochondrial function was measured. Hepatocytes stored in the complete L-15 solution were about 90% viable at the end of 48 hr of storage, while cells stored in a solution containing only the principle electrolytes (PE) lost viability (70% viable). Only the addition of a combination of divalent cations (Ca/Mg) and amino acids was sufficient to maintain viability equivalent to that obtained in the complete L-15 mixture. Hepatocytes suspended in L-15 maintained normal cell volumes (3.85 microliters/mg protein), while cells in the PE solution were swollen with cell volumes of 4.66 microliters/mg protein. Only the addition of Ca/Mg to the PE solution was effective at suppressing cell swelling similar to the complete L-15 media. Both basal and uncoupler-stimulated respiration were depressed in cells stored in the PE solution (15 and 28 nmol O2/min/mg protein) as compared to cells in L-15 (21 and 41 nmol O2/min/mg protein).(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

分析了组织培养基Leibovitz-15(L-15)的成分对低温保存肝细胞活力维持的重要性。从大鼠肝脏分离的肝细胞在5摄氏度的充氧环境中持续振荡孵育(以模拟器官灌注保存)。L-15 + 5 g%聚乙二醇(PEG)或该溶液的变体用作保存培养基。储存48小时后,通过测量乳酸脱氢酶(LDH)释放到孵育培养基中的量来评估肝细胞活力,并测定细胞体积。在常温孵育90分钟(以模拟器官再灌注)后,测量线粒体功能。储存在完整L-15溶液中的肝细胞在储存48小时结束时约90%存活,而储存在仅含主要电解质(PE)溶液中的细胞失去活力(70%存活)。仅添加二价阳离子(钙/镁)和氨基酸的组合足以维持与完整L-15混合物相当的活力。悬浮在L-15中的肝细胞保持正常细胞体积(3.85微升/毫克蛋白),而PE溶液中的细胞肿胀,细胞体积为4.66微升/毫克蛋白。仅向PE溶液中添加钙/镁可有效抑制细胞肿胀,类似于完整的L-15培养基。与L-15中的细胞(21和41纳摩尔氧气/分钟/毫克蛋白)相比,储存在PE溶液中的细胞的基础呼吸和解偶联剂刺激的呼吸均受到抑制(15和28纳摩尔氧气/分钟/毫克蛋白)。(摘要截断于250字)

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