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采用一种新的高产洋地黄皂苷/胶原酶灌注技术分离大鼠肝脏门周和肝静脉周围肝细胞中的糖异生作用。

Gluconeogenesis in periportal and perivenous hepatocytes of rat liver, isolated by a new high-yield digitonin/collagenase perfusion technique.

作者信息

Quistorff B

出版信息

Biochem J. 1985 Jul 1;229(1):221-6. doi: 10.1042/bj2290221.

Abstract

A technique is described which allows preparations of hepatocytes, enriched in either periportal or perivenous hepatocytes ('PP-cells' and 'PV-cells' respectively), in a yield of about 30-50% compared with control cell preparations. The liver is first perfused for 40-60s with digitonin (4 mg/ml) to destroy selectively either the periportal or the perivenous part of the microcirculatory unit, and then the remaining hepatocytes are isolated by the ordinary collagenase perfusion technique. In periportal cells the activities of alanine aminotransferase and pyruvate kinase were 29.4 and 18.7 mumol/min per mg of DNA respectively. The rate of gluconeogenesis was 0.402 mumol/min per mg of DNA. In perivenous cells the corresponding values were 9.55, 22.1 and 0.244 mumol/min per mg of DNA respectively. These data support the concept of a zonation of glucose metabolism within the microcirculatory unit of the liver, with the afferent part (periportal zone) having a 2-fold, more active gluconeogenesis than the efferent part (perivenous zone).

摘要

本文描述了一种技术,该技术能够制备富含门周或中央静脉周围肝细胞(分别为“PP细胞”和“PV细胞”)的肝细胞悬液,与对照细胞悬液相比,产率约为30 - 50%。首先用洋地黄皂苷(4 mg/ml)对肝脏进行40 - 60秒的灌注,以选择性破坏微循环单位的门周或中央静脉周围部分,然后通过常规胶原酶灌注技术分离剩余的肝细胞。在门周细胞中,丙氨酸转氨酶和丙酮酸激酶的活性分别为每毫克DNA 29.4和18.7 μmol/分钟。糖异生速率为每毫克DNA 0.402 μmol/分钟。在中央静脉周围细胞中,相应的值分别为每毫克DNA 9.55、22.1和0.244 μmol/分钟。这些数据支持肝脏微循环单位内葡萄糖代谢呈区域化的概念,即传入部分(门周区)的糖异生活性比传出部分(中央静脉周围区)高2倍,更具活性。

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