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The Caco-2 Cell Monolayers as an Intestinal Metabolism Model: Metabolism of Dipeptide Phe-Pro

 

作者: HuM.,   ChenJ.,   TranD.,   ZhuY.,   LeonardoG.,  

 

期刊: Journal of Drug Targeting  (Taylor Available online 1994)
卷期: Volume 2, issue 1  

页码: 79-89

 

ISSN:1061-186X

 

年代: 1994

 

DOI:10.3109/10611869409015895

 

出版商: Taylor&Francis

 

关键词: Peptide;Intracellular Metabolism;Caco-2;Transcellular Transport;Intestinal Epithelium

 

数据来源: Taylor

 

摘要:

AbstractThe metabolism of Phe-Pro was investigated in Caco-2 cell monolayers, a model of small intestinal epithelium. The results indicate that the majority of Phe-Pro was hydrolyzed during passage from the apical (AP) to basolateral (BL) side. The enzyme responsible for the hydrolysis is prolidase, a cytosolic enzyme. Through kinetic studies of a supernatant enzyme preparation, a Kmof 30.4μM and Vmaxof 38.9 nmol/min per mg of protein were obtained. The enzyme catalyzed hydrolysis was inhibited by proline (66%), Zn++(86%), Cu++(100%), Fe+++(100%), PCMB (89%), and captopril (66%), but not by leucine. We also studied the transcellular transport of Phe-Pro by measuring the amount of Phe in the receiver media. In the presence of a proton gradient (AP pH6, BL pH7.4), the appearance rate of Phe in the BL media after Phe-Pro was loaded apically was at least 100 times faster than that in the AP media after Phe-Pro was loaded basolaterally. The former is also higher than the appearance rate of Phe without a transepithelial proton gradient (pH 6–pH 6) or against a proton gradient (pH7.4–pH6). The rate of appearance of Phe in the BL media (pH7.4) after Phe-Pro was loaded on the AP side (pH 6) was decreased by the presence in the AP media of proline (42%), leucine (40%), and captopril (17%), but not by Zn++. In conclusion, the transmembrane uptake of Phe-Pro is dependent on a proton gradient, and the intracellular metabolism of Phe-Pro is complete via hydrolysis by prolidase.

 

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