SEPARATION OF RAT PANCREATIC SECRETORY PROTEINS BY CATION-EXCHANGE FAST PROTEIN LIQUID-CHROMATOGRAPHY

被引：5

作者：

FUCHS, MJ ^{[1
]}

KEIM, V ^{[1
]}

机构：

[1] UNIV HEIDELBERG,KLINIKUM MANNHEIM,MED KLIN,THEODOR KUTZER UFER,W-6800 MANNHEIM,GERMANY

来源：

JOURNAL OF CHROMATOGRAPHY-BIOMEDICAL APPLICATIONS | 1992年 / 576卷 / 02期

关键词：

D O I：

10.1016/0378-4347(92)80202-2

中图分类号：

O65 [分析化学];

学科分类号：

070302 ; 081704 ;

摘要：

Rat pancreatic secretory proteins were separated by an automated liquid chromatography system utilizing a Mono S cation-exchange column. Optimal resolution was obtained with a multistep salt and pH gradient (0.01-2 M LiCl, pH 5.3-63.). A total of fourteen well-separated peaks, as well as several minor peaks, were detected by UV absorption. The main pancreatic enzymes were resolved (two amylases, two chymotrypsinogens, two trypsinogens, proelastase, lipase, prophospholipase A2, procarboxypeptidase A, procarboxy-peptidase B, and ribonuclease). In addition, proteins without enzymic activity, such as lithostathine and pancreatitis-associated protein, were identified. Activation of proenzymes did not occur during the separation. At a flow-rate of 0.5 ml/min, ca. 250-mu-g to 5 mg of protein could be applied with equal resolution. The reproducibility of retention volumes and peak areas was high (less than 1% or 5% variation, respectively). When radiolabeled proteins were separated, a comparable pattern of peaks was obtained. The technique described is, therefore, not only useful for analytical and preparative separation of pancreatic proteins but can additionally serve for quantitative determination of the pancreatic isoenzyme pattern.

引用

页码：287 / 295

页数：9

共 22 条

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