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人小肠麦芽糖酶、异麦芽糖酶和蔗糖酶活性的柱色谱分析

Column chromatography of human small-intestinal maltase, isomaltase and invertase activities.

作者信息

Dahlqvist A, Telenius U

出版信息

Biochem J. 1969 Jan;111(2):139-46. doi: 10.1042/bj1110139.

Abstract
  1. The maltase, isomaltase and invertase (sucrase) activities of solubilized mucosal preparations from human jejunum and ileum were studied with column chromatography on anion-exchange (diethylaminoethyl- and triethylaminoethyl-)cellulose and Sephadex G-200 gel. 2. On ion-exchange cellulose columns both kinds of enzyme preparations yielded two major disaccharidase peaks. The first peak contained maltase Ia (=isomaltase) and maltase Ib (=invertase). The second peak contained maltase II and maltase III. 3. On Sephadex G-200 gel columns jejunal preparations yielded the corresponding peaks as on ion-exchange columns, but the peaks appeared in the reverse order in the effluent. The ileal preparation studied yielded a single peak on gel columns, containing all the activities studied and eluted with the ;void volume'. 4. Precipitation with ethanol did not affect the behaviour of the enzymes during ion-exchange chromatography. When gel filtration was performed after ethanol precipitation of the enzymes, however, two peaks were obtained also with the ileal preparation, and subfractionation of the invertase was obtained with both kinds of preparations. 5. The second peak from ion-exchange chromatograms, containing maltase II and maltase III, on concentration was found to have very weak isomaltase activity, probably exerted by these enzymes as such. This activity accounts for only about 1% of the total isomaltase activity of the mucosa. 6. The results support the concept of the specificity of the human small-intestinal disaccharidases previously described after heat-inactivation experiments. The subfractionation of the invertase that under certain conditions is seen on Sephadex G-200 columns appears most likely to be an artifact. Consequently the nomenclature for the human maltose-, isomaltose- and sucrose-splitting enzymes proposed by another research group after gel-filtration chromatography studies should be abandoned. It seems more logical to keep the nomenclature based on heat inactivation [maltase Ia (=isomaltase), maltase Ib (=invertase or sucrase), maltase II and maltase III] until increased knowledge about the specificity and structure of these enzymes makes possible a more rational nomenclature.
摘要
  1. 采用阴离子交换(二乙氨基乙基纤维素和三乙氨基乙基纤维素)柱色谱法和葡聚糖凝胶G - 200凝胶,对人空肠和回肠可溶性黏膜制剂中的麦芽糖酶、异麦芽糖酶和转化酶(蔗糖酶)活性进行了研究。2. 在离子交换纤维素柱上,两种酶制剂均产生了两个主要的双糖酶峰。第一个峰含有麦芽糖酶Ia(=异麦芽糖酶)和麦芽糖酶Ib(=转化酶)。第二个峰含有麦芽糖酶II和麦芽糖酶III。3. 在葡聚糖凝胶G - 200柱上,空肠制剂产生了与离子交换柱上相应的峰,但峰在流出物中的出现顺序相反。所研究的回肠制剂在凝胶柱上产生了一个单峰,包含所有研究的活性,并以“空体积”洗脱。4. 乙醇沉淀不影响酶在离子交换色谱过程中的行为。然而,当对酶进行乙醇沉淀后进行凝胶过滤时,回肠制剂也获得了两个峰,并且两种制剂都实现了转化酶的亚分级分离。5. 离子交换色谱图中的第二个峰,包含麦芽糖酶II和麦芽糖酶III,浓缩后发现其异麦芽糖酶活性非常弱,可能是由这些酶本身发挥的作用。这种活性仅占黏膜总异麦芽糖酶活性的约1%。6. 这些结果支持了先前在热失活实验后描述的人小肠双糖酶特异性的概念。在某些条件下在葡聚糖凝胶G - 200柱上观察到的转化酶亚分级分离很可能是一种假象。因此,另一个研究小组在凝胶过滤色谱研究后提出的人麦芽糖、异麦芽糖和蔗糖裂解酶的命名法应该被摒弃。在对这些酶的特异性和结构有更多了解,从而有可能采用更合理的命名法之前,保留基于热失活的命名法[麦芽糖酶Ia(=异麦芽糖酶)、麦芽糖酶Ib(=转化酶或蔗糖酶)、麦芽糖酶II和麦芽糖酶III]似乎更合理。

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