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牛胰蛋白酶的亲和层析。牛α-胰蛋白酶和β-胰蛋白酶的快速分离。

Affinity chromatography of bovine trypsin. A rapid separation of bovine alpha- and beta-trypsin.

作者信息

Jameson G W, Elmore D T

出版信息

Biochem J. 1974 Aug;141(2):555-65. doi: 10.1042/bj1410555.

Abstract

Affinity adsorbents for bovine trypsin were prepared by covalently coupling p-(p'-amino-phenoxypropoxy)benzamidine to cellulose and to agarose. Trypsin binds to both adsorbents at pH6-8 and is released at low pH values or in the presence of n-butylamine hydrochloride. Pure beta-trypsin may be eluted from crude trypsin bound at pH8.0 to the cellulose adsorbent by stepwise elution with an acetate buffer, pH5.0. Both alpha- and beta-trypsin may be isolated by chromatography of crude trypsin on the agarose derivative in an acetate buffer, pH4.0. These two methods for purifying the trypsin are specific to the particular adsorbents. They are rapid and convenient in use. Both methods leave a mixture of the two enzymes bound to the adsorbent and release occurs only at low pH values. The effects of pH, composition and ionic strength of buffer and other variables on both purification methods are described. Affinity adsorbents of soya-bean trypsin inhibitor and of N-alpha-(N'-methyl-N'-sulphanilyl) sulphanilylagmatine bound to agarose were prepared, but were found to be of limited usefulness in the purification of trypsin.

摘要

通过将对(对'-氨基苯氧基丙氧基)苯甲脒共价偶联到纤维素和琼脂糖上,制备了用于牛胰蛋白酶的亲和吸附剂。胰蛋白酶在pH6 - 8时与两种吸附剂结合,并在低pH值或存在盐酸正丁胺的情况下被释放。在pH8.0结合到纤维素吸附剂上的粗胰蛋白酶,通过用pH5.0的醋酸盐缓冲液逐步洗脱,可以洗脱出纯的β-胰蛋白酶。通过在pH4.0的醋酸盐缓冲液中,在琼脂糖衍生物上对粗胰蛋白酶进行色谱分离,可以分离出α-和β-胰蛋白酶。这两种纯化胰蛋白酶的方法对特定的吸附剂具有特异性。它们使用起来快速且方便。两种方法都会使两种酶的混合物结合在吸附剂上,并且只有在低pH值时才会发生释放。描述了pH、缓冲液的组成和离子强度以及其他变量对这两种纯化方法的影响。制备了结合到琼脂糖上的大豆胰蛋白酶抑制剂和N-α-(N'-甲基-N'-磺酰基)磺酰基胍丁胺的亲和吸附剂,但发现它们在胰蛋白酶的纯化中用途有限。

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Affinity chromatography of enzymes on insolubilized cofactors.
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Differential titration of trypsin-like enzymes.类胰蛋白酶的差异滴定
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