Simple and rapid procedure for the purification of lipoprotein(a)

Escherichia coZi alkaline phosphatase is a heat-stable, mukimeCc:, metallo-enzyme localized to the periplasmic space of the bacterial cell (I-5). The protein's stability and its specific location have been c>xploited in procedures for purifying this enzyme; for example, after treating bacterial cell

An improvement to the purification method for human salivary peroxidase is presented. The enzyme is obtained at a higher degree of purity in two chromatographic steps instead of four, and avoiding lyophilation treatment. Differences in electrophoretic pattern confirm the genetic polymorphism of the

A protocol of purification is devised that gave high recovery of homogeneous arginase from ox erythrocytes. The protocol involved haemolysis, heat treatment, CM-and DEAE-Sepharose chromatography, arginine AH-Sepharose chromatography and molecular sieving through Biogel P-150, all in the presence of

## Indiana (/rtiversity, Blootnirlgtorr , hrd. 47401 (U.S.A.)

## Abstract A simple and rapid procedure for the preparation of [16,16‐^2^H~2~]‐and [16,16,17‐^2^H~3~]testosterone of high isotopic purity is described. [16,16‐^2^H~2~]DehydrOepiandrosterone is obtained by base‐catalysed exchange; reduction of the 17‐keto group using lithium aluminium hydride or li