A New Combined Purification/Phosphorylation Procedure for Oligodeoxynucleotides

## Methods for growing the fungus, Dactylium dendroides, and for purifying the secreted protein, galactose oxidase, are described. Fungal growth takes 1 week. Enzyme purification takes 2 days and yields 70 mg homogeneous enzyme per 25 liters growth medium.

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

During the preparation of this manuscript, we realized that 3b was also used by others for phosphorylation of DNA [l I].

A general procedure for the purification of chemically synthesized oligoribonucleotides is reported. Purification based on the use of a single reverse-phase HPLC column with buffer systems of differing ion-pairing capacity is described. These methods have been applied to the preparation of a series

A simplified procedure for the preparation of deoxynucleoside methyl-and arylphosphoramidites is described. Both types of phosphoramidites can be conveniently activated by N-methylaniline trifluoracetate for their use in oligodeoxynucleotide synthesis.