Enzymatic preparation of [3H]NADH

## Abstract We have synthesized β‐aminoisobutyric acid (3‐amino‐2‐[^3^H]methyl‐propanoic acid) and β‐ureidoisobutyric acid (3‐[(aminocarbonyl)amino]‐2‐[^3^H]methyl‐propanoic acid) starting with [^3^]thymidine (1‐(2‐deoxy‐β‐D‐ribo‐furanosyl)‐5‐[^3^H]methyluracil). We have developed a simplified enzy

The S y n t h e s i s of t h e bromoprazosin, i n which bromination and a c y l a t i o n of f u r o i c a c i d were completed by means of v e r y simple method was d e s c r i b e d . The r e d u c t i v e c a t a l y z e d debromination with t r i t i u m gas a f f o r d e d t h e ?H)-prazosin.

## Abstract L(+)‐3‐hydroxy(3‐^14^C)butyrate was prepared by treating the D, L‐racemic mixture with the stereospecific D‐(−)‐3‐hydroxybutyrate dehydrogenase enzyme. The unfavorable equilibrium position of the dehydrogenase was overcome by the addition of acetaldehyde and alcohol dehydrogenase. The D

## Abstract ^3^H‐Ochratoxins A, B, and C were obtained by tritiation of the toxins with tritiated water in acetic acid and platinum at 80° C overnight. The toxins were purified by solvent partition and thin layer chromatography with the recovery yield being 80% and the specific activity being 2.6 –

## Abstract Glucocerebroside (1–0‐β‐glucosyl ceramide) can be labeled with ^3^H‐borohydride at the 6‐position of the glucose moiety. The 6‐trityl ether of cerebroside is formed first, the remaining hydroxyl groups are acetylated, the trityl group is removed, and the free 6‐hydroxyl group is oxidize