Hypertension, Vol 5, 205-210, Copyright © 1983 by American Heart Association
K Nishimura, H Shimizu and T Kokubu
Prokallikrein in the kidney was partially purified with immunoaffinity and
DEAE Sephadex A-50 column chromatographies, and its biochemical properties
were studied in comparison to three active glandular kallikreins purified
from kidney, serum, and urine of the rat. The properties of the enzyme
obtained by trypsin activation of prokallikrein were identical with those
of active glandular kallikreins from the kidney, serum, and urine of the
rat. Apparent molecular weights of prokallikrein, trypsin-activated
kallikrein, active renal kallikrein, and glandular kallikrein in rat serum
were 38,000 and of active urinary kallikrein, 37,000. Prokallikrein
fraction was activated only by trypsin, but not by acidification, pepsin,
and rat urinary esterase A treatments. Renal kallikrein, purified in the
presence of soybean trypsin inhibitor (SBTI), contained 85% prokallikrein,
but the enzymic fraction, purified in the absence of SBTI, contained 23%
prokallikrein. Prokallikrein contents of urinary kallikrein and glandular
kallikrein in rat serum were 16% and 20% respectively. These results
suggest that prokallikrein is produced in the kidney and activated easily
by a trypsin-like enzyme. Since rat serum contains active glandular
kallikrein, kallikrein in the kidney may be secreted not only into the
urine, but also into the blood.
ARTICLES
Existence of prokallikrein in the kidney. Its biochemical properties compared to three active glandular kallikreins from the kidney, serum, and urine of the rat
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