Hypertension, Vol 2, 595-603, Copyright © 1980 by American Heart Association
G Sagnella, R Price and W Peart
The subcellular distribution and nature of rat renal renin has been
investigated by means of analytical subcellular fractionation and gel
filtration on Sephadex G-100. During differential centrifugation, renin
activity was recovered mainly in soluble and heavy mitochondrial fractions.
On sucrose gradient centrifugation in either a conventional or in a B XIV
zonal rotor, renin activity equilibrated at 1.54 M sucrose and was
partially resolved from marker enzymes for mitochondria (succinate
dehydrogenase), lysosomes (acid phosphatase), plasma membranes (alkaline
phosphatase), and peroxisomes (catalase). On gel filtration of the soluble
or extracts of the renin-granular fractions on Sephadex G-100, renin
activity eluted as a single peak with an apparent molecular weight (MW) of
42,000; no change in activity was found when these fractions were acidified
to pH 3.0. When kidney homogenates were prepared in the presence of the
proteolytic inhibitor N-ethylmaleimide (NEM, 10 mM), whereas the renin from
the granular fractions displayed a MW of 44,000, that from the soluble
fraction was apparently higher (69,000). Addition of NEM (10 mM) to the
soluble fraction previously shown to contain only the low MW form of renin
also resulted in an apparently high MW form of renin. These results
indicate that rat renal renin is associated with a mechanically fragile,
distinct type of subcellular organelle. Renin within this structure is of
the low MW form and is not acid activatable. The soluble fraction, however,
contains a factor(s) that, in the presence of NEM, combines with the low MW
renin to form a complex of apparently high MW.
ARTICLES
Subcellular distribution and storage form of rat renal renin