Abstract
Isolated rat pancreatic islets were pulse-labeled for 5 min with [3H]leucine then chased for 25 min, during which time endogenously labeled [3H]proinsulin becomes predominantly compartmented in immature secretory granules. The islets were then homogenized in isotonic sucrose (pH 7.4) and a beta-granule preparation obtained by differential centrifugation and discontinuous sucrose gradient ultracentrifugation. This preparation was enriched 8-fold in beta-granules. Aside from contamination with mitochondria and a limited number of lysosomes, the beta-granule preparation was essentially free of any other organelles involved in proinsulin synthesis and packaging (i.e. microsomal elements and, more particularly, Golgi complex). Conversion of endogenously labeled [3H]proinsulin was followed in this beta-granule fraction for up to 2 h at 37 degrees C in a buffer (pH 7.3) that mimicked the cationic constituents of B-cell cytosol, during which time 92% of the beta-granules remained intact. Proinsulin conversion was analyzed by high performance liquid chromatography. The rate of proinsulin conversion to insulin was stimulated by 2.2 +/- 0.1-fold (n = 6) (at a 60-min incubation) in the presence of ATP (2 mM) and an ATP regenerating system compared to beta-granule preparations incubated without ATP. This ATP stimulation was abolished in the presence of beta-granule proton pump ATPase inhibitors (tributyltin, 2.5 microM, or 1,3-dicyclohexylcarbodiimide, 50 microM). Inhibitors of mitochondrial proton pump ATPases (sodium azide, 20 mM, or oligomycin, 10 micrograms/ml) had no effect on the ATP stimulation of proinsulin conversion. When granules were incubated in a more acidic buffer (pH 5.5), proinsulin conversion was increased relative to that at pH 7.3. At pH 5.5, ATP no longer stimulated conversion, and tributyltin and 1,3-dicyclohexylcarbodiimide had no effect. Disrupted granules only converted proinsulin to a limited extent, and neither ATP nor the inhibitors affected conversion. It is therefore suggested that ATP stimulation of proinsulin conversion in isolated, intact, beta-granules is secondary to intragranular acidification by an ATP-dependent proton pump (reflecting the low pH optimum for proinsulin conversion), rather than ATP dependence of converting activity per se.
Highlights
Whichtimeendogenouslylabeled[3H]proinsulin becomes predominantly compartmented in immature secretory granules
Again in contrast to previous studies [10,11,12,13,14], in order to ensure that this in vitro endogenous proinsulin conversion was only monitored in @granules, the granule purification methodology was focused toward purification away from other organelles involved in the proinsulin synthesis and packaging pathway (i.e. endoplasmic reticulum and Golgi complex [6])
In afirst series of experiments, the effect of 2 mM ATP on proinsulin conversion was studied over a2-h incubation period at 37 “C. The percentage of conversion in the isolated @-granulesat the starotf the incubation, which was 8.4 f 1.7% ( n= 3) for this series, was subtracted from the later values in order to obtain data for specific conversion during the incubation period
Summary
$Recipient of a Wellcome Trust Travel Award. Towhom all DCCD, 1,3-dicyclohexylcarbodiimideE; GTA, [ethylenebis(oxyethylcorrespondence should be addressed (present address): University of enenitri1o)ltetraacetic acid HEPES, 4-(2-hydroxyethyl)-l-piperaCambridge, Dept. of Clinical Biochemistry, Addenbrookes Hospital, zineethanesulfonic acid HPLC, high performance liquid chromatog-. Again in contrast to previous studies [10,11,12,13,14], in order to ensure that this in vitro endogenous proinsulin conversion was only monitored in @granules, the granule purification methodology was focused toward purification away from other organelles involved in the proinsulin synthesis and packaging pathway (i.e. endoplasmic reticulum and Golgi complex [6]) By using this i n vitro system it may be possible to demonstrate the additional factors needed to allow proinsulin conversion rates in isolated secretory granule preparations to approach thoseobserved in intact cells
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