Characterization of a ribosomal inhibitory polypeptide of protein phosphatase-1 from rat liver

被引：23

作者：

Beullens, M ^{[1
]}

Stalmans, W ^{[1
]}

Bollen, M ^{[1
]}

机构：

[1] CATHOLIC UNIV LEUVEN, AFDELING BIOCHEM, FAC GENEESKUNDE, B-3000 LOUVAIN, BELGIUM

来源：

EUROPEAN JOURNAL OF BIOCHEMISTRY | 1996年 / 239卷 / 01期

关键词：

protein phosphatase; ribosome; dephosphorylation;

D O I：

10.1111/j.1432-1033.1996.0183u.x

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

About 4% of the spontaneous phosphorylase phosphatase activity in a rat liver extract was associated with the ribosomal fraction and stemmed from both protein phosphatase-1 (PP-1) and protein phosphatase-2a (PP-2A). However, after repeated washing: only PP-1 remained bound to the ribosomes. The activity of ribosome-associated PP-1 (PP-1R) was partially latent and could be increased 2-3-fold by incubation with trypsin and an additional 50% by incubation with low concentrations of exogenous type-1 catalytic subunit. In contrast, incubation of the ribosomal fraction with MgATP resulted in a 50% drop in the activity of PP-1R. We have purified from a ribosomal extract a basic polypeptide (pI greater than or equal to 10.5) of 23 kDa that potently inhibited PP-1. This ribosomal inhibitor of PP-1, termed RIPP-1, was at least 30-times less efficient in inhibiting other major Ser/Thr protein phosphatases (PP-2A, PP-2B and PP-2C). RIPP-1 was identified as a non-competitive inhibitor of PP-1 with a substrate-dependent potency. The lowest K-i (approximately 20 nM) was obtained with phosphorylase and myelin basic protein as substrates. Besides instantaneously inhibiting the type-1 catalytic subunit, RIPP-1 also converted the catalytic subunit in a time-dependent manner (t(1/2) = 45 min at 25 degrees C) into a less active conformation. Unlike the inhibition, this slow inactivation was not reversed by the removal of RIPP-1. We propose that RIPP-1 accounts, at least in part, for the latency of PP-1R.

引用

页码：183 / 189

页数：7

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