Degradation of Newly Synthesized Ribosomal Proteins and Histones in Regenerating Rat Liver with and without Treatment with a Low Dose of Actinomycin D

Tsurugi, Kunio; Ogata, Kazuhiro

doi:10.1111/j.1432-1033.1979.tb04233.x

Cited by 21 publications

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“…In this paper we describe the presence of a thiol protease in nuclei of regenerating rat liver which may participate in the degradation of newly synthesized ribosomal proteins and histones as reported previously [4]. Partial purification of the enzyme and some properties of it are also reported.…”

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confidence: 60%

“…Radioactivity was measured using a toluene-based scintillater containing 30 o/, Triton X-100 as described previously [4] and protein was determined by the method of Lowry et al [16].…”

Section: Determination Of Radioactivity and Proteinmentioning

confidence: 99%

“…It was found that newly synthesized ribosomal proteins are degraded rapidly with a half-life of 20-40 min [l] in regenerating rat liver treated with actinomycin D. Recently we showed that the newly synthesized ribosomal proteins accumulated in liver nuclei after injection of E-64, a thiol protease inhibitor [2,3], into actinomycin-D-treated rat liver [4]. Newly synthesized histones also accumulated in nuclei after E-64 treatment, regardless of actinomycin D pretreatment [4]. From these results we concluded that these two kinds of proteins which have not associated with the nascent rRNA or DNA are degraded post-translationally by thiol protease(s) in regenerating rat liver nuclei.…”

mentioning

confidence: 99%

“…Bonner and colleagues isolated a 200 000-M, protease [5,6] and Carter and Chae reported a protease which is active in 2 M NaCl and 5 M urea [7,8]. Since these proteases are inhibited by diisopropylfluorophosphate (iPrd'-F), a specific inhibitor of serine protease, they are different from the protease which were inhibited by administration of E-64 in vivo as described previously [4].…”

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Presence of a Thiol Protease in Regenerating Rat-Liver Nuclei. Partial Purification and Some Properties

1980

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1. Nuclei of regenerating rat liver washed with Triton X-100 were found to contain a new protease. Since the enzymatic activity for degrading ribosomal proteins was inhibited in vivo by administration of E-64, a thiol protease inhibitor, the enzyme may participate in the degradation of newly synthesized ribosomal proteins and histones in regenerating rat liver nuclei as reported previously by us [Biochem. Biophys. Res. Commun. 75, 525-531 (1977)]. The optimum pH was 5.5.2. The enzyme was extracted from washed nuclei and partially purified by gel filtration through Sepharose 6B. Its molecular weight was about 40000. A maximal activity of partially purified enzyme was observed in the presence of 1 mM EDTA and 2 mM dithiothreitol at pH 5.5. It was inhibited by thiol reagents, E-64, leupeptin and heavy metal ions. The enzyme degraded ribosomal proteins endoproteolytically and degraded most proteins tested as substrates, although liver cell sap proteins and serum albumin were less degraded than ribosomal proteins and histones. E-N-Benzoylarginineb-naphthylamide and benzoylarginine amide were not hydrolyzed.When the synthesis of rRNA in regenerating rat liver was selectively inhibited by administration of a low dose of actinomycin D in vivo, the synthesis of ribosomal proteins decreased only slightly [l]. Therefore, ribosomal proteins are synthesized in excess over rRNA. It was found that newly synthesized ribosomal proteins are degraded rapidly with a half-life of 20-40 min [l] in regenerating rat liver treated with actinomycin D. Recently we showed that the newly synthesized ribosomal proteins accumulated in liver nuclei after injection of E-64, a thiol protease inhibitor [2,3], into actinomycin-D-treated rat liver [4]. Newly synthesized histones also accumulated in nuclei after E-64 treatment, regardless of actinomycin D pretreatment [4]. From these results we concluded that these two kinds of proteins which have not associated with the nascent rRNA or DNA are degraded post-translationally by thiol protease(s) in regenerating rat liver nuclei. A few studies on chromatin-bound protease(s) have been reported in rat liver ;

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confidence: 60%

“…Radioactivity was measured using a toluene-based scintillater containing 30 o/, Triton X-100 as described previously [4] and protein was determined by the method of Lowry et al [16].…”

Section: Determination Of Radioactivity and Proteinmentioning

confidence: 99%

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confidence: 99%

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confidence: 99%

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Presence of a Thiol Protease in Regenerating Rat-Liver Nuclei. Partial Purification and Some Properties

1980

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“…From the results we have concluded that these two kinds of proteins, which are not associated with the nascent rRNA or DNA, are degraded post-translationally by thiol protease(s) in the nuclei of regenerating rat liver. It must be added that the degradation of newly synthesized and unassociated ribosomal proteins and especially that of histones may occur in the regenerating liver even without actinomycin D treatment [2]. More recently we demonstrated the presence of an acidic protease in the pure nuclei of regenerating rat liver.…”

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Purification and properties of a thiol protease from rat liver nuclei

Motizuki

Tsurugi

Ogata

1984

European Journal of Biochemistry

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A thiol protease was purified about 800-fold from the chromatin fraction of rat liver by employing Sepharose 6B gel filtration, chromatofocusing and Sephadex G-100 gel filtration. It was nearly homogeneous on sodium dodecyl sulfate/polyacrylamide gel electrophoresis and its molecular weight was about 29 000. The isoelectric point of the enzyme was 7.1. The pH optimum for degradation of 3H-labelled ribosomal proteins was 4.5. It is noticeable that the maximal activity was shifted to pH 5.5 by DNA, and that 30 -40 % of the maximal activity was observed at neutral pH in the presence of DNA. The activity was increased about twice by 2-4 mM dithiothreitol. The protease may be specific for the nuclei because it is different from all lysosomal thiol proteases ever known.When the synthesis of rRNA in regenerating rat liver was selectively inhibited by the administration of a low dose of actinomycin D in vivo, the synthesis of ribosomal proteins remained almost normal 1 h after the actinomycin D treatment. These newly synthesized and unbound ribosomal proteins were found to be degraded rapidly with a half-life of 20 -40 min [I]. Furthermore, we found that the ribosomal proteins and histones, synthesized in actinomycin-D-treated rat liver under the conditions as described above, accumulated in liver nuclei after injection of E-64, a thiol protease inhibitor [2]. From the results we have concluded that these two kinds of proteins, which are not associated with the nascent rRNA or DNA, are degraded post-translationally by thiol protease(s) in the nuclei of regenerating rat liver. It must be added that the degradation of newly synthesized and unassociated ribosomal proteins and especially that of histones may occur in the regenerating liver even without actinomycin D treatment [2]. More recently we demonstrated the presence of an acidic protease in the pure nuclei of regenerating rat liver. It was extracted with 0.7 M NaCl from the chromatin fraction and partially purified with Sepharose 6B. The acidic protease was endopeptidase of a thiol type [3]. During the course of these experiments the presence of the same kind of acidic protease was shown in normal rat liver. Partially purified enzyme from normal rat liver was also sensitive to -SH reagents and had almost the same molecular weight as the enzyme from regenerating rat liver. In the present report the purification of the thiol protease to near homogeneity from normal rat liver chromatin, and some of its characteristics are described. MATERIALS AND METHODS MaterialsWistar strain rats weighing 200 -300 g were used. Iodo-[l-14C]acetamide (23 Ci/mol) was obtained from New England Nuclear Co. Sepharose 6B, Sephadex G-100, PBE94 and Chromatin preparationThe chromatin fraction was prepared from rat liver nuclei as described previously [3]. Briefly, rat liver homogenate in medium A (0.25 M sucrose, 5 mM MgCl,, 25 mM KCl and 50 mM Tris/HCl buffer, pH 7.6) was centrifuged at 10000 x g for 10 min and the precipitate was suspended in 10 volumes of 2.3 M sucrose containing 5 m M MgC...

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Control of protein synthesis and ribosome formation in rat heart

Russo

Morgan

1989

Diabetes Metab. Rev.

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Degradation of Newly Synthesized Ribosomal Proteins and Histones in Regenerating Rat Liver with and without Treatment with a Low Dose of Actinomycin D

Cited by 21 publications

References 28 publications

Presence of a Thiol Protease in Regenerating Rat-Liver Nuclei. Partial Purification and Some Properties

Presence of a Thiol Protease in Regenerating Rat-Liver Nuclei. Partial Purification and Some Properties

Purification and properties of a thiol protease from rat liver nuclei

Control of protein synthesis and ribosome formation in rat heart

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