The Iron-Sulfur Cluster of Iron Regulatory Protein 1 Modulates the Accessibility of RNA Binding and Phosphorylation Sites

Iron regulatory protein 1 (IRP1) modulates iron metabolism by binding to mRNAs encoding proteins involved in the uptake, storage, and metabolic utilization of iron. Iron regulates IRP1 function by promoting assembly of an iron-sulfur cluster in the apo or RNA binding form, thereby converting it to t...

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Veröffentlicht in:	Biochemistry (Easton) 1997-04, Vol.36 (13), p.3950-3958
Hauptverfasser:	Schalinske, Kevin L, Anderson, Sheila A, Tuazon, Polygena T, Chen, Opal S, Kennedy, M. Claire, Eisenstein, Richard S
Format:	Artikel
Sprache:	eng
Schlagworte:	Aconitate Hydratase - metabolism Animals Apoproteins - metabolism Cattle Chymotrypsin - metabolism Electrophoresis, Polyacrylamide Gel Iron - chemistry Iron - metabolism Iron - pharmacology Iron Regulatory Protein 1 Iron-Regulatory Proteins Iron-Sulfur Proteins - chemistry Iron-Sulfur Proteins - isolation & purification Iron-Sulfur Proteins - metabolism Iron-Sulfur Proteins - pharmacology Kinetics Liver - metabolism Mercaptoethanol - pharmacology Peptides - chemistry Phosphorylation Protein Binding Protein Kinase C - antagonists & inhibitors Protein Kinase C - metabolism Rats RNA, Messenger - metabolism RNA-Binding Proteins - chemistry RNA-Binding Proteins - isolation & purification RNA-Binding Proteins - metabolism RNA-Binding Proteins - pharmacology Sulfur - chemistry
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container_issue	13
container_start_page	3950
container_title	Biochemistry (Easton)
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creator	Schalinske, Kevin L Anderson, Sheila A Tuazon, Polygena T Chen, Opal S Kennedy, M. Claire Eisenstein, Richard S
description	Iron regulatory protein 1 (IRP1) modulates iron metabolism by binding to mRNAs encoding proteins involved in the uptake, storage, and metabolic utilization of iron. Iron regulates IRP1 function by promoting assembly of an iron-sulfur cluster in the apo or RNA binding form, thereby converting it to the active holo or cytoplasmic aconitase form. In continuing our studies on phosphoregulation of IRP1 by protein kinase C (PKC), we noted that the purified apoprotein was more efficiently phosphorylated than was the form partially purified from liver cytosol by chromatography on DEAE-Sepharose which had characteristics of the [3Fe-4S] form of the protein. RNA binding measurements revealed a 20-fold increase in RNA binding affinity and a 4−5-fold higher rate of phosphorylation after removal of the Fe-S cluster from the highly purified [4Fe-4S] form. Phosphorylation of apo-IRP1 by PKC was specifically inhibited by IRE-containing RNA. The RNA binding form had a more open structure as judged by its much greater sensitivity to limited cleavage by a number of proteases. N-Terminal sequencing of chymotryptic peptides of apo-IRP1 demonstrated an increased accessibility to proteolysis of sites (residues 132 and 504) near or within the putative cleft of the protein, including regions that are thought to be involved in RNA binding (residues 116−151) and phosphoregulation (Ser 138). Enhanced cleavage was also observed in the proposed hinge linker region (residue 623) on the surface of the protein opposite from the cleft. Taken together, our results indicate that significant structural changes occur in IRP1 during cluster insertion or removal that affect the accessibility to RNA binding and phosphorylation sites.
doi_str_mv	10.1021/bi9624447
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Claire</creatorcontrib><creatorcontrib>Eisenstein, Richard S</creatorcontrib><title>The Iron-Sulfur Cluster of Iron Regulatory Protein 1 Modulates the Accessibility of RNA Binding and Phosphorylation Sites</title><title>Biochemistry (Easton)</title><addtitle>Biochemistry</addtitle><description>Iron regulatory protein 1 (IRP1) modulates iron metabolism by binding to mRNAs encoding proteins involved in the uptake, storage, and metabolic utilization of iron. Iron regulates IRP1 function by promoting assembly of an iron-sulfur cluster in the apo or RNA binding form, thereby converting it to the active holo or cytoplasmic aconitase form. In continuing our studies on phosphoregulation of IRP1 by protein kinase C (PKC), we noted that the purified apoprotein was more efficiently phosphorylated than was the form partially purified from liver cytosol by chromatography on DEAE-Sepharose which had characteristics of the [3Fe-4S] form of the protein. RNA binding measurements revealed a 20-fold increase in RNA binding affinity and a 4−5-fold higher rate of phosphorylation after removal of the Fe-S cluster from the highly purified [4Fe-4S] form. Phosphorylation of apo-IRP1 by PKC was specifically inhibited by IRE-containing RNA. The RNA binding form had a more open structure as judged by its much greater sensitivity to limited cleavage by a number of proteases. N-Terminal sequencing of chymotryptic peptides of apo-IRP1 demonstrated an increased accessibility to proteolysis of sites (residues 132 and 504) near or within the putative cleft of the protein, including regions that are thought to be involved in RNA binding (residues 116−151) and phosphoregulation (Ser 138). Enhanced cleavage was also observed in the proposed hinge linker region (residue 623) on the surface of the protein opposite from the cleft. Taken together, our results indicate that significant structural changes occur in IRP1 during cluster insertion or removal that affect the accessibility to RNA binding and phosphorylation sites.</description><subject>Aconitate Hydratase - metabolism</subject><subject>Animals</subject><subject>Apoproteins - metabolism</subject><subject>Cattle</subject><subject>Chymotrypsin - metabolism</subject><subject>Electrophoresis, Polyacrylamide Gel</subject><subject>Iron - chemistry</subject><subject>Iron - metabolism</subject><subject>Iron - pharmacology</subject><subject>Iron Regulatory Protein 1</subject><subject>Iron-Regulatory Proteins</subject><subject>Iron-Sulfur Proteins - chemistry</subject><subject>Iron-Sulfur Proteins - isolation & purification</subject><subject>Iron-Sulfur Proteins - metabolism</subject><subject>Iron-Sulfur Proteins - pharmacology</subject><subject>Kinetics</subject><subject>Liver - metabolism</subject><subject>Mercaptoethanol - pharmacology</subject><subject>Peptides - chemistry</subject><subject>Phosphorylation</subject><subject>Protein Binding</subject><subject>Protein Kinase C - antagonists & inhibitors</subject><subject>Protein Kinase C - metabolism</subject><subject>Rats</subject><subject>RNA, Messenger - metabolism</subject><subject>RNA-Binding Proteins - chemistry</subject><subject>RNA-Binding Proteins - isolation & purification</subject><subject>RNA-Binding Proteins - metabolism</subject><subject>RNA-Binding Proteins - pharmacology</subject><subject>Sulfur - chemistry</subject><issn>0006-2960</issn><issn>1520-4995</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>1997</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNqFkcFP2zAYxa0JxArbgT9gki9M4hCwYzuJj121DQRjFY24Wo7zmRrSuLMTaf3v59KqJ6SdLH_v957l9yF0TskVJTm9bpwscs55-QFNqMhJxqUUR2hCCCmyXBbkIzqN8SVdOSn5CTqRROZVLiZoUy8B3wbfZ4uxs2PAs26MAwTs7dsYP8Lz2OnBhw2eBz-A6zHFv3y7HULEQ7JPjYEYXeM6N2y2xseHKf7m-tb1z1j3LZ4vfVwvU0TyuJS5cMn6CR1b3UX4vD_PUP3jez27ye5__7ydTe8zzbkYMloJEBKanDEo0l8LWxiwpGkrI3kFhDIqCWNtzppGGk0Msy1jBZVparVlZ-jrLnYd_J8R4qBWLhroOt2DH6MqK0ko4fK_IBVSsqrcgpc70AQfYwCr1sGtdNgoStR2HeqwjsR-2YeOzQraA7nvP-nZTnep9L8HWYdXVZSsFKqeL9TNk6hqOr9TLPEXO16bqF78GPpU3Tvv_gP1yp_f</recordid><startdate>19970401</startdate><enddate>19970401</enddate><creator>Schalinske, Kevin L</creator><creator>Anderson, Sheila A</creator><creator>Tuazon, Polygena T</creator><creator>Chen, Opal S</creator><creator>Kennedy, M. Claire</creator><creator>Eisenstein, Richard S</creator><general>American Chemical Society</general><scope>BSCLL</scope><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>7TM</scope><scope>7X8</scope></search><sort><creationdate>19970401</creationdate><title>The Iron-Sulfur Cluster of Iron Regulatory Protein 1 Modulates the Accessibility of RNA Binding and Phosphorylation Sites</title><author>Schalinske, Kevin L ; Anderson, Sheila A ; Tuazon, Polygena T ; Chen, Opal S ; Kennedy, M. Claire ; Eisenstein, Richard S</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-a445t-185e59eb233e60216f6cef0bd8c948e01319033d23bb9ca0c3fd33619903faf3</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>1997</creationdate><topic>Aconitate Hydratase - metabolism</topic><topic>Animals</topic><topic>Apoproteins - metabolism</topic><topic>Cattle</topic><topic>Chymotrypsin - metabolism</topic><topic>Electrophoresis, Polyacrylamide Gel</topic><topic>Iron - chemistry</topic><topic>Iron - metabolism</topic><topic>Iron - pharmacology</topic><topic>Iron Regulatory Protein 1</topic><topic>Iron-Regulatory Proteins</topic><topic>Iron-Sulfur Proteins - chemistry</topic><topic>Iron-Sulfur Proteins - isolation & purification</topic><topic>Iron-Sulfur Proteins - metabolism</topic><topic>Iron-Sulfur Proteins - pharmacology</topic><topic>Kinetics</topic><topic>Liver - metabolism</topic><topic>Mercaptoethanol - pharmacology</topic><topic>Peptides - chemistry</topic><topic>Phosphorylation</topic><topic>Protein Binding</topic><topic>Protein Kinase C - antagonists & inhibitors</topic><topic>Protein Kinase C - metabolism</topic><topic>Rats</topic><topic>RNA, Messenger - metabolism</topic><topic>RNA-Binding Proteins - chemistry</topic><topic>RNA-Binding Proteins - isolation & purification</topic><topic>RNA-Binding Proteins - metabolism</topic><topic>RNA-Binding Proteins - pharmacology</topic><topic>Sulfur - chemistry</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Schalinske, Kevin L</creatorcontrib><creatorcontrib>Anderson, Sheila A</creatorcontrib><creatorcontrib>Tuazon, Polygena T</creatorcontrib><creatorcontrib>Chen, Opal S</creatorcontrib><creatorcontrib>Kennedy, M. Claire</creatorcontrib><creatorcontrib>Eisenstein, Richard S</creatorcontrib><collection>Istex</collection><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>CrossRef</collection><collection>Nucleic Acids Abstracts</collection><collection>MEDLINE - Academic</collection><jtitle>Biochemistry (Easton)</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Schalinske, Kevin L</au><au>Anderson, Sheila A</au><au>Tuazon, Polygena T</au><au>Chen, Opal S</au><au>Kennedy, M. Claire</au><au>Eisenstein, Richard S</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>The Iron-Sulfur Cluster of Iron Regulatory Protein 1 Modulates the Accessibility of RNA Binding and Phosphorylation Sites</atitle><jtitle>Biochemistry (Easton)</jtitle><addtitle>Biochemistry</addtitle><date>1997-04-01</date><risdate>1997</risdate><volume>36</volume><issue>13</issue><spage>3950</spage><epage>3958</epage><pages>3950-3958</pages><issn>0006-2960</issn><eissn>1520-4995</eissn><abstract>Iron regulatory protein 1 (IRP1) modulates iron metabolism by binding to mRNAs encoding proteins involved in the uptake, storage, and metabolic utilization of iron. Iron regulates IRP1 function by promoting assembly of an iron-sulfur cluster in the apo or RNA binding form, thereby converting it to the active holo or cytoplasmic aconitase form. In continuing our studies on phosphoregulation of IRP1 by protein kinase C (PKC), we noted that the purified apoprotein was more efficiently phosphorylated than was the form partially purified from liver cytosol by chromatography on DEAE-Sepharose which had characteristics of the [3Fe-4S] form of the protein. RNA binding measurements revealed a 20-fold increase in RNA binding affinity and a 4−5-fold higher rate of phosphorylation after removal of the Fe-S cluster from the highly purified [4Fe-4S] form. Phosphorylation of apo-IRP1 by PKC was specifically inhibited by IRE-containing RNA. The RNA binding form had a more open structure as judged by its much greater sensitivity to limited cleavage by a number of proteases. N-Terminal sequencing of chymotryptic peptides of apo-IRP1 demonstrated an increased accessibility to proteolysis of sites (residues 132 and 504) near or within the putative cleft of the protein, including regions that are thought to be involved in RNA binding (residues 116−151) and phosphoregulation (Ser 138). Enhanced cleavage was also observed in the proposed hinge linker region (residue 623) on the surface of the protein opposite from the cleft. Taken together, our results indicate that significant structural changes occur in IRP1 during cluster insertion or removal that affect the accessibility to RNA binding and phosphorylation sites.</abstract><cop>United States</cop><pub>American Chemical Society</pub><pmid>9092825</pmid><doi>10.1021/bi9624447</doi><tpages>9</tpages></addata></record>
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subjects	Aconitate Hydratase - metabolism Animals Apoproteins - metabolism Cattle Chymotrypsin - metabolism Electrophoresis, Polyacrylamide Gel Iron - chemistry Iron - metabolism Iron - pharmacology Iron Regulatory Protein 1 Iron-Regulatory Proteins Iron-Sulfur Proteins - chemistry Iron-Sulfur Proteins - isolation & purification Iron-Sulfur Proteins - metabolism Iron-Sulfur Proteins - pharmacology Kinetics Liver - metabolism Mercaptoethanol - pharmacology Peptides - chemistry Phosphorylation Protein Binding Protein Kinase C - antagonists & inhibitors Protein Kinase C - metabolism Rats RNA, Messenger - metabolism RNA-Binding Proteins - chemistry RNA-Binding Proteins - isolation & purification RNA-Binding Proteins - metabolism RNA-Binding Proteins - pharmacology Sulfur - chemistry
title	The Iron-Sulfur Cluster of Iron Regulatory Protein 1 Modulates the Accessibility of RNA Binding and Phosphorylation Sites
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