FAS activation induces dephosphorylation of SR proteins; dependence on the de novo generation of ceramide and activation of protein phosphatase 1
The search for potential targets for ceramide action led to the identification of ceramide-activated protein phosphatases (CAPP). To date, two serine/threonine protein phosphatases, protein phosphatase 2A (PP2A) and protein phosphatase 1 (PP1), have been demonstrated to function as ceramide-activate...
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| Veröffentlicht in: | The Journal of biological chemistry 2001-11, Vol.276 (48), p.44848 |
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| creator | Chalfant, C E Ogretmen, B Galadari, S Kroesen, B J Pettus, B J Hannun, Y A |
| description | The search for potential targets for ceramide action led to the identification of ceramide-activated protein phosphatases (CAPP). To date, two serine/threonine protein phosphatases, protein phosphatase 2A (PP2A) and protein phosphatase 1 (PP1), have been demonstrated to function as ceramide-activated protein phosphatases. In this study, we show that treatment with either anti-FAS IgM (CH-11) (150 ng/ml) or exogenous d-(e)-C(6-)ceramide (20 microm) induces the dephosphorylation of the PP1 substrates, serine/arginine-rich (SR) proteins, in Jurkat acute leukemia T-cells. The serine/threonine protein phosphatase inhibitor, calyculin A, but not the PP2A-specific inhibitor, okadaic acid, inhibited both FAS- and ceramide-induced dephosphorylation of SR proteins. Anti-FAS IgM treatment of Jurkat cells led to a significant increase in levels of endogenous ceramide beginning at 2 h with a maximal increase of 10-fold after 7 h. A 2-h pretreatment of Jurkat cells with fumonisin B(1) (100 microm), a specific inhibitor of CoA-dependent ceramide synthase, blocked 80% of the ceramide generated and completely inhibited the dephosphorylation of SR proteins in response to anti-FAS IgM. Moreover, pretreatment of Jurkat cells with myriocin, a specific inhibitor of serine-palmitoyl transferase (the first step in de novo synthesis of ceramide), also blocked FAS-induced SR protein dephosphorylation, thus demonstrating a role for de novo ceramide. These results were further supported using A549 lung adenocarcinoma cells treated with d-(e)-C(6-)ceramide. Dephosphorylation of SR proteins was inhibited by fumonisin B(1) and by overexpression of glucosylceramide synthase; again implicating endogenous ceramide generated de novo in regulating the dephosphorylation of SR proteins in response to FAS activation. These results establish a specific intracellular pathway involving both de novo ceramide generation and activation of PP1 to mediate the effects of FAS activation on SR proteins. |
| doi_str_mv | 10.1074/jbc.M106291200 |
| format | Article |
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To date, two serine/threonine protein phosphatases, protein phosphatase 2A (PP2A) and protein phosphatase 1 (PP1), have been demonstrated to function as ceramide-activated protein phosphatases. In this study, we show that treatment with either anti-FAS IgM (CH-11) (150 ng/ml) or exogenous d-(e)-C(6-)ceramide (20 microm) induces the dephosphorylation of the PP1 substrates, serine/arginine-rich (SR) proteins, in Jurkat acute leukemia T-cells. The serine/threonine protein phosphatase inhibitor, calyculin A, but not the PP2A-specific inhibitor, okadaic acid, inhibited both FAS- and ceramide-induced dephosphorylation of SR proteins. Anti-FAS IgM treatment of Jurkat cells led to a significant increase in levels of endogenous ceramide beginning at 2 h with a maximal increase of 10-fold after 7 h. A 2-h pretreatment of Jurkat cells with fumonisin B(1) (100 microm), a specific inhibitor of CoA-dependent ceramide synthase, blocked 80% of the ceramide generated and completely inhibited the dephosphorylation of SR proteins in response to anti-FAS IgM. Moreover, pretreatment of Jurkat cells with myriocin, a specific inhibitor of serine-palmitoyl transferase (the first step in de novo synthesis of ceramide), also blocked FAS-induced SR protein dephosphorylation, thus demonstrating a role for de novo ceramide. These results were further supported using A549 lung adenocarcinoma cells treated with d-(e)-C(6-)ceramide. Dephosphorylation of SR proteins was inhibited by fumonisin B(1) and by overexpression of glucosylceramide synthase; again implicating endogenous ceramide generated de novo in regulating the dephosphorylation of SR proteins in response to FAS activation. 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To date, two serine/threonine protein phosphatases, protein phosphatase 2A (PP2A) and protein phosphatase 1 (PP1), have been demonstrated to function as ceramide-activated protein phosphatases. In this study, we show that treatment with either anti-FAS IgM (CH-11) (150 ng/ml) or exogenous d-(e)-C(6-)ceramide (20 microm) induces the dephosphorylation of the PP1 substrates, serine/arginine-rich (SR) proteins, in Jurkat acute leukemia T-cells. The serine/threonine protein phosphatase inhibitor, calyculin A, but not the PP2A-specific inhibitor, okadaic acid, inhibited both FAS- and ceramide-induced dephosphorylation of SR proteins. Anti-FAS IgM treatment of Jurkat cells led to a significant increase in levels of endogenous ceramide beginning at 2 h with a maximal increase of 10-fold after 7 h. A 2-h pretreatment of Jurkat cells with fumonisin B(1) (100 microm), a specific inhibitor of CoA-dependent ceramide synthase, blocked 80% of the ceramide generated and completely inhibited the dephosphorylation of SR proteins in response to anti-FAS IgM. Moreover, pretreatment of Jurkat cells with myriocin, a specific inhibitor of serine-palmitoyl transferase (the first step in de novo synthesis of ceramide), also blocked FAS-induced SR protein dephosphorylation, thus demonstrating a role for de novo ceramide. These results were further supported using A549 lung adenocarcinoma cells treated with d-(e)-C(6-)ceramide. Dephosphorylation of SR proteins was inhibited by fumonisin B(1) and by overexpression of glucosylceramide synthase; again implicating endogenous ceramide generated de novo in regulating the dephosphorylation of SR proteins in response to FAS activation. These results establish a specific intracellular pathway involving both de novo ceramide generation and activation of PP1 to mediate the effects of FAS activation on SR proteins.</description><subject>Blotting, Western</subject><subject>Carboxylic Acids - pharmacology</subject><subject>Cell Line</subject><subject>Ceramides - biosynthesis</subject><subject>Diacylglycerol Kinase - metabolism</subject><subject>Electrophoresis, Polyacrylamide Gel</subject><subject>Enzyme Activation</subject><subject>Enzyme Inhibitors - pharmacology</subject><subject>fas Receptor - metabolism</subject><subject>Fumonisins</subject><subject>Humans</subject><subject>Jurkat Cells</subject><subject>Palmitic Acid - metabolism</subject><subject>Phosphoprotein Phosphatases - metabolism</subject><subject>Phosphoric Monoester Hydrolases - metabolism</subject><subject>Phosphorylation</subject><subject>Protein Phosphatase 1</subject><subject>Protein Phosphatase 2</subject><subject>Sarcoplasmic Reticulum - metabolism</subject><subject>Serine - metabolism</subject><subject>Sphingolipids - metabolism</subject><subject>Threonine - metabolism</subject><subject>Time Factors</subject><issn>0021-9258</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2001</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNpNkNtKA0EMhudCsbV666XMC2xNZg-zxatSrAoVwep1mUPGbmlnl51toY_hGzuyVQyEhHzJ_0MYu0EYI8jsbqPN-AWhEBMUAGdsCCAwmYi8HLDLEDYQI5vgBRsg5iBkDkP2NZ8uuTJddVBdVXteebs3FLilZl2HmO1x25Pa8eUbb9q6o8qH-58N8pa8IR5pt6Y44b4-1PyTPLV_Ryb2uyoy5e1_p4hOYry3Up0KxPGKnTu1DXR9qiP2MX94nz0li9fH59l0kTQCZJc4gaRzh1I4KmJBC9KVgoAwLWSKpkwNGiG1LkAo5SjXmUtFZjNBRpQ6HbHbXrfZ6x3ZVdNWO9UeV7-_Sb8BqfpnhA</recordid><startdate>20011130</startdate><enddate>20011130</enddate><creator>Chalfant, C E</creator><creator>Ogretmen, B</creator><creator>Galadari, S</creator><creator>Kroesen, B J</creator><creator>Pettus, B J</creator><creator>Hannun, Y A</creator><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope></search><sort><creationdate>20011130</creationdate><title>FAS activation induces dephosphorylation of SR proteins; dependence on the de novo generation of ceramide and activation of protein phosphatase 1</title><author>Chalfant, C E ; Ogretmen, B ; Galadari, S ; Kroesen, B J ; Pettus, B J ; Hannun, Y A</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-p207t-f21eb5f172fe6f171d07f82e0e136731c83c1c27bb602aafe5b4f324d42ec28b3</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2001</creationdate><topic>Blotting, Western</topic><topic>Carboxylic Acids - pharmacology</topic><topic>Cell Line</topic><topic>Ceramides - biosynthesis</topic><topic>Diacylglycerol Kinase - metabolism</topic><topic>Electrophoresis, Polyacrylamide Gel</topic><topic>Enzyme Activation</topic><topic>Enzyme Inhibitors - pharmacology</topic><topic>fas Receptor - metabolism</topic><topic>Fumonisins</topic><topic>Humans</topic><topic>Jurkat Cells</topic><topic>Palmitic Acid - metabolism</topic><topic>Phosphoprotein Phosphatases - metabolism</topic><topic>Phosphoric Monoester Hydrolases - metabolism</topic><topic>Phosphorylation</topic><topic>Protein Phosphatase 1</topic><topic>Protein Phosphatase 2</topic><topic>Sarcoplasmic Reticulum - metabolism</topic><topic>Serine - metabolism</topic><topic>Sphingolipids - metabolism</topic><topic>Threonine - metabolism</topic><topic>Time Factors</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Chalfant, C E</creatorcontrib><creatorcontrib>Ogretmen, B</creatorcontrib><creatorcontrib>Galadari, S</creatorcontrib><creatorcontrib>Kroesen, B J</creatorcontrib><creatorcontrib>Pettus, B J</creatorcontrib><creatorcontrib>Hannun, Y A</creatorcontrib><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><jtitle>The Journal of biological chemistry</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Chalfant, C E</au><au>Ogretmen, B</au><au>Galadari, S</au><au>Kroesen, B J</au><au>Pettus, B J</au><au>Hannun, Y A</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>FAS activation induces dephosphorylation of SR proteins; dependence on the de novo generation of ceramide and activation of protein phosphatase 1</atitle><jtitle>The Journal of biological chemistry</jtitle><addtitle>J Biol Chem</addtitle><date>2001-11-30</date><risdate>2001</risdate><volume>276</volume><issue>48</issue><spage>44848</spage><pages>44848-</pages><issn>0021-9258</issn><abstract>The search for potential targets for ceramide action led to the identification of ceramide-activated protein phosphatases (CAPP). To date, two serine/threonine protein phosphatases, protein phosphatase 2A (PP2A) and protein phosphatase 1 (PP1), have been demonstrated to function as ceramide-activated protein phosphatases. In this study, we show that treatment with either anti-FAS IgM (CH-11) (150 ng/ml) or exogenous d-(e)-C(6-)ceramide (20 microm) induces the dephosphorylation of the PP1 substrates, serine/arginine-rich (SR) proteins, in Jurkat acute leukemia T-cells. The serine/threonine protein phosphatase inhibitor, calyculin A, but not the PP2A-specific inhibitor, okadaic acid, inhibited both FAS- and ceramide-induced dephosphorylation of SR proteins. Anti-FAS IgM treatment of Jurkat cells led to a significant increase in levels of endogenous ceramide beginning at 2 h with a maximal increase of 10-fold after 7 h. A 2-h pretreatment of Jurkat cells with fumonisin B(1) (100 microm), a specific inhibitor of CoA-dependent ceramide synthase, blocked 80% of the ceramide generated and completely inhibited the dephosphorylation of SR proteins in response to anti-FAS IgM. Moreover, pretreatment of Jurkat cells with myriocin, a specific inhibitor of serine-palmitoyl transferase (the first step in de novo synthesis of ceramide), also blocked FAS-induced SR protein dephosphorylation, thus demonstrating a role for de novo ceramide. These results were further supported using A549 lung adenocarcinoma cells treated with d-(e)-C(6-)ceramide. Dephosphorylation of SR proteins was inhibited by fumonisin B(1) and by overexpression of glucosylceramide synthase; again implicating endogenous ceramide generated de novo in regulating the dephosphorylation of SR proteins in response to FAS activation. These results establish a specific intracellular pathway involving both de novo ceramide generation and activation of PP1 to mediate the effects of FAS activation on SR proteins.</abstract><cop>United States</cop><pmid>11502750</pmid><doi>10.1074/jbc.M106291200</doi><oa>free_for_read</oa></addata></record> |
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| subjects | Blotting, Western Carboxylic Acids - pharmacology Cell Line Ceramides - biosynthesis Diacylglycerol Kinase - metabolism Electrophoresis, Polyacrylamide Gel Enzyme Activation Enzyme Inhibitors - pharmacology fas Receptor - metabolism Fumonisins Humans Jurkat Cells Palmitic Acid - metabolism Phosphoprotein Phosphatases - metabolism Phosphoric Monoester Hydrolases - metabolism Phosphorylation Protein Phosphatase 1 Protein Phosphatase 2 Sarcoplasmic Reticulum - metabolism Serine - metabolism Sphingolipids - metabolism Threonine - metabolism Time Factors |
| title | FAS activation induces dephosphorylation of SR proteins; dependence on the de novo generation of ceramide and activation of protein phosphatase 1 |
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