Characterisation of lipofuscin-like lysosomal inclusion bodies from human placenta

A structural hallmark of lysosomes is heterogeneity of their contents. We describe a method for isolation of particulate materials from human placental lysosomes. After a methionine methyl ester-induced disruption of lysosomes and two density gradient centrifugations we obtained a homogeneous membra...

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Veröffentlicht in:	FEBS letters 2007-01, Vol.581 (1), p.102-108
Hauptverfasser:	Schröder, Bernd, Elsässer, Hans-Peter, Schmidt, Bernhard, Hasilik, Andrej
Format:	Artikel
Sprache:	eng
Schlagworte:	2D-PAGE Ageing Cellular Senescence - physiology CTAB Female Humans Inclusion Bodies - chemistry Inclusion Bodies - enzymology Intracellular Membranes - chemistry Intracellular Membranes - enzymology Lipofuscin Lipofuscin - chemistry Lipofuscin - metabolism Lysosomal membrane Lysosomes - chemistry Lysosomes - enzymology methionine methyl ester MME N-cetyl-N,N,N-trimethylammonium bromide Placenta Placenta - chemistry Placenta - enzymology Pregnancy Pregnancy Proteins - chemistry Pregnancy Proteins - metabolism TPPI Tripeptidyl peptidase I two-dimensional gel electrophoresis
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description	A structural hallmark of lysosomes is heterogeneity of their contents. We describe a method for isolation of particulate materials from human placental lysosomes. After a methionine methyl ester-induced disruption of lysosomes and two density gradient centrifugations we obtained a homogeneous membrane fraction and another one enriched in particulate inclusions. The latter exhibited a yellow-brown coloration and contained bodies lacking a delimiting membrane, which were characterised by a granular pattern and high electron density. The lipofuscin-like inclusion materials were rich in tripeptidyl peptidase I, β-glucuronidase, acid ceramidase and apolipoprotein D and contained proteins originating from diverse subcellular localisations. Here we show that human term placenta contains lipofuscin-like lysosomal inclusions, a phenomenon usually associated with senescence in postmitotic cells. These findings imply that a simple pelleting of a lysosomal lysate is not appropriate for the isolation of lysosomal membranes, as the inclusions tend to be sedimented with the membranes.
doi_str_mv	10.1016/j.febslet.2006.12.005
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We describe a method for isolation of particulate materials from human placental lysosomes. After a methionine methyl ester-induced disruption of lysosomes and two density gradient centrifugations we obtained a homogeneous membrane fraction and another one enriched in particulate inclusions. The latter exhibited a yellow-brown coloration and contained bodies lacking a delimiting membrane, which were characterised by a granular pattern and high electron density. The lipofuscin-like inclusion materials were rich in tripeptidyl peptidase I, β-glucuronidase, acid ceramidase and apolipoprotein D and contained proteins originating from diverse subcellular localisations. Here we show that human term placenta contains lipofuscin-like lysosomal inclusions, a phenomenon usually associated with senescence in postmitotic cells. 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We describe a method for isolation of particulate materials from human placental lysosomes. After a methionine methyl ester-induced disruption of lysosomes and two density gradient centrifugations we obtained a homogeneous membrane fraction and another one enriched in particulate inclusions. The latter exhibited a yellow-brown coloration and contained bodies lacking a delimiting membrane, which were characterised by a granular pattern and high electron density. The lipofuscin-like inclusion materials were rich in tripeptidyl peptidase I, β-glucuronidase, acid ceramidase and apolipoprotein D and contained proteins originating from diverse subcellular localisations. Here we show that human term placenta contains lipofuscin-like lysosomal inclusions, a phenomenon usually associated with senescence in postmitotic cells. These findings imply that a simple pelleting of a lysosomal lysate is not appropriate for the isolation of lysosomal membranes, as the inclusions tend to be sedimented with the membranes.</description><subject>2D-PAGE</subject><subject>Ageing</subject><subject>Cellular Senescence - physiology</subject><subject>CTAB</subject><subject>Female</subject><subject>Humans</subject><subject>Inclusion Bodies - chemistry</subject><subject>Inclusion Bodies - enzymology</subject><subject>Intracellular Membranes - chemistry</subject><subject>Intracellular Membranes - enzymology</subject><subject>Lipofuscin</subject><subject>Lipofuscin - chemistry</subject><subject>Lipofuscin - metabolism</subject><subject>Lysosomal membrane</subject><subject>Lysosomes - chemistry</subject><subject>Lysosomes - enzymology</subject><subject>methionine methyl ester</subject><subject>MME</subject><subject>N-cetyl-N,N,N-trimethylammonium bromide</subject><subject>Placenta</subject><subject>Placenta - chemistry</subject><subject>Placenta - enzymology</subject><subject>Pregnancy</subject><subject>Pregnancy Proteins - chemistry</subject><subject>Pregnancy Proteins - metabolism</subject><subject>TPPI</subject><subject>Tripeptidyl peptidase I</subject><subject>two-dimensional gel electrophoresis</subject><issn>0014-5793</issn><issn>1873-3468</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2007</creationdate><recordtype>article</recordtype><sourceid>EIF</sourceid><recordid>eNqNkU9P3DAQxS3UCraUjwDKqbek_pM48akqq6VUQqpU6NmynbHw4sRbOwHtt8dhV-qRnmZGeu_N6DcIXRJcEUz4121lQScPU0Ux5hWhFcbNCVqRrmUlq3n3Aa0wJnXZtIKdoU8pbXGeOyJO0RlpSVuLplmh3-tHFZWZILqkJhfGItjCu12wczJuLL17gsLvU0hhUL5wo_FzWmQ69A5SYWMYisd5UGOx88rAOKnP6KNVPsHFsZ6jPzebh_Vteffrx8_197vS1LQTZQuk6YRRqtWc1IYKow2j0GNNrQbeEK446RjUuq85Zx3raxB5sq3NLqHZOfpyyN3F8HeGNMnBJQPeqxHCnCTvWCtoI7KwOQhNDClFsHIX3aDiXhIsF5hyK48w5QJTEiozzOy7Oi6Y9QD9P9eRXhbcHgQvzsP-_1Llzeaa3i-fWR6DeW7Y243fDlGQiT07iDLjh9FA7yKYSfbBvXPtK1WNn7k</recordid><startdate>20070109</startdate><enddate>20070109</enddate><creator>Schröder, Bernd</creator><creator>Elsässer, Hans-Peter</creator><creator>Schmidt, Bernhard</creator><creator>Hasilik, Andrej</creator><general>Elsevier B.V</general><scope>6I.</scope><scope>AAFTH</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>7X8</scope></search><sort><creationdate>20070109</creationdate><title>Characterisation of lipofuscin-like lysosomal inclusion bodies from human placenta</title><author>Schröder, Bernd ; 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subjects	2D-PAGE Ageing Cellular Senescence - physiology CTAB Female Humans Inclusion Bodies - chemistry Inclusion Bodies - enzymology Intracellular Membranes - chemistry Intracellular Membranes - enzymology Lipofuscin Lipofuscin - chemistry Lipofuscin - metabolism Lysosomal membrane Lysosomes - chemistry Lysosomes - enzymology methionine methyl ester MME N-cetyl-N,N,N-trimethylammonium bromide Placenta Placenta - chemistry Placenta - enzymology Pregnancy Pregnancy Proteins - chemistry Pregnancy Proteins - metabolism TPPI Tripeptidyl peptidase I two-dimensional gel electrophoresis
title	Characterisation of lipofuscin-like lysosomal inclusion bodies from human placenta
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