A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum
博士 === 國立清華大學 === 分子醫學研究所 === 99 === Postsynaptic density (PSD) is a protein supramolecule lying underneath the postsynaptic membrane of excitatory synapses and has been implicated to play important roles in synaptic structure and function in mammalian central nervous system. Here, PSDs were isolate...
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ndltd-TW-099NTHU55380192015-10-13T20:23:00Z http://ndltd.ncl.edu.tw/handle/72419789991381232509 A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum 豬大腦皮質和小腦後突觸質密區內蛋白質空間排列結構之研究 Yen, Yun-Hong 嚴元宏 博士 國立清華大學 分子醫學研究所 99 Postsynaptic density (PSD) is a protein supramolecule lying underneath the postsynaptic membrane of excitatory synapses and has been implicated to play important roles in synaptic structure and function in mammalian central nervous system. Here, PSDs were isolated from two distinct regions of porcine brain, cerebral cortex and cerebellum. SDS-PAGE and Western blotting analyses indicated that cerebral and cerebellar PSDs consisted of a similar set of proteins with noticeable differences in the abundance of various proteins between these samples. Subsequently, protein localization in these PSDs was analyzed by using the Nano-Depth-Tagging (NDT) method. This method involved the use of three synthetic reagents, as agarose beads whose surface was covalently linked with a fluorescent, photoactivable and cleavable chemical crosslinker by spacers of varied lengths. After its application was verified by using a synthetic complex consisting of four layers of different proteins, the NDT method was used here to yield information concerning the depth distribution of various proteins in the PSD. The results indicated that in both cerebral and cerebellar PSDs, glutamate receptors, actin and actin binding proteins resided in the peripheral regions within ~10 nm deep from the surface and that scaffold proteins, tubulin subunits, microtubule-binding proteins, membrane cytoskeleton proteins found in mammalian erythrocytes resided in the interiors deeper than 10 nm from the surface in the PSD. Finally, by using immunoabsorption method, binding partner proteins of two proteins residing in the interiors, PSD-95 and α-tubulin, and those of two proteins residing in the peripheral regions, elongation factor-1α and calcium, calmodulin-dependent protein kinase II α subunit, of cerebral and cerebellar PSDs were identified. Overall, the results indicate a striking similarity in protein organization between the PSDs isolated from porcine cerebral cortex and cerebellum. A model of the molecular structure of the PSD has also been proposed here. Chang, Yen-Chung 張兗君 2011 學位論文 ; thesis 87 zh-TW |
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博士 === 國立清華大學 === 分子醫學研究所 === 99 === Postsynaptic density (PSD) is a protein supramolecule lying underneath the postsynaptic membrane of excitatory synapses and has been implicated to play important roles in synaptic structure and function in mammalian central nervous system. Here, PSDs were isolated from two distinct regions of porcine brain, cerebral cortex and cerebellum. SDS-PAGE and Western blotting analyses indicated that cerebral and cerebellar PSDs consisted of a similar set of proteins with noticeable differences in the abundance of various proteins between these samples. Subsequently, protein localization in these PSDs was analyzed by using the Nano-Depth-Tagging (NDT) method. This method involved the use of three synthetic reagents, as agarose beads whose surface was covalently linked with a fluorescent, photoactivable and cleavable chemical crosslinker by spacers of varied lengths. After its application was verified by using a synthetic complex consisting of four layers of different proteins, the NDT method was used here to yield information concerning the depth distribution of various proteins in the PSD. The results indicated that in both cerebral and cerebellar PSDs, glutamate receptors, actin and actin binding proteins resided in the peripheral regions within ~10 nm deep from the surface and that scaffold proteins, tubulin subunits, microtubule-binding proteins, membrane cytoskeleton proteins found in mammalian erythrocytes resided in the interiors deeper than 10 nm from the surface in the PSD. Finally, by using immunoabsorption method, binding partner proteins of two proteins residing in the interiors, PSD-95 and α-tubulin, and those of two proteins residing in the peripheral regions, elongation factor-1α and calcium, calmodulin-dependent protein kinase II α subunit, of cerebral and cerebellar PSDs were identified. Overall, the results indicate a striking similarity in protein organization between the PSDs isolated from porcine cerebral cortex and cerebellum. A model of the molecular structure of the PSD has also been proposed here.
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author2 |
Chang, Yen-Chung |
author_facet |
Chang, Yen-Chung Yen, Yun-Hong 嚴元宏 |
author |
Yen, Yun-Hong 嚴元宏 |
spellingShingle |
Yen, Yun-Hong 嚴元宏 A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum |
author_sort |
Yen, Yun-Hong |
title |
A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum |
title_short |
A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum |
title_full |
A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum |
title_fullStr |
A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum |
title_full_unstemmed |
A study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum |
title_sort |
study of the spatial protein organization of the postsynaptic density isolated from porcine cerebral cortex and cerebellum |
publishDate |
2011 |
url |
http://ndltd.ncl.edu.tw/handle/72419789991381232509 |
work_keys_str_mv |
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