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外排-内吞机制蛋白在U373胶质瘤细胞中的表达与分布:与长期培养的星形胶质细胞的相似性

Expression and allocation of proteins of the exo-endocytotic machinery in U373 glioma cells: similarities to long-term cultured astrocytes.

作者信息

Volknandt Walter, Küster Friederike, Wilhelm Alexander, Obermüller Eva, Steinmann Arthur, Zhang Lixia, Zimmermann Herbert

机构信息

Biozentrum der J.W. Goethe-Universität, AK Neurochemie, Zoologisches Institut, Frankfurt am Main, Germany.

出版信息

Cell Mol Neurobiol. 2002 Apr;22(2):153-69. doi: 10.1023/a:1019809704322.

Abstract
  1. Cultured astrocytes cells release a variety of low and high molecular weight messenger substances and express proteins of the exocytotic pathway including synaptic SNARE proteins. For analyzing the molecular mechanisms of astrocytic messenger release, permanent cell lines with astrocytic properties would provide useful tools. 2. We analyzed the potential of the human malignant astrocytoma-derived cell line U373 MG to express proteins involved in regulated exo- and endocytosis. An immunoblot analysis identified the astrocyte marker glial fibrillary acidic protein, microtubule-associated protein 2, the v-SNAREs VAMP I, VAMP II, and cellubrevin and the t-SNAREs syntaxin I, SNAP-23, and SNAP-25. 3. The cells also express the secretory granule protein secretogranin II. Although secretogranin II immunofluorescence reveals larger fluorescence spots, the majority of the SNARE proteins is associated with smaller organelles. The immunofluorescence is distributed throughout the cytoplasm and accumulates at processes and the growing edges of cells. 4. The organellar association of SNARE proteins was confirmed by heterologous expression of recombinant fusion proteins. Following subcellular fractionation organelles of lower buoyant density carried the majority of VAMP 11. Secretogranin II was associated with organelles of high buoyant density containing a small contribution of VAMP II. 5. The results suggest that U373 MG cells have in common a considerable number of properties with long-term cultured astrocytes rather than with cultured oligodendrocytes or neurons. They contain two types of organelles that can be physically separated and may be employed in the differential release of messengers.
摘要
  1. 培养的星形胶质细胞会释放多种低分子量和高分子量的信使物质,并表达胞吐途径的蛋白质,包括突触SNARE蛋白。为了分析星形胶质细胞信使释放的分子机制,具有星形胶质细胞特性的永久细胞系将提供有用的工具。2. 我们分析了源自人恶性星形细胞瘤的细胞系U373 MG表达参与调节胞吐和胞吞作用的蛋白质的潜力。免疫印迹分析鉴定出星形胶质细胞标志物胶质纤维酸性蛋白、微管相关蛋白2、v-SNARE蛋白VAMP I、VAMP II和细胞ubrevin以及t-SNARE蛋白 syntaxin I、SNAP-23和SNAP-25。3. 这些细胞还表达分泌颗粒蛋白分泌粒蛋白II。虽然分泌粒蛋白II免疫荧光显示较大的荧光斑点,但大多数SNARE蛋白与较小的细胞器相关。免疫荧光分布在整个细胞质中,并在细胞的突起和生长边缘积累。4. 通过重组融合蛋白的异源表达证实了SNARE蛋白与细胞器的关联。亚细胞分级分离后,较低浮力密度的细胞器携带了大部分VAMP 11。分泌粒蛋白II与高浮力密度的细胞器相关,其中VAMP II的含量较少。5. 结果表明,U373 MG细胞与长期培养的星形胶质细胞有相当多的共同特性,而与培养的少突胶质细胞或神经元不同。它们含有两种可以物理分离的细胞器,可能用于信使的差异释放。

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