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在凋亡神经细胞中鉴定“组织”转谷氨酰胺酶结合蛋白。

Identification of 'tissue' transglutaminase binding proteins in neural cells committed to apoptosis.

作者信息

Piredda L, Farrace M G, Lo Bello M, Malorni W, Melino G, Petruzzelli R, Piacentini M

机构信息

Department of Biology, University of Rome 'Tor Vergata' Rome, Italy.

出版信息

FASEB J. 1999 Feb;13(2):355-64. doi: 10.1096/fasebj.13.2.355.

DOI:10.1096/fasebj.13.2.355
PMID:9973324
Abstract

Overexpression of 'tissue' transglutaminase (tTG) in the human neuroblastoma cells increases spontaneous apoptosis and renders these cells highly susceptible to death induced by various stimuli. We used immunoprecipitation to identify cellular proteins that interact specifically with tTG in SK-N-BE(2) -derived stable transfectants. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis analysis showed that tTG binding proteins have molecular masses of 110, 50, 22, 14, and 12 kDa. Microsequencing and computer search analyses allowed us to identify these polypeptides as the beta-tubulin (50 kDa), the histone H2B (14 kDa), and two GST P1-1-truncated forms (22 and 12 kDa). The specificity of the interaction between tTG and these proteins was confirmed by competing tTG binding with purified enzyme and by detecting tTG in immunoprecipitates obtained using beta-tubulin or GST P1-1 mAb's. Here we demonstrate that the GST P1-1 acts as an efficient acyl donor as well as acceptor tTG substrate both in cells and in vitro. The tTG-catalyzed polymerization of GST P1-1 leads to its functional inactivation and is competitively inhibited by GSH. By contrast, the tTG-beta-tubulin interaction does not result in the cross-linking of this cytoskeletal protein, which suggests that microtubules act as the anchorage site for tTG and GST P1-1 interaction.

摘要

人神经母细胞瘤细胞中“组织”转谷氨酰胺酶(tTG)的过表达会增加自发凋亡,并使这些细胞对各种刺激诱导的死亡高度敏感。我们使用免疫沉淀法来鉴定在SK-N-BE(2)衍生的稳定转染子中与tTG特异性相互作用的细胞蛋白。十二烷基硫酸钠-聚丙烯酰胺凝胶电泳分析表明,tTG结合蛋白的分子量分别为110、50、22、14和12 kDa。通过微测序和计算机搜索分析,我们确定这些多肽分别为β-微管蛋白(50 kDa)、组蛋白H2B(14 kDa)以及两种GST P1-1截短形式(22和12 kDa)。tTG与这些蛋白质之间相互作用的特异性通过用纯化酶竞争tTG结合以及用β-微管蛋白或GST P1-1单克隆抗体获得的免疫沉淀物中检测tTG来证实。在此我们证明,GST P1-1在细胞内和体外均作为一种有效的酰基供体以及tTG底物的受体。tTG催化的GST P1-1聚合导致其功能失活,并受到谷胱甘肽的竞争性抑制。相比之下,tTG与β-微管蛋白的相互作用不会导致这种细胞骨架蛋白的交联,这表明微管作为tTG与GST P1-1相互作用的锚定位点。

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