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转谷氨酰胺酶催化蛋白质 - 多胺复合物的解离和缔合。

Transglutaminase catalyzed dissociation and association of protein-polyamine complex.

作者信息

Ohtake Yosuke, Nagashima Tomomi, Suyama-Satoh Satoko, Maruko Akiko, Shimura Noriko, Ohkubo Yasuhito

机构信息

Department of Radiopharmacy, Tohoku Pharmaceutical University, 4-4-1 Komatsushima, Sendai, Miyagi, Japan.

出版信息

Life Sci. 2007 Jul 26;81(7):577-84. doi: 10.1016/j.lfs.2007.06.017. Epub 2007 Jul 3.

DOI:10.1016/j.lfs.2007.06.017
PMID:17673261
Abstract

Transglutaminase 2 (TG2) has been reported to be involved in cell growth through the formation of epsilon-(gamma-glutamyl) lysine (Gln-Lys) or N-(gamma-glutamyl) polyamine (Gln-polyamine). We have recently reported that the inhibition of Gln-Lys cross-linking by the formation of Gln-spermidine led to the increase of DNA synthesis in regenerating rat liver. TG2 may catalyze the replacement reaction between Lys residues in protein and polyamines. In the present study, we attempted to develop an experimental model for ascertaining this replacement reaction. We examined whether or not TG2 exhibited the association and dissociation reaction of Gln-polyamine bond in protein, using N,N-dimethylcasein (DC). The dissociated polyamines were identified by autoradiography. The dissociation of [(14)C] polyamines from DC bond [(14)C] polyamines complex by TG2 could occur in the presence of non-radioactive polyamines as second amine donor, whereas in the absence, could not almost occur. Moreover, it was indicated that this release of old [(14)C] polyamine bonded to DC was due to binding of added new [(14)C] polyamine to Gln residues in DC. These results demonstrate that TG2 catalyzes the replacement reaction between added [(14)C] polyamine and DC bond [(14)C] polyamine. The dissociation and association reaction may both occur together, the new DC-polyamine complex being formed at the same time as the dissociation of old DC-polyamine complex, since readying a second amine donor is necessary to dissociate DC-polyamine complex. These results indicate that this experimental model is successful in the study of TG2-catalyzed dissociation and association reaction of Gln-polyamine bond in protein.

摘要

据报道,转谷氨酰胺酶2(TG2)通过形成ε-(γ-谷氨酰基)赖氨酸(Gln-Lys)或N-(γ-谷氨酰基)多胺(Gln-多胺)参与细胞生长。我们最近报道,通过形成Gln-亚精胺抑制Gln-Lys交联导致再生大鼠肝脏中DNA合成增加。TG2可能催化蛋白质中Lys残基与多胺之间的置换反应。在本研究中,我们试图建立一个实验模型来确定这种置换反应。我们使用N,N-二甲基酪蛋白(DC)研究了TG2是否表现出蛋白质中Gln-多胺键的缔合和解离反应。通过放射自显影鉴定解离的多胺。在作为第二胺供体的非放射性多胺存在下,TG2可使[(14)C]多胺从DC键[(14)C]多胺复合物中解离,而在不存在的情况下,几乎不会发生解离。此外,结果表明,与DC结合的旧[(14)C]多胺的释放是由于添加的新[(14)C]多胺与DC中的Gln残基结合所致。这些结果表明,TG2催化添加的[(14)C]多胺与DC键[(14)C]多胺之间的置换反应。解离和缔合反应可能同时发生,新的DC-多胺复合物在旧的DC-多胺复合物解离的同时形成,因为解离DC-多胺复合物需要准备第二胺供体。这些结果表明,该实验模型成功用于研究TG2催化的蛋白质中Gln-多胺键的解离和缔合反应。

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