组织转谷氨酰胺酶Gh的核心结构域可水解鸟苷三磷酸(GTP)和三磷酸腺苷(ATP)。
The core domain of the tissue transglutaminase Gh hydrolyzes GTP and ATP.
作者信息
Iismaa S E, Chung L, Wu M J, Teller D C, Yee V C, Graham R M
机构信息
Victor Chang Cardiac Research Institute, St Vincent's Hospital, Darlinghurst, NSW, 2010, Australia.
出版信息
Biochemistry. 1997 Sep 30;36(39):11655-64. doi: 10.1021/bi970545e.
Tissue transglutaminase (TGase II) catalyzes the posttranslational modification of proteins by transamidation of available glutamine residues and is also a guanosinetriphosphatase (GTPase) and adenosinetriphosphatase (ATPase). Based on its homology with factor XIIIA, an extracellular transglutaminase, the structure of TGase II is likely composed of an N-terminal beta-sandwich domain, an alpha/beta catalytic core, and two C-terminally located beta-barrels. Here we used a domain-deletion approach to identify the GTP and ATP hydrolytic domains of TGase II. Full-length TGase II and two domain-deletion mutants, one retaining the N-terminal beta-sandwich and core domains (betaSCore) and the other retaining only the core domain, were expressed as glutathione S-transferase (GST) fusion proteins and purified. GST-Full and GST-betaSCore exhibited calcium-dependent TGase activity, whereas GST-Core had no detectable TGase activity, indicating the beta-sandwich domain is required for TGase activity but the C-terminal beta-barrels are not. All three GST-TGase II fusion proteins were photoaffinity-labeled with [alpha-32P]-8-azidoGTP and were able to bind GTP-agarose. The GTPase activity of GST-betaSCore was equivalent to that of GST-Full, whereas the ATPase activity was approximately 40% higher than GST-Full. GST-Core had approximately 50% higher GTPase activity and approximately 75% higher ATPase activity than GST-Full. The GTPase and ATPase activities of each of the GST-TGase II fusion proteins were inhibited in a dose-dependent manner by both GTPgammaS and ATPgammaS. These results demonstrate that the GTP and ATP hydrolysis sites are localized within the core domain of TGase II and that neither the N-terminal beta-sandwich domain nor the C-terminal beta-barrels are required for either GTP or ATP hydrolysis. Taken together with previous work [Singh, U. S., Erickson, J. W., & Cerione, R. A. (1995) Biochemistry 34, 15863-15871; Lai, T.-S., Slaughter, T. F., Koropchak, C. M., Haroon, Z. A., & Greenberg, C. S. (1996) J. Biol. Chem. 271, 31191-31195] the results of this study indicate that the GTP and ATP hydrolysis sites are localized to a 5. 5 kDa (47 amino acid) region at the start of the core domain.
组织转谷氨酰胺酶(TGase II)通过使可用的谷氨酰胺残基转酰胺化来催化蛋白质的翻译后修饰,并且还是一种鸟苷三磷酸酶(GTPase)和腺苷三磷酸酶(ATPase)。基于其与细胞外转谷氨酰胺酶因子 XIIIA 的同源性,TGase II 的结构可能由一个 N 端β-折叠结构域、一个α/β催化核心和两个位于 C 端的β-桶结构组成。在这里,我们使用结构域缺失方法来鉴定 TGase II 的 GTP 和 ATP 水解结构域。全长 TGase II 和两个结构域缺失突变体,一个保留 N 端β-折叠和核心结构域(βSCore),另一个仅保留核心结构域,被表达为谷胱甘肽 S-转移酶(GST)融合蛋白并进行纯化。GST-Full 和 GST-βSCore 表现出钙依赖性 TGase 活性,而 GST-Core 没有可检测到的 TGase 活性,这表明β-折叠结构域是 TGase 活性所必需的,但 C 端β-桶结构不是。所有三种 GST-TGase II 融合蛋白都用[α-32P]-8-叠氮基 GTP 进行光亲和标记,并且能够结合 GTP-琼脂糖。GST-βSCore 的 GTPase 活性与 GST-Full 相当,而其 ATPase 活性比 GST-Full 高约 40%。GST-Core 的 GTPase 活性比 GST-Full 高约 50%,ATPase 活性比 GST-Full 高约 75%。每种 GST-TGase II 融合蛋白的 GTPase 和 ATPase 活性都被 GTPγS 和 ATPγS 以剂量依赖性方式抑制。这些结果表明,GTP 和 ATP 水解位点位于 TGase II 的核心结构域内,并且 N 端β-折叠结构域和 C 端β-桶结构对于 GTP 或 ATP 水解都不是必需的。结合先前的工作[Singh, U. S., Erickson, J. W., & Cerione, R. A. (1995) Biochemistry 34, 15863 - 15871; Lai, T.-S., Slaughter, T. F., Koropchak, C. M., Haroon, Z. A., & Greenberg, C. S. (1996) J. Biol. Chem. 2, 31191 - 31195],本研究结果表明,GTP 和 ATP 水解位点位于核心结构域起始处的一个 5.5 kDa(47 个氨基酸)区域。
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