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利用乙酰氧基香豆素作为乙酰基供体对纯化的钙网蛋白转乙酰酶进行自身乙酰化。

Autoacetylation of purified calreticulin transacetylase utilizing acetoxycoumarin as the acetyl group donor.

作者信息

Bansal Seema, Ponnan Prija, Raj Hanumantharao G, Weintraub Susan T, Chopra Madhu, Kumari Ranju, Saluja Daman, Kumar Ajit, Tyagi Tapesh K, Singh Prabhjot, Prasad Ashok K, Saso Luciano, Rastogi Ramesh C, Parmar Virinder S

机构信息

Department of Biochemistry, V. P. Chest Institute, University of Delhi, Delhi 1100 07, India.

出版信息

Appl Biochem Biotechnol. 2009 May;157(2):285-98. doi: 10.1007/s12010-008-8357-2. Epub 2008 Sep 16.

DOI:10.1007/s12010-008-8357-2
PMID:18795239
Abstract

Our earlier reports documented that calreticulin, a multifunctional Ca2+-binding protein in endoplasmic reticulum lumen, possessed protein acetyltransferase function termed Calreticulin Transacetylase (CRTAase). The autoacetylation of purified human placental CRTAase concomitant with the acetylation of receptor proteins by a model acetoxycoumarin, 7,8-Diacetoxy-4-methylcoumarin, was observed. Here, we have examined the autoacetylation property of CRTAase by immunoblotting and mass spectrometry. Ca2+ was found to inhibit CRTAase activity. The inhibition of both autoacetylation of CRTAase as well as acetylation of the receptor protein was apparent when Ca2+) was included in the reaction mixture as visualized by interaction with anti-acetyl lysine antibody. The acetylation of lysines residues: -48, -62, -64, -153, and -159 in N-domain and -206, -207, -209, and -238 in P-domain of CRTAase were located by high-performance liquid chromatography-electronspray ionization tandem mass spectrometry. Further, computer assisted protein structure modeling studies were undertaken to probe the effect of autoacetylation of CRTAase. Accordingly, the predicted CRTAase 3D model showed that all the loop regions of both N- and P-domain bear the acetylated lysines. Energy minimization of the acetylated residues revealed charge neutralization of lysines due to the N-epsilon-acetylation which may facilitate the interaction of CRTAase with the protein substrate and the subsequent transacetylase action.

摘要

我们早期的报告记录了钙网蛋白,一种内质网腔中的多功能钙离子结合蛋白,具有名为钙网蛋白转乙酰酶(CRTAase)的蛋白质乙酰转移酶功能。观察到纯化的人胎盘CRTAase的自乙酰化与模型乙酰氧基香豆素7,8 - 二乙酰氧基 - 4 - 甲基香豆素对受体蛋白的乙酰化同时发生。在这里,我们通过免疫印迹和质谱法研究了CRTAase的自乙酰化特性。发现钙离子会抑制CRTAase的活性。当反应混合物中加入钙离子时,通过与抗乙酰赖氨酸抗体的相互作用可视化,CRTAase的自乙酰化以及受体蛋白的乙酰化均受到明显抑制。通过高效液相色谱 - 电喷雾电离串联质谱法确定了CRTAase的N结构域中赖氨酸残基 - 48、 - 62、 - 64、 - 153和 - 159以及P结构域中赖氨酸残基 - 206、 - 207、 - 209和 - 238的乙酰化情况。此外,进行了计算机辅助蛋白质结构建模研究以探究CRTAase自乙酰化的影响。因此,预测的CRTAase三维模型显示N结构域和P结构域的所有环区域都带有乙酰化的赖氨酸。对乙酰化残基进行能量最小化显示,由于N - ε - 乙酰化,赖氨酸的电荷中和,这可能有助于CRTAase与蛋白质底物的相互作用以及随后的转乙酰酶作用。

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