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纯化的钙网蛋白的蛋白质酰基转移酶功能:P 结构域在利用酰氧基香豆素和乙酰辅酶 A 作为酰基供体介导蛋白质酰化中的独特作用。

Protein acyltransferase function of purified calreticulin: the exclusive role of P-domain in mediating protein acylation utilizing acyloxycoumarins and acetyl CoA as the acyl group donors.

作者信息

Singh Prabhjot, Ponnan Prija, Priya Nivedita, Tyagi Tapesh K, Gaspari Marco, Krishnan Shibu, Cuda Giovanni, Joshi Paritosh, Gambhir Jasvinder K, Sharma Sunil K, Prasad Ashok K, Saso Luciano, Rastogi Ramesh C, Parmar Virinder S, Raj Hanumantharao G

机构信息

Department of Biochemistry, VP Chest Institute, University of Delhi, Delhi, India.

出版信息

Protein Pept Lett. 2011 May;18(5):507-17. doi: 10.2174/092986611794927938.

DOI:10.2174/092986611794927938
PMID:21235489
Abstract

The distinct biochemical function of endoplasmic reticulum (ER) protein Calreticulin (CR) catalyzing the transfer of acyl group from acyloxycoumarin to a receptor protein was termed calreticulin transacylase (CRTAase). The present study, unlike the previous reports of others utilizing CR-deficient cells alone, dealt with the recombinant CR domains of Heamonchus contortus (rhCRTAase) in order to examine their CRTAase activity. P-domain of rhCR unlike N- and C-domains was found to be endowed with CRTAase function. We have also observed for the first time acetyl CoA, as a substrate for rhCRTAase/P-domain mediated acetylation of recombinant Schistosoma japonicum glutathione S-transferase (rGST). rhCRTAase/P-domain were also found to undergo autoacylation by acyloxycoumarins. Also, the isolated autoacylated rhCRTAase/P-domain in non-denatured form alone exhibited the ability to transfer acyl group to rGST indicating the stable intermediate nature of acylated CR. P-domain catalyzed acetylation of rGST by 7,8-Diacetoxy-4-methylcoumarin or acetyl CoA resulted in the modification of several lysine residues in common was evidenced by LC-MS/MS analysis. The putative site of the binding of acyloxycoumarins with CR was predicted by computational blind docking studies. The results showed the involvement of two lysine residues Lys-173 and Lys-174 present in P-domain for binding acyloxycoumarins and acetyl CoA thus highlighting that the active site for the CRTAase activity would reside in the P-domain of CR. Certain ER proteins are known to undergo acetylation under the physiological conditions involving acetyl CoA. These results demonstrating CRTAase mediated protein acetylation by acetyl CoA may hint at CR as the possible protein acetyltransferase of the ER lumen.

摘要

内质网(ER)蛋白钙网蛋白(CR)催化酰基从酰氧基香豆素转移至受体蛋白的独特生化功能被称为钙网蛋白转酰基酶(CRTAase)。与其他仅利用CR缺陷细胞的先前报道不同,本研究针对捻转血矛线虫的重组CR结构域(rhCRTAase)展开研究,以检测其CRTAase活性。结果发现,rhCR的P结构域与N结构域和C结构域不同,具有CRTAase功能。我们还首次观察到乙酰辅酶A可作为rhCRTAase/P结构域介导的重组日本血吸虫谷胱甘肽S-转移酶(rGST)乙酰化的底物。rhCRTAase/P结构域也被发现可被酰氧基香豆素自身酰化。此外,单独以非变性形式分离得到的自身酰化rhCRTAase/P结构域表现出将酰基转移至rGST的能力,这表明酰化CR具有稳定的中间性质。P结构域催化7,8-二乙酰氧基-4-甲基香豆素或乙酰辅酶A对rGST的乙酰化,液相色谱-串联质谱(LC-MS/MS)分析证实,这导致多个赖氨酸残基发生了常见的修饰。通过计算盲对接研究预测了酰氧基香豆素与CR的结合位点。结果表明,P结构域中的两个赖氨酸残基Lys-173和Lys-174参与了酰氧基香豆素和乙酰辅酶A的结合,从而突出表明CRTAase活性的活性位点位于CR的P结构域中。已知某些内质网蛋白在涉及乙酰辅酶A的生理条件下会发生乙酰化。这些结果表明CRTAase介导乙酰辅酶A对蛋白的乙酰化,这可能暗示CR是内质网腔中可能的蛋白乙酰转移酶。

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