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来自念珠藻PCC7120的类CpcS和类CpcT蛋白的裂合酶活性以及藻红青素和藻蓝蛋白β亚基结合位点的顺序重建

Lyase activities of CpcS- and CpcT-like proteins from Nostoc PCC7120 and sequential reconstitution of binding sites of phycoerythrocyanin and phycocyanin beta-subunits.

作者信息

Zhao Kai-Hong, Zhang Juan, Tu Jun-Ming, Böhm Stephan, Plöscher Matthias, Eichacker Lutz, Bubenzer Claudia, Scheer Hugo, Wang Xing, Zhou Ming

机构信息

College of Life Science and Technology, Huazhong University of Science and Technology, Wuhan, Hubei, China.

出版信息

J Biol Chem. 2007 Nov 23;282(47):34093-103. doi: 10.1074/jbc.M703038200. Epub 2007 Sep 25.

DOI:10.1074/jbc.M703038200
PMID:17895251
Abstract

Genes all5292 (cpcS2) and alr0617 (cpcS1) in the cyanobacterium Nostoc PCC7120 are homologous to the biliprotein lyase cpcS, and genes all5339 (cpcT1) and alr0647 (cpcT2) are homologous to the lyase cpcT. The functions of the encoded proteins were screened in vitro and in a heterologous Escherichia coli system with plasmids conferring biosynthesis of the phycocyanobilin chromophore and of the acceptor proteins beta-phycoerythrocyanin (PecB) or beta-phycocyanin (CpcB). CpcT1 is a regioselective biliprotein lyase attaching phycocyanobilin exclusively to cysteine beta155 but does not discriminate between CpcB and PecB. The in vitro reconstitutions required no cofactors, and kinetic constants were determined for CpcT1 under in vitro conditions. No lyase activity was found for the lyase homologues CpcS2 and CpcT2, but complexes are formed in vitro between CpcT1 and CpcS1, CpcT2, or PecE (subunit of phycoviolobilin:alpha-phycoerythrocyanin isomerase lyase). The genes coding the inactive homologues, cpcS2 and cpcT2, are transcribed in N-starved Nostoc. In sequential binding experiments with CpcT1 and CpcS1, a chromophore at cysteine 84 inhibited the subsequent attachment to cysteine 155, whereas the inverse sequence generates subunits carrying both chromophores.

摘要

蓝藻念珠藻Nostoc PCC7120中的基因all5292(cpcS2)和alr0617(cpcS1)与胆色素蛋白裂合酶cpcS同源,基因all5339(cpcT1)和alr0647(cpcT2)与裂合酶cpcT同源。通过体外实验以及在异源大肠杆菌系统中,利用携带藻蓝胆素发色团和受体蛋白β-藻红青蛋白(PecB)或β-藻蓝蛋白(CpcB)生物合成质粒的方法,对编码蛋白的功能进行了筛选。CpcT1是一种区域选择性胆色素蛋白裂合酶,仅将藻蓝胆素连接到半胱氨酸β155上,且对CpcB和PecB没有区分作用。体外重组不需要辅因子,并在体外条件下测定了CpcT1的动力学常数。未发现裂合酶同源物CpcS2和CpcT2具有裂合酶活性,但在体外CpcT1与CpcS1、CpcT2或PecE(藻紫胆素:α-藻红青蛋白异构酶裂合酶的亚基)之间形成了复合物。编码无活性同源物cpcS2和cpcT2的基因在氮饥饿的念珠藻中进行转录。在CpcT1和CpcS1的顺序结合实验中,半胱氨酸84处的发色团会抑制随后与半胱氨酸155的连接,而相反的顺序则会产生携带两种发色团的亚基。

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