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钙网蛋白在大肠杆菌中的表达及其钙离子结合结构域的鉴定。

Expression of calreticulin in Escherichia coli and identification of its Ca2+ binding domains.

作者信息

Baksh S, Michalak M

机构信息

Cardiovascular Disease Research Group, University of Alberta, Edmonton, Canada.

出版信息

J Biol Chem. 1991 Nov 15;266(32):21458-65.

PMID:1939178
Abstract

Recombinant calreticulin and discrete domains of calreticulin were expressed in Escherichia coli, using the glutathione S-transferase fusion protein system, and their Ca2+ binding properties were determined. Native calreticulin bound 1 mol of Ca2+/mol of protein with high affinity, and also bound approximately 20 mol of Ca2+/mol of protein with low affinity. Both Ca2+ binding sites were present in the recombinant calreticulin indicating that proper folding of the protein was achieved using this system. Calreticulin is structurally divided into three distinct domains: the N-domain encompassing the first 200 residues; the P-domain which is enriched in proline residues (residue 187-317); and the C-domain which covers the carboxyl-terminal quarter of the protein (residues 310-401), and contains a high concentration of acidic residues. These domains were expressed in E. coli, isolated, and purified, and their Ca2+ binding properties were analyzed. The C-domain bound approximately 18 mol of Ca2+/mol of protein with a dissociation constant of approximately 2 mM. The P-domain bound approximately 0.6-1 mol of Ca2+/mol of protein with a dissociation constant of approximately 10 microM. The P-domain and the C-domain, when expressed together as the P+C-domain, bound Ca2+ with both high affinity and low affinity, reminiscent of both full length recombinant calreticulin and native calreticulin. In contrast the N-domain, did not bind any detectable amount of 45Ca2+. We conclude that calreticulin has two quite distinct types of Ca2+ binding sites, and that these sites are in different structural regions of the molecule. The P-domain binds Ca2+ with high affinity and low capacity, whereas the C-domain binds Ca2+ with low affinity and high capacity.

摘要

利用谷胱甘肽S-转移酶融合蛋白系统在大肠杆菌中表达重组钙网蛋白及其不同结构域,并测定其Ca2+结合特性。天然钙网蛋白以高亲和力结合1 mol Ca2+/mol蛋白,还以低亲和力结合约20 mol Ca2+/mol蛋白。两个Ca2+结合位点均存在于重组钙网蛋白中,表明使用该系统可实现蛋白的正确折叠。钙网蛋白在结构上分为三个不同的结构域:包含前200个残基的N结构域;富含脯氨酸残基(第187 - 317位残基)的P结构域;以及覆盖蛋白羧基末端四分之一(第310 - 401位残基)且含有高浓度酸性残基的C结构域。这些结构域在大肠杆菌中表达、分离和纯化,并分析其Ca2+结合特性。C结构域以约2 mM的解离常数结合约18 mol Ca2+/mol蛋白。P结构域以约10 μM的解离常数结合约0.6 - 1 mol Ca2+/mol蛋白。P结构域和C结构域一起作为P + C结构域表达时,以高亲和力和低亲和力结合Ca2+,这类似于全长重组钙网蛋白和天然钙网蛋白。相比之下,N结构域未结合任何可检测量的45Ca2+。我们得出结论,钙网蛋白有两种截然不同的Ca2+结合位点,且这些位点位于分子的不同结构区域。P结构域以高亲和力和低容量结合Ca2+,而C结构域以低亲和力和高容量结合Ca2+。

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