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首页> 外文期刊>Plant Physiology and Biochemistry >Soluble expression of Spinach psbC gene in Escherichia coli and in vitro reconstitution of CP43 coupled with chlorophyll a only
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Soluble expression of Spinach psbC gene in Escherichia coli and in vitro reconstitution of CP43 coupled with chlorophyll a only

机译:菠菜psbC基因在大肠杆菌中的可溶性表达以及CP43和叶绿素a的体外重组

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摘要

CP43 is α chlorophyll α (Chl α) and β-carotene (β-Car) binding protein encoded by psbC gene. In this study, psbC gene isolated from Spinach was expressed in Escherichia coli in soluble state. After lysis of the cells, the apoproteins purified by nickel affinity chromatography were examined by SDS-PAGE and Western-blot. Next, reconstitution experiment was carried out in vitro and the formation of stable pigmenteprotein complex was analyzed by partially denaturing electrophoresis. After purifying reconstituted CP43 (rCP43) from free pigments (FPs) by sucrose gradient ultracentrifugation and subsequently ion exchange chromatography (IEC), the eluate was analyzed by partially denaturing electrophoresis to confirm stability of the reconstructed complex. Finally, analyses of spectroscopic character of the eluate revealed that in vitro reconstitution was achieved and FPs were completely removed from the pigment eprotein complex. Comparison between the absorption spectra of the rCP43 and native CP43 (nCP43) showed the lack of peaks between 450 and 500 nm, illustrating that the β-Car was stripped off rCP43. In brief, it is feasible to obtain a reconstituted protein binding Chl a only, indicating that the occupancy of the β-Car site has small impact on the stabilization of CP43. However, β-Car shows strong interaction with Chl a, inducing the hyperchromic effect in blue region of spectrum and the blue shift of the 438.5 nm and 673.5 nm absorption band to 437 nm and 671 nm respectively. To some extent, our research is suggestive that β-Car, coupled loosely with CP43, contributes to the precise orientation of Chl a in vivo.
机译:CP43是由psbC基因编码的α叶绿素α(Chlα)和β-胡萝卜素(β-Car)结合蛋白。在这项研究中,从菠菜中分离出的psbC基因在大肠杆菌中以可溶状态表达。细胞裂解后,通过SDS-PAGE和Western-blot检查通过镍亲和层析纯化的载脂蛋白。接下来,在体外进行重构实验,并通过部分变性电泳分析稳定的色素蛋白复合物的形成。通过蔗糖梯度超速离心和随后的离子交换色谱(IEC)从游离色素(FPs)纯化重构的CP43(rCP43)后,通过部分变性电泳分析洗脱液,以确认重构复合物的稳定性。最后,对洗脱液的光谱特性进行分析表明,可以实现体外重构,并且从色素e蛋白复合物中完全去除了FP。 rCP43和天然CP43(nCP43)的吸收光谱之间的比较表明,在450和500 nm之间没有峰,说明β-Car被剥离了rCP43。简而言之,仅获得重构的结合Chl a的蛋白质是可行的,这表明β-Car位点的占用对CP43的稳定性影响很小。但是,β-Car与Chla具有强相互作用,在光谱的蓝色区域引起增色效应,吸收谱带的蓝移分别从438.5 nm和673.5 nm分别移至437 nm和671 nm。在某种程度上,我们的研究表明,β-Car与CP43松散结合,有助于Chl a在体内的精确定向。

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