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首页> 外文期刊>Acta Biologica Szegediensis >Characterization of an ascorbate-reducible cytochrome b561 by site-directed mutagenesis
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Characterization of an ascorbate-reducible cytochrome b561 by site-directed mutagenesis

机译:通过定点诱变表征抗坏血酸可还原的细胞色素b561

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Ascorbate(ASC)-reducible cytochrome b561 (Cyt-b561) proteins are present in both plants and animals and create a well-distinguished protein family amongst the two-heme containing b-type cytochromes. One isoform of the Cyts-b561 identified by genomic analysis of Arabidopsis thaliana has been localized in the tonoplast. We have expressed the tonoplastlocalized Cyt-b561 (TCyt-b561) in yeast (Saccharomyces serevisiae) cells and shown that the biophysical properties of the recombinant TCyt-b561 is very similar to those of the chromaffin granule Cyt-b561 (CGCyt-b561). Mutation of 4 well-conserved histidine residues (H50, H83, H117, H156) resulted in different expression levels and revealed the importance of these 4 His residues in heme binding and protein expression. Modification of the protein by FLAG-tag or His6-tag resulted in different degrees of reduced expression levels. When all lysine residues (K70, K76, K79, K80, and K159) in the vicinity of the putative ASC-binding motive were one-by-one replaced by alanine, no major changes in the expression levels were observed. Except in case of the K80A mutant, where the low-affinity ASC-binding constant increased significantly, there were no significant changes in either kinetic parameter characterizing the bi-phase ASC-dependent reduction of TCytb-b561. These observations are discussed in comparison to properties of the recombinant CGCyt-b561.
机译:抗坏血酸(ASC)可还原的细胞色素b561(Cyt-b561)蛋白同时存在于动植物中,并在含有两个血红素的b型细胞色素中建立了一个区分良好的蛋白质家族。通过拟南芥的基因组分析鉴定的Cyts-b561的一种同工型已经位于液泡膜中。我们已经在酵母(Saccharomyces serevisiae)细胞中表达了经液泡定位的Cyt-b561(TCyt-b561),并表明重组TCyt-b561的生物物理特性与嗜铬粒Cyt-b561(CGCyt-b561)的生物学特性非常相似。 4个高度保守的组氨酸残基(H50,H83,H117,H156)的突变导致不同的表达水平,并揭示了这4个His残基在血红素结合和蛋白质表达中的重要性。通过FLAG标签或His6标签对蛋白质的修饰导致不同程度的表达水平降低。当假定的ASC结合动机附近的所有赖氨酸残基(K70,K76,K79,K80和K159)被丙氨酸一一取代时,未观察到表达水平的重大变化。除了在K80A突变体中低亲和力ASC结合常数显着增加的情况外,在表征TCytb-b561的双相ASC依赖性还原的任一动力学参数中均无显着变化。与重组CGCyt-b561的性质相比,讨论了这些观察结果。

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