海兔肌红蛋白cDNA克隆:通过活性位点诱变研究的氧稳定化替代机制
Aplysia limacina myoglobin cDNA cloning: an alternative mechanism of oxygen stabilization as studied by active-site mutagenesis.
作者信息
Cutruzzolà F, Travaglini Allocatelli C, Brancaccio A, Brunori M
机构信息
Istituto Pasteur-Fondazione Cenci Bolognetti, Università di Roma 'La Sapienza', Italia.
出版信息
Biochem J. 1996 Feb 15;314 ( Pt 1)(Pt 1):83-90. doi: 10.1042/bj3140083.
The isolation and cloning of the cDNA coding for myoglobin (Mb) from the mollusc Aplysia limacina is reported here. Five amino acid differences from the previously published protein sequence have been found in positions 22, 26, 27, 77 and 80 by back transplanting the cDNA; some of these may be relevant for overall structure stabilization in this Mb. High-level expression of the holoprotein in Escherichia coli has been achieved in the presence of the haem precursor delta-aminolevulinic acid, underlying the importance of tuning haem and apoprotein biosynthesis to achieve high-level expression of haemproteins in bacteria. The recombinant protein is identical to the protein purified from the mollusc buccal muscle. Native A. limacina Mb has an oxygen dissociation rate constant of 70 s(-1) [as compared with the value of 15 s(-1) for sperm whale Mb, which displays His(E7) and Thr(E10)] (amino acid positions are referred to within the eight helices A-H of the globin fold). In order to understand the mechanism of oxygen stabilization in A. limacina Mb, we have prepared and investigated three active-site mutants: two single mutants in which Val(E7) and Arg(E10) have been replaced by His and Thr, respectively, and a double mutant carrying both mutations. When Arg(E10) is substituted with Thr, the oxygen dissociation rate constant is increased from 70 s(-1) to more than 700 s(-1), in complete agreement with the previously proposed role of the former residue in ligand stabilization. In the His(E7)-containing single and double mutants, both displaying high oxygen dissociation rates, the stabilization of bound oxygen by the distal His is insufficient to slow down the ligand dissociation rate constant to the value of sperm whale Mb. These results essentially prove the hypothesis that in A. limacina Mb a mechanism of oxygen stabilization involving Arg(E10), and thus different from that mediated by His(E7), has evolved.
本文报道了从海兔(Aplysia limacina)中分离和克隆编码肌红蛋白(Mb)的cDNA。通过回移cDNA发现在第22、26、27、77和80位与先前发表的蛋白质序列存在五个氨基酸差异;其中一些差异可能与该肌红蛋白的整体结构稳定性有关。在血红素前体δ-氨基乙酰丙酸存在的情况下,已在大肠杆菌中实现了全蛋白的高水平表达,这表明调节血红素和脱辅基蛋白的生物合成对于在细菌中实现血红素蛋白的高水平表达很重要。重组蛋白与从海兔颊肌中纯化的蛋白相同。天然海兔肌红蛋白的氧解离速率常数为70 s⁻¹[相比之下,抹香鲸肌红蛋白的值为15 s⁻¹,其具有His(E7)和Thr(E10)](氨基酸位置是指球蛋白折叠的八个螺旋A - H内)。为了了解海兔肌红蛋白中氧稳定的机制,我们制备并研究了三个活性位点突变体:两个单突变体,其中Val(E7)和Arg(E10)分别被His和Thr取代,以及一个携带这两个突变的双突变体。当Arg(E10)被Thr取代时,氧解离速率常数从70 s⁻¹增加到超过700 s⁻¹,这与先前提出的前一个残基在配体稳定中的作用完全一致。在含有His(E7)的单突变体和双突变体中,两者都表现出高氧解离速率,远端His对结合氧的稳定作用不足以将配体解离速率常数减慢到抹香鲸肌红蛋白的值。这些结果基本上证明了这样一个假设,即在海兔肌红蛋白中,一种涉及Arg(E10)的氧稳定机制已经进化,因此不同于由His(E7)介导的机制。
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