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人铁蛋白H链通道和环序列的突变分析

Mutational analysis of the channel and loop sequences of human ferritin H-chain.

作者信息

Levi S, Luzzago A, Franceschinelli F, Santambrogio P, Cesareni G, Arosio P

机构信息

Dipartimento di Scienze e Tecnologie Biomediche, Università di Milano, Ospedale San Raffaele, Italy.

出版信息

Biochem J. 1989 Dec 1;264(2):381-8. doi: 10.1042/bj2640381.

DOI:10.1042/bj2640381
PMID:2690826
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1133592/
Abstract

Human ferritin H-chain mutants were obtained by engineering the recombinant protein expressed by Escherichia coli. The mutagenesis were directed to the C-terminal sequence forming the hydrophobic channel, to the hydrophilic channel and to the loop sequence. The mutants were analysed for extent of expression, for stability, for capacity to incorporate iron and for kinetics of iron uptake and iron oxidation. Of the 22 mutants analysed only two with deletions of single residues in the loop sequence and one with deletion of the last 28 amino acid residues did not assemble into ferritin-like proteins. The other mutants assembled correctly and showed similar chemical/physical properties to the wild-type; they included duplication of an 18-amino acid-residue stretch, deletion of the last 22 and the last seven residues and various mutations of single amino acid residues. Two mutants with extensive alteration in the C-terminal sequence had a diminished thermostability associated with incapability to incorporate iron though they still catalysed iron oxidation. The mutants with alterations of the sequence around the hydrophilic channel showed diminished iron uptake and oxidation kinetics, together with a slightly larger apparent molecular size. The results indicate (i) that two of the sequences are important for ferritin assembly/stability, (ii) that the presence of the hydrophobic channel is essential for formation of the iron core and (iii) that the sites of iron interaction and the path of iron penetration into ferritin remain unidentified.

摘要

人铁蛋白H链突变体是通过对大肠杆菌表达的重组蛋白进行工程改造获得的。诱变针对形成疏水通道的C末端序列、亲水通道和环序列。对突变体进行了表达程度、稳定性、铁掺入能力以及铁摄取和铁氧化动力学的分析。在分析的22个突变体中,只有两个环序列中单个残基缺失的突变体和一个最后28个氨基酸残基缺失的突变体没有组装成铁蛋白样蛋白。其他突变体正确组装,并表现出与野生型相似的化学/物理性质;它们包括18个氨基酸残基片段的重复、最后22个和最后7个残基的缺失以及单个氨基酸残基的各种突变。两个C末端序列发生广泛改变的突变体热稳定性降低,且无法掺入铁,尽管它们仍能催化铁氧化。亲水通道周围序列发生改变的突变体铁摄取和氧化动力学降低,同时表观分子大小略大。结果表明:(i)其中两个序列对铁蛋白组装/稳定性很重要;(ii)疏水通道的存在对铁核心的形成至关重要;(iii)铁与铁蛋白相互作用的位点以及铁进入铁蛋白的途径仍未确定。

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本文引用的文献

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Amino acid sequence of horse spleen apoferritin.马脾脱铁铁蛋白的氨基酸序列。
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铁蛋白纳米笼作为高效的纳米载体,为 COVID-19 和其他疫苗的开发提供了有前途的平台。
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Mutant L-chain ferritins that cause neuroferritinopathy alter ferritin functionality and iron permeability.突变的 L 链铁蛋白导致神经铁蛋白病,改变了铁蛋白的功能和铁的通透性。
Metallomics. 2019 Oct 16;11(10):1635-1647. doi: 10.1039/c9mt00154a.
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Engineering intracellular biomineralization and biosensing by a magnetic protein.利用磁性蛋白构建细胞内生物矿化与生物传感
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The C-terminal regions have an important role in the activity of the ferroxidase center and the stability of Chlorobium tepidum ferritin.C 末端区域在铁氧化酶中心的活性和 Chlorobium tepidum 铁蛋白的稳定性中具有重要作用。
Protein J. 2014 Jun;33(3):211-20. doi: 10.1007/s10930-014-9552-3.
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Coordinating subdomains of ferritin protein cages with catalysis and biomineralization viewed from the C4 cage axes.从 C4 笼轴的角度看与催化和生物矿化作用相协调的铁蛋白蛋白笼亚结构域。
J Biol Inorg Chem. 2014 Jun;19(4-5):615-22. doi: 10.1007/s00775-014-1103-z. Epub 2014 Feb 7.
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Human L-ferritin deficiency is characterized by idiopathic generalized seizures and atypical restless leg syndrome.人 L 铁蛋白缺乏症的特征是特发性全身性癫痫和非典型不宁腿综合征。
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Ferritin ion channel disorder inhibits Fe(II)/O2 reactivity at distant sites.铁蛋白离子通道紊乱抑制远距离位点的 Fe(II)/O2 反应性。
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Self-assembly in the ferritin nano-cage protein superfamily.铁蛋白纳米笼蛋白超家族中的自组装
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