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突变的重组人重链铁蛋白与体内外骨髓抑制:铁蛋白铁氧化酶活性与生物学功能之间的联系。

Mutated recombinant human heavy-chain ferritins and myelosuppression in vitro and in vivo: a link between ferritin ferroxidase activity and biological function.

作者信息

Broxmeyer H E, Cooper S, Levi S, Arosio P

机构信息

Department of Medicine, Hematology/Oncology, Indiana University School of Medicine, Indianapolis 46202.

出版信息

Proc Natl Acad Sci U S A. 1991 Feb 1;88(3):770-4. doi: 10.1073/pnas.88.3.770.

Abstract

Human heavy-chain (H-) ferritin muteins obtained by oligonucleotide site-directed mutagenesis, together with wild-type recombinant human H- and light-chain (L-) ferritins, were evaluated for in vitro effects on the suppression of human bone marrow myeloid progenitor cells and for in vivo effects on marrow and splenic myelopoiesis in C3H/HeJ mice. The 10 H-ferritin muteins exhibited alterations of various regions of the molecule, including ones exposed on the outer surface, on the inner cavity, and on the hydrophilic and hydrophobic channels and of the four-alpha-helix bundle forming the subunit structure. They were stable and were electrophoretically analogous to wild-type H-ferritin. The muteins showed in vitro and in vivo myelosuppressive activity analogous to wild type, except for mutein 222, which was totally inactive and which lacked ferroxidase activity. Recombinant human L-ferritin, devoid of ferroxidase activity, was also inactive as a suppressor. The results demonstrate that H-ferritin myelosuppressive and ferroxidase activities are linked. One possibility is that ferroxidase activity may interfere with the cellular uptake of transferrin iron that is needed for cell proliferation, an interpretation consistent with the presently described ability of hemin to overcome H-ferritin suppressive effects.

摘要

通过寡核苷酸定点诱变获得的人重链(H-)铁蛋白突变体,与野生型重组人H-和轻链(L-)铁蛋白一起,评估其对人骨髓髓系祖细胞抑制的体外作用以及对C3H/HeJ小鼠骨髓和脾脏髓系造血的体内作用。这10种H-铁蛋白突变体在分子的各个区域表现出改变,包括暴露于外表面、内腔、亲水和疏水通道的区域以及形成亚基结构的四螺旋束区域。它们很稳定,电泳性质与野生型H-铁蛋白相似。除了完全无活性且缺乏铁氧化酶活性的突变体222外,这些突变体在体外和体内均表现出与野生型类似的骨髓抑制活性。缺乏铁氧化酶活性的重组人L-铁蛋白作为抑制剂也无活性。结果表明,H-铁蛋白的骨髓抑制活性和铁氧化酶活性相关。一种可能性是,铁氧化酶活性可能会干扰细胞增殖所需的转铁蛋白铁的细胞摄取,这一解释与目前所描述的血红素克服H-铁蛋白抑制作用的能力一致。

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