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未结合在血红素和铁硫中心的线粒体铁及其在体外血红素合成中的可用性。

Mitochondrial iron not bound in heme and iron-sulfur centers and its availability for heme synthesis in vitro.

作者信息

Tangerås A

出版信息

Biochim Biophys Acta. 1985 Dec 13;843(3):199-207. doi: 10.1016/0304-4165(85)90140-0.

Abstract

Rat liver mitochondrial fractions have previously been shown to contain a pool of iron which was bound neither in cytochromes nor in iron-sulfur centers (Tangerås, A., Flatmark, T., Bãckstrõm, D. and Ehrenberg, A. (1980) Biochim. Biophys. Acta 589, 162-175), and in the present study the availability of this iron pool for heme synthesis has been studied in isolated mitochondria. A minor fraction of this iron is here shown to originate from iron-rich lysosomes present as a contaminant in mitochondrial fractions isolated by differential centrifugation, and a method for the selective quantitation of this iron pool was developed. The availability of the mitochondrial iron pool for heme synthesis by mitochondria in vitro was studied using a recently developed HPLC method for the assay of ferrochelatase activity. When deuteroporphyrin was used as the substrate, 1.04 +/- 0.13 nmol/mg protein of deuteroheme was formed after 6 h incubation at 37 degrees C when a plateau was approached, and the initial rate of heme synthesis was 0.3 nmol/h per mg protein. Heme formation from the physiological substrate protoporphyrin was also seen. The heme synthesis increased with the amount of mitochondria used and was blocked by both Fe(II) and Fe(III) chelators. The heme synthesis was independent of mitochondrial oxidizable substrates and no difference was observed between pH 7.4 and 6.5. FMN slightly stimulated the formation of heme from endogenous iron, probably by mobilization of a small amount of contaminating lysosomal iron present in the preparations. The possibility that the mitochondrial iron pool functions as the proximate iron donor for heme synthesis by ferrochelatase in vivo is discussed.

摘要

先前已表明,大鼠肝脏线粒体组分含有一组铁,该铁既不与细胞色素结合,也不与铁硫中心结合(坦格罗斯,A.,弗拉特马克,T.,巴克斯特伦,D.和埃伦贝格,A.(1980年)《生物化学与生物物理学报》589,162 - 175),在本研究中,已在分离的线粒体中研究了该铁池用于血红素合成的可用性。此处显示,该铁的一小部分源自富含铁的溶酶体,这些溶酶体作为污染物存在于通过差速离心分离的线粒体组分中,并且开发了一种选择性定量该铁池的方法。使用最近开发的用于测定亚铁螯合酶活性的高效液相色谱法,研究了体外线粒体中铁池用于线粒体血红素合成的可用性。当使用氘代卟啉作为底物时,在37℃孵育6小时接近平台期时,形成了1.04±0.13 nmol/mg蛋白质的氘代血红素,血红素合成的初始速率为每毫克蛋白质0.3 nmol/小时。也观察到了由生理底物原卟啉形成血红素的情况。血红素合成随着所用线粒体的量增加而增加,并且被Fe(II)和Fe(III)螯合剂阻断。血红素合成与线粒体可氧化底物无关,在pH 7.4和6.5之间未观察到差异。黄素单核苷酸略微刺激了内源性铁形成血红素,可能是通过动员制剂中存在的少量污染性溶酶体铁。讨论了线粒体铁池在体内作为亚铁螯合酶血红素合成的直接铁供体发挥作用的可能性。

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