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Synthesis of haem cytochrome c prosthetic group from δ-aminolaevulinate by the cell sap from rat liver

机译:大鼠肝脏细胞液由δ-氨基戊酸酯合成血红素细胞色素c假体

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摘要

To determine whether the prosthetic group of cytochrome c is synthesized and linked to the apoprotein in the cytosol or in connexion with the endoplasmic reticulum, we have studied the incorporation in vitro of δ-amino[14C]laevulinate into porphyrin compounds and cytochrome c by the cell sap from rat liver. The radioactive precursor was incorporated into a trichloroacetic acid-precipitable form partially resistant to extractions by acid solvents, suggesting the existence of a fraction covalently linked to protein. The activity was proportional to the amount of protein incubated, did not increase substantially by supplementation with the microsomal fraction and an energy source, and was very low in the pH5 fraction. Addition of increasing amounts of haemin inhibited the incorporation, as with purified δ-aminolaevulinate dehydratase. [14C]Protoporphyrin IX was identified by paper chromatography, together with a shoulder running as protohaem IX. The cell sap in the absence of ribosomes was also able to incorporate radioactivity into purified cytochrome c, and the addition of ribosomes significantly enhanced the activity. The precursors of haem c were synthesized in the soluble system by the known haem-synthetic pathway, as shown by the kinetics of labelling of the coproporphyrin, protoporphyrin and haem fractions, and the activities were concentrated in the precipitate obtained between 40 and 60% saturation with (NH4)2SO4. The presence of ferrochelatase was indicated by the incorporation of 55Fe into proto- and haemato-haem identified by paper chromatography. It is concluded that the cell sap from rat liver contains the complete set of enzymes for the synthesis from δ-aminolaevulinate of haem c and its linkage to a small pool of free apoprotein c present in soluble form. This suggests that an ancillary pathway of haem synthesis occurs in the cytosol for at least the formation of the prosthetic group, which is linked post-translationally to that pool of apoprotein c synthesized by free polyribosomes.
机译:为了确定是否合成了细胞色素c的修复基团并与胞浆中的载脂蛋白连接或与内质网连接,我们研究了δ-氨基[ 14 C]乳清蛋白的体外结合通过大鼠肝脏中的细胞液转化为卟啉化合物和细胞色素c将放射性前体掺入部分可抵抗酸性溶剂萃取的三氯乙酸可沉淀形式,这表明存在与蛋白质共价连接的馏分。活性与温育的蛋白质量成比例,通过添加微粒体级分和能量来源基本上没有增加,并且pH5级分非常低。与纯化的δ-氨基戊酸甘油酯脱水酶一样,添加增加量的血红素可抑制掺入。通过纸色谱法鉴定了[ 14 C]原卟啉IX,并肩部运行了原血红蛋白IX。在不存在核糖体的情况下,细胞液液也能够将放射性结合到纯化的细胞色素c中,并且添加核糖体显着增强了活性。血红素c的前体通过已知的血红素合成途径在可溶性系统中合成,如共卟啉,原卟啉和血红素级分的标记动力学所示,其活性集中在饱和度为40%至60%的沉淀中(NH4)2SO4。通过纸层析法鉴定的 55 Fe掺入原血和血红细胞中,表明了铁螯合酶的存在。结论是,来自大鼠肝脏的细胞液含有完整的酶,用于由血红素c的δ-氨基乳油酸酯合成,以及与少量可溶形式的游离载脂蛋白c的连接。这表明血红素合成的辅助途径至少在修复基团的形成中出现在胞质溶胶中,该基团在翻译后与游离多核糖体合成的载脂蛋白c池连接。

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