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K562细胞中的铁转运:一项使用天然凝胶电泳和59Fe放射自显影术的动力学研究。

Iron transport in K562 cells: a kinetic study using native gel electrophoresis and 59Fe autoradiography.

作者信息

Vyoral D, Petrák J

机构信息

Institute of Hematology and Blood Transfusion, U nemocnice 1, 128 20, Praha 2, Czech Republic.

出版信息

Biochim Biophys Acta. 1998 Jun 22;1403(2):179-88. doi: 10.1016/s0167-4889(98)00039-1.

Abstract

The exact mechanisms of iron transport from endosomes to the target iron containing cellular proteins are currently unknown. To investigate this problem, we used the gradient gel electrophoresis and the sensitive detection of 59Fe by autoradiography to detect separate cellular iron compounds and their iron kinetics. Cells of human leukemic line K562 were labeled with [59Fe]transferrin for 30-600 s and cellular iron compounds in cell lysates were analyzed by native electrophoretic separation followed by 59Fe autoradiography. Starting with the first 30 s of iron uptake, iron was detectable in a large membrane bound protein complex (Band I) and in ferritin. Significant amounts of iron were also found in labile iron compound(s) with the molecular weight larger than 5000 as judged by ultrafiltration. Iron kinetics in these compartments was studied. Band I was the only compound with the kinetic properties of an intermediate. Transferrin, transferrin receptor and additional proteins of the approximate molecular weights of 130000, 66000 and 49000 were found to be present in Band I. The labile iron compounds and ferritin behaved kinetically as end products. No evidence for low molecular weight transport intermediates was found. These results suggest that intracellular iron transport is highly compartmentalized, that iron released from endosomal transferrin passes to its cellular targets in a direct contact with the endosomal membrane complex assigned as Band I. The nature of the labile iron pool and its susceptibility to iron chelation is discussed.

摘要

目前尚不清楚铁从内体转运至含铁血细胞蛋白的确切机制。为研究此问题,我们使用梯度凝胶电泳和放射自显影对⁵⁹Fe进行灵敏检测,以检测不同的细胞铁化合物及其铁动力学。用人白血病细胞系K562细胞用[⁵⁹Fe]转铁蛋白标记30 - 600秒,通过天然电泳分离细胞裂解物中的细胞铁化合物,随后进行⁵⁹Fe放射自显影分析。从摄取铁的最初30秒开始,在一个大的膜结合蛋白复合物(带I)和铁蛋白中可检测到铁。通过超滤判断,在分子量大于5000的不稳定铁化合物中也发现了大量铁。研究了这些区室中的铁动力学。带I是唯一具有中间体动力学性质的化合物。发现转铁蛋白、转铁蛋白受体以及分子量约为130000、66000和49000的其他蛋白质存在于带I中。不稳定铁化合物和铁蛋白在动力学上表现为终产物。未发现低分子量转运中间体的证据。这些结果表明,细胞内铁转运高度区室化,内体转铁蛋白释放的铁通过与指定为带I的内体膜复合物直接接触传递至其细胞靶点。讨论了不稳定铁池的性质及其对铁螯合的敏感性。

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