Walzel Bernd, Speer Oliver, Boehm Ernie, Kristiansen Søren, Chan Sharon, Clarke Kierian, Magyar Joseph P, Richter Erik A, Wallimann Theo
Institute of Cell Biology, Eidgenössische Technische Hochschule-Zurich, Hönggerberg, CH-8093 Zurich, Switzerland.
Am J Physiol Endocrinol Metab. 2002 Aug;283(2):E390-401. doi: 10.1152/ajpendo.00428.2001.
Despite the pivotal role of creatine (Cr) and phosphocreatine (PCr) in muscle metabolism, relatively little is known about sarcolemmal creatine transport, creatine transporter (CRT) isoforms, and subcellular localization of the CRT proteins. To be able to quantify creatine transport across the sarcolemma, we have developed a new in vitro assay using rat sarcolemmal giant vesicles. The rat giant sarcolemmal vesicle assay reveals the presence of a specific high-affinity and saturable transport system for Cr in the sarcolemma (Michaelis-Menten constant 52.4 +/- 9.4 microM and maximal velocity value 17.3 +/- 3.1 pmol x min(-1) x mg vesicle protein(-1)), which cotransports Cr into skeletal muscle together with Na(+) and Cl(-) ions. The regulation of Cr transport in giant vesicles by substrates, analogs, and inhibitors, as well as by phorbol 12-myristate 13-acetate and insulin, was studied. Two antibodies raised against COOH- and NH(2)-terminal synthetic peptides of CRT sequences both recognize two major polypeptides on Western blots with apparent molecular masses of 70 and 55 kDa, respectively. The highest CRT expression occurs in heart, brain, and kidney, and although creatine kinase is absent in liver cells, CRT is also found in this tissue. Surprisingly, immunofluorescence staining of cultured adult rat heart cardiomyocytes with specific anti-CRT antibodies, as well as cell fractionation and cell surface biotinylation studies, revealed that only a minor CRT species with an intermediate molecular mass of approximately 58 kDa is present in the sarcolemma, whereas the previously identified major CRT-related protein species of 70 and 55 kDa are specifically located in mitochondria. Our studies indicate that mitochondria may represent a major compartment of CRT localization, thus providing a new aspect to the current debate about the existence and whereabouts of intracellular Cr and PCr compartments that have been inferred from [(14)C]PCr/Cr measurements in vivo as well as from recent in vivo NMR studies.
尽管肌酸(Cr)和磷酸肌酸(PCr)在肌肉代谢中起着关键作用,但对于肌膜肌酸转运、肌酸转运体(CRT)亚型以及CRT蛋白的亚细胞定位,我们所知甚少。为了能够量化肌酸跨肌膜的转运,我们开发了一种使用大鼠肌膜巨型囊泡的新体外测定法。大鼠巨型肌膜囊泡测定法揭示了肌膜中存在一种针对Cr的特异性高亲和力和可饱和转运系统(米氏常数为52.4±9.4μM,最大速度值为17.3±3.1 pmol·min⁻¹·mg囊泡蛋白⁻¹),该系统将Cr与Na⁺和Cl⁻离子共转运到骨骼肌中。研究了底物、类似物、抑制剂以及佛波醇12 - 肉豆蔻酸酯13 - 乙酸酯和胰岛素对巨型囊泡中Cr转运的调节作用。针对CRT序列的COOH末端和NH₂末端合成肽产生的两种抗体,在蛋白质印迹上均识别出两条主要多肽,其表观分子量分别为70 kDa和55 kDa。CRT表达最高的部位是心脏、大脑和肾脏,尽管肝细胞中不存在肌酸激酶,但在该组织中也发现了CRT。令人惊讶的是,用特异性抗CRT抗体对培养的成年大鼠心脏心肌细胞进行免疫荧光染色,以及细胞分级分离和细胞表面生物素化研究表明,肌膜中仅存在一种分子量约为58 kDa的中等分子量的次要CRT物种,而先前鉴定的分子量为70 kDa和55 kDa的主要CRT相关蛋白物种则特异性地位于线粒体中。我们的研究表明,线粒体可能是CRT定位的主要区域,从而为当前关于细胞内Cr和PCr区域的存在及位置的争论提供了一个新的方面,这些区域已通过体内[(14)C]PCr/Cr测量以及最近的体内核磁共振研究推断得出。
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