首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Molecular cloning and characterization of the ryanodine receptor/junctional channel complex cDNA from skeletal muscle sarcoplasmic reticulum.
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Molecular cloning and characterization of the ryanodine receptor/junctional channel complex cDNA from skeletal muscle sarcoplasmic reticulum.

机译:骨骼肌肌浆网中ryanodine受体/连接通道复合物cDNA的分子克隆和表征。

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摘要

Major progress has been made in elucidating the calcium release mechanism involved in excitation-contraction coupling. The ryanodine receptor of sarcoplasmic reticulum has been isolated and found to be morphologically identical to the foot structure, which is involved in the junctional association of terminal cisternae with the transverse tubule. The foot structure also contains the calcium release channel itself. For this reason, we refer to the foot structure as the junctional channel complex (JCC). The JCC consists of an oligomer of a single high molecular weight protein. Although progress has been made in characterizing important aspects of the structure and function of the JCC, further understanding of the JCC protein subunit awaits the molecular cloning of the JCC. We report on the isolation of cDNA clones encoding portions of the JCC from rabbit fast-twitch skeletal muscle and its tissue distribution and expression. The large size and lack of solubility of the JCC protein posed particular challenges to cloning this molecule. Among these was the necessity to develop techniques for partially digesting the JCC protein subunit with endoproteases in the presence of detergent. With this approach we obtained partial amino acid sequences from regions of the JCC and designed oligonucleotide primers and probes to synthesize and screen cDNA libraries. The rabbit skeletal muscle JCC mRNA encodes an approximately 16-kilobase mRNA present in skeletal, heart, and aortic smooth muscle, as determined by RNA blot analysis with a 700-base-pair cDNA probe. Whereas the JCC mRNA appears to be relatively abundant in adult rabbit fast-twitch skeletal muscle, it is much less abundant in heart and smooth muscle. The JCC mRNA in BC3H1 (a myoblast cell line) is reversibly regulated by growth factors in a manner similar to muscle-specific contractile protein genes.
机译:在阐明涉及激发-收缩偶联的钙释放机制方面已取得重大进展。肌浆网的莱丹胺受体已被分离出来,并在形态上与足部结构相同,该结构参与了末端水箱与横管的连接。足部结构还包含钙释放通道本身。因此,我们将脚部结构称为接合通道复合体(JCC)。 JCC由单个高分子量蛋白质的寡聚物组成。尽管在表征JCC的结构和功能的重要方面已经取得了进展,但对JCC蛋白亚基的进一步了解有待JCC的分子克隆。我们报告了从兔快速抽搐骨骼肌中分离出编码JCC部分的cDNA克隆及其组织分布和表达。 JCC蛋白的大尺寸和缺乏溶解性给克隆该分子带来了特殊的挑战。其中有必要开发在去污剂存在下用内切蛋白酶部分消化JCC蛋白亚基的技术。通过这种方法,我们从JCC区域获得了部分氨基酸序列,并设计了寡核苷酸引物和探针以合成和筛选cDNA文库。兔骨骼肌JCC mRNA编码存在于骨骼,心脏和主动脉平滑肌中的约16碱基碱基的mRNA,这是通过使用700个碱基对cDNA探针进行RNA印迹分析确定的。 JCC mRNA在成年兔快速抽搐骨骼肌中似乎相对丰富,而在心脏和平滑肌中则少得多。 BC3H1(成肌细胞细胞系)中的JCC mRNA由生长因子可逆地调节,其作用方式类似于肌肉特异性收缩蛋白基因。

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