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>Disulphide cross-linking of smooth-muscle and non-muscle caldesmon to the C-terminus of actin in reconstituted and native thin filaments
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Disulphide cross-linking of smooth-muscle and non-muscle caldesmon to the C-terminus of actin in reconstituted and native thin filaments
pIt was reported that chicken gizzard smooth-muscle caldesmon Cys-580 can be disulphide-cross-linked to the C-terminal pen-ultimate residue (Cys-374) of actin, indicating that these residues are close in the protein complex [Graceffa, P. and Jancso, A. (1991) J. Biol. Chem. 266, 20305-20310]. Since the possibility that the cross-link involves a cysteine residue other than actin Cys-374 was not absolutely excluded, more direct evidence was sought for the identify of the cysteine residues involved in the cross-link. We show here that caldesmon could not be disulphide-cross-linked to actin which had Cys-374 removed by carboxypeptidase A digestion, providing direct support for the participation of actin Cys-374 in the cross-link to caldesmon. In order to assign the caldesmon cysteine residue involved in the cross-link, use was made of caldesmon from porcine stomach muscle, which is shown to contain one cysteine residue close to, or at, position 580, in contrast with chicken gizzard caldesmon, which has an additional cysteine residue at position 153. The porcine stomach caldesmon also formed a disulphide-cross-link to actin, further supporting the original conclusion that Cys-580 of the chicken gizzard caldesmon had been cross-linked to actin. Disulphide-cross-linking with similar yield was also observed in native chicken gizzard muscle thin filaments, indicating that the interaction between actin and the C-terminal domain of caldesmon is the same in native and reconstituted thin filaments. The much smaller non-muscle isoform of caldesmon, from rabbit liver, could be similarly cross-linked to actin, consistent with the sequence similarity between the C-terminal domain of muscle and non-muscle caldesmon. The ability to cross-link caldesmon Cys-580 to actin Cys-374 suggests the possibility that the Cys-580 region of caldesmon and the C-terminus of actin form part of the actin-caldesmon binding interface./p
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机译:>据报道,鸡g平滑肌卡尔德斯蒙Cys-580可以与肌动蛋白的C端五末端最终残基(Cys-374)二硫键交联,表明这些残基在蛋白复合物中是紧密的[Graceffa,P. and Jancso,A.(1991)J. Biol。化学266,20305-20310]。由于没有绝对排除交联涉及除肌动蛋白Cys-374以外的半胱氨酸残基的可能性,因此寻求更直接的证据来鉴定参与交联的半胱氨酸残基。我们在这里显示卡尔德斯蒙不能被二硫键交联到通过羧肽酶A消化去除了Cys-374的肌动蛋白上,为肌动蛋白Cys-374参与与卡尔德斯蒙的交联提供了直接支持。为了指定参与交联的卡尔德斯蒙半胱氨酸残基,使用了来自猪胃肌的卡尔德斯蒙,与鸡g卡尔德蒙相比,该半胱氨酸残基显示出一个接近或位于580位的半胱氨酸残基。在153位具有一个额外的半胱氨酸残基。猪胃Caldesmon还与肌动蛋白形成了二硫键交联,进一步支持了鸡izz Caldesmon的Cys-580已与肌动蛋白交联的最初结论。在天然鸡g肌细丝中也观察到了二硫化物交联,收率相近,这表明肌动蛋白与卡尔德蒙C末端结构域之间的相互作用在天然和重组细丝中是相同的。来自兔子肝脏的卡尔德斯蒙的小得多的非肌肉同种型可以相似地交联到肌动蛋白上,这与肌肉和非肌肉卡尔德斯蒙的C端结构域之间的序列相似性一致。能够使Caldesmon Cys-580与肌动蛋白Cys-374交联,这表明Caldesmon的Cys-580区和肌动蛋白的C端形成肌动蛋白与Caldesmon结合界面的一部分的可能性。
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