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P13suc1在鱿鱼轴质的多聚体细胞骨架复合体中与一种类cdc2激酶相关联。

P13suc1 associates with a cdc2-like kinase in a multimeric cytoskeletal complex in squid axoplasm.

作者信息

Takahashi M, Amin N, Grant P, Pant H C

机构信息

Laboratory of Neurochemistry, National Institute of Neurological Disorders and Stroke, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

J Neurosci. 1995 Sep;15(9):6222-9. doi: 10.1523/JNEUROSCI.15-09-06222.1995.

Abstract

P13suc1 sepharose-conjugated beads were used to extract the kinases that phosphorylate neurofilaments in the squid giant axon. Using Western blots and in vitro kinase assays, we demonstrated the presence of an active cdc2-like kinase and its putative regulators such as cyclin E, p13, and p67 in axoplasm and a P13-axoplasm complex (P13-Ax). Protein kinase A (PKA) and casein kinase (CK) I and II were also found in the P13-Ax. Western blot analysis of the P13-Ax also demonstrated several axonal cytoskeletal components; e.g., neurofilaments (NFs; NF 60, 70, and 220), tubulin, actin, and microtubule-associated proteins. NF 220 and tubulin were phosphorylated by the kinases in the P13-Ax. To determine whether NFs bound directly to the P13 beads, or bound indirectly by association with cdc2 kinase, a washed, axon-derived neurofilament preparation that contained NFs, PKA, CKl, and tubulin, but no cdc2-like kinase, yielded no bound proteins after incubation with P13suc1. The wash supernatant from the neurofilament preparation, however, containing the cdc2-like kinase, did yield cytoskeletal components that bound to P13suc1. Moreover, a bacterial-expressed cdk5 associated with P13 beads was able to complex with selected cytoskeletal components in the washed neurofilament preparation. These data indicate that direct binding of P13 beads with a cdc2-like kinase could extract active multimeric complexes composed of axonal cytoskeletal proteins and kinases. Application of P13 chromatography may be useful in characterizing the network of functional interactions among cytoskeletal elements and protein kinases in neurons.

摘要

用P13suc1琼脂糖偶联珠来提取鱿鱼巨大轴突中使神经丝磷酸化的激酶。通过蛋白质免疫印迹法和体外激酶分析,我们证实在轴浆和P13 - 轴浆复合物(P13 - Ax)中存在一种活性cdc2样激酶及其假定的调节因子,如细胞周期蛋白E、p13和p67。在P13 - Ax中还发现了蛋白激酶A(PKA)以及酪蛋白激酶(CK)I和II。对P13 - Ax进行的蛋白质免疫印迹分析还显示了几种轴突细胞骨架成分,例如神经丝(NFs;NF 60、70和220)、微管蛋白、肌动蛋白以及微管相关蛋白。NF 220和微管蛋白在P13 - Ax中被激酶磷酸化。为了确定神经丝是直接与P13珠结合,还是通过与cdc2激酶结合而间接结合,一种经过洗涤的、源自轴突的神经丝制剂,其中含有神经丝、PKA、CK1和微管蛋白,但不含cdc2样激酶,在与P13suc1孵育后未产生结合蛋白。然而,来自神经丝制剂的洗涤上清液,其中含有cdc2样激酶,确实产生了与P13suc1结合的细胞骨架成分。此外,与P13珠结合的细菌表达的cdk5能够与洗涤后的神经丝制剂中的选定细胞骨架成分形成复合物。这些数据表明,P13珠与cdc2样激酶的直接结合能够提取由轴突细胞骨架蛋白和激酶组成的活性多聚体复合物。P13色谱法的应用可能有助于表征神经元中细胞骨架成分和蛋白激酶之间的功能相互作用网络。

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