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轴突切断后,由轴突运输的肌动蛋白和微管蛋白组装成微丝和微管。

Assembly of microfilaments and microtubules from axonally transported actin and tubulin after axotomy.

作者信息

Jacob J M, McQuarrie I G

机构信息

Neural Regeneration Center, Cleveland Veterans Affairs Medical Center, Ohio 44106, USA.

出版信息

J Neurosci Res. 1996 Feb 15;43(4):412-9. doi: 10.1002/(SICI)1097-4547(19960215)43:4<412::AID-JNR3>3.0.CO;2-I.

Abstract

The slow component (SC) of axonal transport conveys structural proteins, regulatory proteins, and glycolytic enzymes toward the axon tip at 1-6 mm/day. Following axon interruption (axotomy), the rate of outgrowth corresponds to the rate of SCb-the fastest subcomponent of SC. Both axonal outgrowth and SCb accelerate 20-25% after axotomy. Tubulin and actin are the major proteins being carried by SCb. To further characterize the acceleration of SCb, we measured the equilibrium between subunits and polymers for both actin and tubulin. We radiolabeled newly synthesized proteins in rat motor neurons by microinjecting [35S]methionine into the spinal cord 7 days after crushing the sciatic nerve (85 mm from the spinal cord). Nerves were removed 7 days later for homogenization in polymer-stabilizing buffer (PSB) and centrifugation, followed by SDS-PAGE of supernatants (S) and pellets (P). We removed beta-tubulin, actin, and the medium-weight neurofilament protein (NF-M) from each gel by using the fluorogram as a template. After solubilizing gel segments for liquid scintillation spectrometry, we expressed counts as a polymerization ratio: P/[S+P]. In the nerve segments that contained radiolabeled Scb proteins, located 24-36 mm from the spinal cord, axotomy increased the polymerization ratio of SCb actin from 0.23 to 0.36 (P < 0.05) but had no effect on SCb beta-tubulin. In a separate experiment, we added 12 microM taxol to PSB to stabilize newly assembled microtubules. Adding taxol did not alter the polymerization ratio for SCb beta-tubulin in sham-axotomized nerves but aid increase the ratio in axotomized nerves, from 0.44 to 0.63 (P < 0.05); polymerization ratios for SCb actin were unaffected. We conclude that the assembly of microfilaments and microtubules increases to provide cytoskeletal elements for axon sprouts. The resulting loss of actin and tubulin subunits may play a role in the acceleration of SCb.

摘要

轴突运输的慢速成分(SC)以每天1 - 6毫米的速度将结构蛋白、调节蛋白和糖酵解酶输送到轴突末端。轴突中断(轴突切断术)后,轴突生长速率与SCb(SC最快的子成分)的速率相对应。轴突切断术后,轴突生长和SCb均加速20 - 25%。微管蛋白和肌动蛋白是由SCb携带的主要蛋白质。为了进一步表征SCb的加速情况,我们测量了肌动蛋白和微管蛋白的亚基与聚合物之间的平衡。在坐骨神经挤压(距脊髓85毫米)7天后,通过向脊髓微量注射[35S]甲硫氨酸,我们对大鼠运动神经元中新合成的蛋白质进行放射性标记。7天后取出神经,在聚合物稳定缓冲液(PSB)中匀浆并离心,然后对上清液(S)和沉淀(P)进行SDS - 聚丙烯酰胺凝胶电泳。我们以荧光自显影片为模板,从每个凝胶中去除β - 微管蛋白、肌动蛋白和中等重量神经丝蛋白(NF - M)。在将凝胶片段溶解用于液体闪烁光谱测定后,我们将计数表示为聚合比:P / [S + P]。在距脊髓24 - 36毫米处含有放射性标记的SCb蛋白的神经节段中,轴突切断术使SCb肌动蛋白的聚合比从0.23增加到0.36(P < 0.05),但对SCbβ - 微管蛋白没有影响。在另一个实验中,我们向PSB中添加12微摩尔紫杉醇以稳定新组装的微管。添加紫杉醇不会改变假轴突切断术神经中SCbβ - 微管蛋白的聚合比,但会使轴突切断术神经中的聚合比从0.44增加到0.63(P < 0.05);SCb肌动蛋白的聚合比不受影响。我们得出结论,微丝和微管的组装增加,为轴突芽提供细胞骨架成分。肌动蛋白和微管蛋白亚基的减少可能在SCb的加速中起作用。

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