显微注射完整的MAP-4及其片段可诱导PtK2细胞骨架的变化。

T Yoshida, K Imanaka-Yoshida, H Murofushi, J Tanaka, H Ito, M Inagaki
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引用次数: 24

摘要

微管相关蛋白(MAP)-4的分子克隆和测序鉴定了c端附近的微管结合重复序列和n端附近的投影结构域。虽然众所周知,MAP-4在体外刺激微管(MT)的组装和稳定,但MAP-4在体内的功能尚不清楚。在这项研究中,我们在体外和体内检测了MAP-4在细胞骨架中的功能。以牛肾上腺皮质为原料制备完整的MAP-4,并在大肠杆菌中表达和分离了N-和c -末端的截断片段(分别命名为NR和PA4片段)。体外研究表明,在含有生理浓度NaCl的溶液中,完整的MAP-4和PA4片段与MT结合,而不是与F-actin结合。NR片段未与MT或F-actin结合。我们还检测了PtK2细胞微注射完整的MAP-4和PA4和NR截短片段后MT的变化。细胞注射完整的MAP-4或PA4诱导细胞质MT数量增加,以及MT捆绑。NR片段不影响MT阵列。注射MAP-4和PA4与MT增加有关。此外,注射MAP-4和PA4与MT干扰药物诺可达唑治疗相关,可以稳定MT。这些结果表明,在体内和体外,完整的MAP-4和PA4片段通过与MT结合,促进了MT的组装并稳定了MT。此外,注射PA4片段诱导应力纤维增加。然而,这些蛋白质没有显示出与应力纤维的任何关联。我们的研究结果表明,MAP-4对应力纤维的影响是间接的,而不是MAP-4和应力纤维之间的直接相互作用。
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Microinjection of intact MAP-4 and fragments induces changes of the cytoskeleton in PtK2 cells.

The molecular cloning and sequencing of microtubule-associated protein (MAP)-4 identified microtubule-binding repeats near the C-terminus and a projection domain near the N-terminus. Although it is well known that MAP-4 stimulates the assembly of and stabilizes microtubules (MT) in vitro, the function of MAP-4 in vivo is still unclear. In this study, we examined the function of MAP-4 in the cytoskeleton both in vitro and in vivo. Intact MAP-4 was prepared from bovine adrenal cortex, and the truncated fragments of the N- and the C-terminal halves (named NR and PA4 fragments, respectively) were expressed in Escherichia coli and isolated. In vitro studies demonstrated that in a solution containing a physiological concentration of NaCl, intact MAP-4 and the PA4 fragment were bound to MT, but not to F-actin. The NR fragment was not bound to MT or to F-actin. We also examined the MT changes in PtK2 cells after they had been microinjected with intact MAP-4 and the truncated fragments of PA4 and NR. The injection of intact MAP-4 or PA4 into the cells induced an increase in the number of cytoplasmic MT, as well as MT bundling. The NR fragment did not affect the MT array. Injected MAP-4 and PA4 were associated with the increased MT. In addition, injection with MAP-4 and PA4 stabilized MT in relation to treatment with the MT-disrupting drug, nocodazole. These results indicated that intact MAP-4 and the PA4 fragment promoted MT assembly and stabilized MT, by binding to MT, in vivo as well as in vitro. Further, the injection of the PA4 fragment induced an increase in stress fibers. However, these proteins did not show any association with the stress fibers. Our results suggest that there is an indirect effect of MAP-4 on stress fibers rather than a direct interaction between MAP-4 and stress fibers.

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