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衣藻鞭毛表面运动的可逆抑制。

Reversible inhibition of Chlamydomonas flagellar surface motility.

作者信息

Bloodgood R A, Leffler E M, Bojczuk A T

出版信息

J Cell Biol. 1979 Sep;82(3):664-74. doi: 10.1083/jcb.82.3.664.

Abstract

Chlamydomonas exhibits force transduction in association with its flagellar surface; this can be visualized by the saltatory movements of attached polystyrene microspheres. This flagellar surface motility has been quantitated by determining the percentage of attached microspheres in motion at the time of observation (60% in the case of control cells at 25 degrees C). A number of experimental treatments reversibly inhibit flagellar surface motility. These include an increase in sodium or potassium chloride concentration, a decrease in temperature, or a decrease in the free calcium concentration in the medium. Many of the conditions that result in inhibition of flagellar surface motility also result in an induction of flagellar resorption. Although both flagellar stability and flagellar surface motility are dependent on the availability of calcium, the two processes are separable; under appropriate conditions, flagellar surface motility can occur at normal levels on flagella that are resorbing. Inhibition of protein synthesis results in a gradual loss of both the binding of microspheres to the flagellum and the flagellar surface motility. After resumption of protein synthesis, both binding and movement return to control levels. The effect of the inhibition of protein synthesis is interpreted in terms of selective turnover of certain components within the intact flagellum, one or more of these components being necessary for the binding of the microspheres and their subsequent movement. If this turnover is inhibited by keeping the cells below 5 degrees C, the absence of protein synthesis no longer has an effect on microsphere attachment and motility, when measured immediately after warming the cells to 25 degrees C.

摘要

衣藻在其鞭毛表面表现出力传导;这可以通过附着的聚苯乙烯微球的跳跃运动来观察到。这种鞭毛表面运动性已通过确定观察时运动的附着微球的百分比来定量(在25摄氏度的对照细胞中为60%)。许多实验处理可可逆地抑制鞭毛表面运动性。这些包括增加氯化钠或氯化钾浓度、降低温度或降低培养基中的游离钙浓度。许多导致鞭毛表面运动性抑制的条件也会导致鞭毛吸收的诱导。尽管鞭毛稳定性和鞭毛表面运动性都依赖于钙的可用性,但这两个过程是可分离的;在适当条件下,鞭毛表面运动性可以在正在吸收的鞭毛上以正常水平发生。蛋白质合成的抑制导致微球与鞭毛的结合以及鞭毛表面运动性逐渐丧失。蛋白质合成恢复后,结合和运动都恢复到对照水平。蛋白质合成抑制的作用是根据完整鞭毛内某些成分的选择性更新来解释的,这些成分中的一种或多种对于微球的结合及其随后的运动是必需的。如果通过将细胞保持在5摄氏度以下来抑制这种更新,当将细胞加热到25摄氏度后立即测量时,蛋白质合成的缺失不再对微球附着和运动性产生影响。

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