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Transients of fluorescence polarization in skeletal muscle fibers labeled with rhodamine on the regulatory light chain.

机译:在调节性轻链上用若丹明标记的骨骼肌纤维中的荧光偏振瞬变。

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摘要

Structural changes of the myosin heads were correlated with mechanical events in the cross-bridge cycle by measuring fluorescence polarization signals at high time resolution from rhodamine probes bound to myosin regulatory light chains in skeletal muscle fibers. Motions of the cross-bridges were partially synchronized either by applying quick length changes to the fibers during active contractions or by activating the fibers from rigor by photolysis of caged ATP in the presence of Ca2+. With fibers in rigor, the fluorescence polarization values indicate that the probe dipoles are quite well ordered and are directed away from the muscle fiber axis. After photorelease of ATP from caged ATP, changes in polarization signals are consistent with broadening of the distribution of probe orientations. The signal deflections occur when ATP binds to actomyosin or when the cross-bridges detach, but the orientational distribution changes surprisingly little during active force development. In contrast, when staircases of quick releases are applied to labeled fibers during active contractions, the fluorescence polarization signals suggest a concerted rotation of the probes. The results indicate that the light chain region of myosin tilts during the quick release and/or during the tension recovery phase within the next few ms.
机译:肌球蛋白头的结构变化与跨桥循环中的机械事件相关联,方法是通过以高分辨力测量来自与骨骼肌纤维中肌球蛋白调节性轻链结合的若丹明探针的荧光偏振信号。通过在主动收缩过程中对纤维施加快速的长度变化,或通过在存在Ca2 +的情况下对笼中的ATP进行光解,使纤维从严密的状态下激活,可以使跨桥的运动部分同步。在纤维严格的情况下,荧光偏振值表明探针偶极子有序排列,并远离肌肉纤维轴。从笼中的ATP光释放ATP后,极化信号的变化与探针方向分布的扩大一致。当ATP结合肌动球蛋白或横桥分离时,就会发生信号偏转,但是在主动力发展过程中,定向分布的变化却很小。相反,当在主动收缩过程中将快速释放阶梯施加到标记纤维上时,荧光偏振信号提示探针一致旋转。结果表明,肌球蛋白的轻链区在快速释放期间和/或在张力恢复阶段在接下来的几毫秒内倾斜。

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