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处于僵直和弱结合状态的脊椎动物骨骼肌中肌动蛋白丝组织和肌球蛋白头部标记模式。

Actin filament organization and myosin head labelling patterns in vertebrate skeletal muscles in the rigor and weak binding states.

作者信息

Squire J M, Harford J J

机构信息

Biophysics Section, Blackett Laboratory, Imperial College, London, U.K.

出版信息

J Muscle Res Cell Motil. 1988 Aug;9(4):344-58. doi: 10.1007/BF01773878.

Abstract

The structures of vertebrate skeletal muscles (particularly from frog and fish) in the rigor state are analysed in terms of the concept of target areas on actin filaments. Assuming that 100% of the heads are to be attached to actin in rigor, then satisfactory qualitative low-resolution modelling of observed X-ray diffraction data is obtained if the outer ends of these myosin heads can move axially (total range about 200A) and azimuthally (total range less than 60 degrees) from their original lattice sites on the myosin filament surface to attach in defined target areas on the actin filaments. On this basis, each actin target area comprises about four actin monomers along one of the two long-pitched helical strands of the actin filament (about 200 A) or an azimuthal range of actin binding sites of about 100 degrees around the thin filament axis. If myosin heads simply label in a non-specific way the nearest actin monomers to them, as could occur with non-specific transient attachment in a 'weak binding' state, then the predicted X-ray diffraction pattern would comprise layer lines at the same axial spacings (orders of 429 A) as those seen in patterns from resting muscle. It is shown that actin target areas in vertebrate skeletal muscles are probably arranged on an approximate 62 (right-handed) helix of pitch (P) of about 720 A, subunit translation P/6 and near repeat P/2. Troponin position need not be considered in defining the labelling pattern of cross-bridges on this 62 helix of target areas; the target areas appear to be defined solely by the azimuthal position of the actin binding sites. The distribution of actin filament labelling patterns could be regular in fish muscle which has a 'crystalline' A-band, but will be irregular in higher vertebrate muscles such as frog sartorius muscle.

摘要

根据肌动蛋白丝上目标区域的概念,对处于僵直状态的脊椎动物骨骼肌(特别是青蛙和鱼类的骨骼肌)结构进行了分析。假设在僵直状态下100%的头部都与肌动蛋白结合,那么如果这些肌球蛋白头部的外端能够从肌球蛋白丝表面的原始晶格位置轴向移动(总范围约200埃)和方位角移动(总范围小于60度),以附着在肌动蛋白丝上特定的目标区域,就可以得到与观察到的X射线衍射数据相符的定性低分辨率模型。在此基础上,每个肌动蛋白目标区域沿着肌动蛋白丝两条长间距螺旋链之一包含约四个肌动蛋白单体(约200埃),或者围绕细肌丝轴的肌动蛋白结合位点方位角范围约为100度。如果肌球蛋白头部只是以非特异性方式标记与其最近的肌动蛋白单体,就像在“弱结合”状态下非特异性瞬时附着时可能发生的那样,那么预测的X射线衍射图谱将包含与静息肌肉图谱中相同轴向间距(429埃量级)的层线。研究表明,脊椎动物骨骼肌中的肌动蛋白目标区域可能排列在一个近似的62(右手)螺旋上,螺距(P)约为720埃,亚基平移为P/6,近重复为P/2。在定义目标区域的这个62螺旋上的横桥标记模式时,无需考虑肌钙蛋白的位置;目标区域似乎仅由肌动蛋白结合位点的方位角位置定义。在具有“晶体状”A带的鱼类肌肉中,肌动蛋白丝标记模式的分布可能是规则的,但在高等脊椎动物肌肉如青蛙缝匠肌中则是不规则的。

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