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通过测量荧光光漂白恢复来检测和表征溶液中的肌动蛋白单体、寡聚体和细丝。

Detection and characterization of actin monomers, oligomers, and filaments in solution by measurement of fluorescence photobleaching recovery.

作者信息

Lanni F, Ware B R

出版信息

Biophys J. 1984 Jul;46(1):97-110. doi: 10.1016/S0006-3495(84)84002-3.

Abstract

Fluorescence photobleaching recovery (FPR) was measured to determine the diffusion coefficient of fluorescein-labeled G-actin in low-salt buffer. The result obtained, 7.15 +/- 0.35 X 10(-7) cm2/s, is in good agreement with that computed from the molecular weight, partial specific volume, and sedimentation coefficient, but is higher than previously obtained values. It is demonstrated from theory that at low ionic strength, the electrostatic contribution to the intrinsic viscosity leads to an overestimate of the hydrodynamic eccentricity of G-actin. Data from FPR, sedimentation, and fluorescence polarization experiments all indicate that the true low-salt form of the actin monomer has an axial ratio less than or equal to 3.0. The G-F transformation of actin was also observed by measurement of FPR during the assembly phase, in the steady state, and in the presence of ligands such as cytochalasin and aldolase. Each FPR record in general yields three data: relative proportion of rapidly and slowly diffusing actin, diffusion coefficient for the high-mobility fraction, and a mean diffusion coefficient for the low-mobility fraction. A relation between the mean low-mobility diffusion coefficient and the number-average filament length is derived and applied to the analysis of FPR data. Under typical conditions, the average filament length was much greater than 10 micron in the steady state. Cytochalasin D was found to decrease filament length and total amount of filament proportionally; total filament number was not greatly affected. In all polymerizations of G-actin, the high-mobility material observed in situ was found to be essentially monomeric actin. Relatively stable oligomers of actin were separated by fractionating G-AF-actin by gel filtration in 50 microM MgCl2 at 4 degrees C. On the basis of the diffusion coefficient, we conclude that monomer and dimer constitute the major particle types present under these conditions. Sedimentation of labeled actin polymerized in 1.0 mM MgCl2 yielded a graded supernatant that contained actin oligomers significantly larger than the monomer.

摘要

通过测量荧光漂白恢复(FPR)来确定荧光素标记的G-肌动蛋白在低盐缓冲液中的扩散系数。得到的结果为7.15±0.35×10⁻⁷ cm²/s,与根据分子量、偏比容和沉降系数计算得出的值吻合良好,但高于先前获得的值。从理论上证明,在低离子强度下,静电对特性粘度的贡献导致对G-肌动蛋白流体动力学偏心率的高估。FPR、沉降和荧光偏振实验的数据均表明,肌动蛋白单体的真正低盐形式的轴比小于或等于3.0。在组装阶段、稳态以及存在诸如细胞松弛素和醛缩酶等配体的情况下,通过测量FPR也观察到了肌动蛋白的G-F转变。一般来说,每条FPR记录会产生三个数据:快速和缓慢扩散的肌动蛋白的相对比例、高迁移率部分的扩散系数以及低迁移率部分的平均扩散系数。推导了平均低迁移率扩散系数与数均细丝长度之间的关系,并将其应用于FPR数据的分析。在典型条件下,稳态时平均细丝长度远大于10微米。发现细胞松弛素D会按比例降低细丝长度和细丝总量;细丝总数受影响不大。在所有G-肌动蛋白的聚合反应中,原位观察到的高迁移率物质基本上是单体肌动蛋白。在4℃下于50μM MgCl₂中通过凝胶过滤对G-AF-肌动蛋白进行分级分离,从而分离出相对稳定的肌动蛋白寡聚体。基于扩散系数,我们得出结论,在这些条件下存在的主要颗粒类型是单体和二聚体。在1.0 mM MgCl₂中聚合的标记肌动蛋白的沉降产生了一个分级上清液,其中包含明显大于单体的肌动蛋白寡聚体。

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本文引用的文献

1
The cooperative nature of G-F transformation of actin.肌动蛋白G-F转换的协同性质
Biochim Biophys Acta. 1962 Feb 12;57:22-31. doi: 10.1016/0006-3002(62)91073-9.
2
The G-F equilibrium in actin solutions under various conditions.不同条件下肌动蛋白溶液中的G-F平衡。
Biochim Biophys Acta. 1962 Feb 12;57:13-21. doi: 10.1016/0006-3002(62)91072-7.
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MOLECULAR CHARACTERISTICS OF G-ADP ACTIN.G-ADP肌动蛋白的分子特征
Arch Biochem Biophys. 1964 Sep;107:441-8. doi: 10.1016/0003-9861(64)90300-5.
7
Spontaneous fragmentation of actin filaments in physiological conditions.
Nature. 1982 Mar 18;296(5854):266-7. doi: 10.1038/296266a0.

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