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[溶液中纤维蛋白原分子的构象:动态光散射光谱法]

[Conformation of the fibrinogen molecule in solution: dynamic light scattering spectroscopy].

作者信息

Serallach E, Hofmann V, Zulnauf M, Kän;ig W, Straub P W

出版信息

Schweiz Med Wochenschr. 1976 Oct 2;106(40):1380.

PMID:1006262
Abstract

Human fibrinogen solutions were prepared either by filtration of ultracentrifugation. The sedimentation coefficient was S20,W = 7,9 S. The translational and the rotational diffusion coefficient DT and DR and the fraction of oligomers were determined using light beating spectroscopy. DT20,W was (2.03 +/- 1%) 10(-7)-cm2-sec-1, DR120,W = 40 000 +/- 10%-sec-1. The sedimentation coefficient and DT were strongly dependent on concentration. For pH values between 6.5 and 9.0, the diffusion coefficient DT at ionic strength greater than 0.2 was constant. The diffusion coefficient as measured by nanosecond fluorescence depolarization was DR//20,W = 1.6 x 10(6) sec-1. At a fibrinogen concentration of 2 mg/ml, these hydrodynamic data are compatible with an elongated molecule of 450 A length and an axial ratio of about 1:7.

摘要

人纤维蛋白原溶液通过过滤或超速离心制备。沉降系数为S20,W = 7.9 S。使用光拍光谱法测定平移扩散系数DT和旋转扩散系数DR以及寡聚体的比例。DT20,W为(2.03±1%)×10(-7) cm2·sec-1,DR120,W = 40000±10%·sec-1。沉降系数和DT强烈依赖于浓度。对于pH值在6.5至9.0之间,离子强度大于0.2时的扩散系数DT是恒定的。通过纳秒荧光去极化测量的扩散系数为DR//20,W = 1.6×10(6) sec-1。在纤维蛋白原浓度为2 mg/ml时,这些流体动力学数据与长度为450 Å且轴比约为1:7的细长分子相符。

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