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蛋白质聚集。对C-藻蓝蛋白更大聚集体的研究。

Protein aggregation. Studies of larger aggregates of C-phycocyanin.

作者信息

Lee J J, Berns D S

出版信息

Biochem J. 1968 Dec;110(3):457-64. doi: 10.1042/bj1100457.

Abstract

Aggregates of phycocyanin sedimenting at 17s, 22s and 27s are demonstrated to constitute more than 40% of crude blue-green-algal extracts, pH6.0 and I0.1, and are retained in highly purified preparations. Sedimentation-velocity studies of the large aggregates as a function of pH are reported. Sucrose-density-gradient experiments performed as a function of time of sedimentation indicate that: (1) with increasing time of sedimentation, the largest aggregates are dissipated at the leading protein boundary and the several phycocyanin species present are not completely resolved; (2) phycocyanin fractions with the largest aggregates exhibit the highest E(620)/E(280) ratio and the largest relative fluorescence efficiency. Gel-filtration experiments with Sephadex G-200 do not resolve the species completely, and reapplication of phycocyanin gel-filtration fractions to the column results in an elution pattern similar to the original, except that there is an enhancement of the allophycocyanin fraction and the amount of denatured protein. Increasing the sedimentation times in a sucrose density gradient also enhances the allophycocyanin fraction. Fluorescence results demonstrate that there are possibly three excitation maxima, one corresponding to the monomer (approx. 600mmu), one for higher aggregates (625-630mmu) and one for the allophycocyanin fraction (approx. 650mmu). Only a single fluorescence-emission band is detected, which is fairly symmetrical and which has a red shift with higher aggregation and with the appearance of allophycocyanin. The appearance of allophycocyanin may be correlated with the irreversible disaggregation of the largest phycocyanin species. It is suggested that the largest protein aggregates are in the size range of the biliprotein aggregates reported in electron microscopy of algal cells.

摘要

沉降系数为17s、22s和27s的藻蓝蛋白聚集体被证明在pH6.0和离子强度0.1的粗蓝绿藻提取物中占比超过40%,并且保留在高度纯化的制剂中。本文报道了大聚集体沉降速度随pH的变化研究。蔗糖密度梯度实验随沉降时间的变化表明:(1)随着沉降时间增加,最大的聚集体在前沿蛋白边界处消散,存在的几种藻蓝蛋白种类没有完全分离;(2)具有最大聚集体的藻蓝蛋白组分表现出最高的E(620)/E(280)比值和最大的相对荧光效率。用葡聚糖凝胶G-200进行的凝胶过滤实验不能完全分离这些种类,将藻蓝蛋白凝胶过滤组分重新上样到柱上会得到与原始洗脱模式相似的结果,只是别藻蓝蛋白组分增加且变性蛋白量增加。在蔗糖密度梯度中增加沉降时间也会增加别藻蓝蛋白组分。荧光结果表明可能有三个激发最大值,一个对应单体(约600nm),一个对应更高聚集体(625 - 630nm),一个对应别藻蓝蛋白组分(约650nm)。只检测到一个相当对称的单一荧光发射带,随着聚集体增加和别藻蓝蛋白出现,该发射带会发生红移。别藻蓝蛋白的出现可能与最大藻蓝蛋白种类的不可逆解聚有关。有人认为最大的蛋白质聚集体大小在藻类细胞电子显微镜报道的双蛋白聚集体范围内。

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