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丹麦赭球藻的鞭毛膜。鞭毛膜、轴丝和茸鞭的分离及电泳分析。

The flagellar membrane of Ochromonas danica. Isolation and electrophoretic analysis of the flagellar membrane, axonemes, and mastigonemes.

作者信息

Chen L L, Haines T H

出版信息

J Biol Chem. 1976 Mar 25;251(6):1828-34.

PMID:943397
Abstract

The isolation and purification of the flagellar membrane of the phytoflagellate, Ochromonas danica, is described. The procedure is simple, mild, rapid, and it produces a pure membrane preparation. The method additionally permits the isolation of clean preparations of axonemes and mastigonemes from a single flagella preparation. Each component was studied by electron microscopy and acrylamide gel electrophroesis. The isolated flagella preparation was nearly free of other cellular organelles as judged by phase contrast and electron microscopy. The purified membrane preparation consisted of small vesicles (500 to 1500 A in diameter) with a trilamellar pattern about 80 A thick. Isolated membrane was analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, displaying five major protein bands, five minor protein bands, and some protein which remained at the origin. The five major protein components had apparent molecular weights of 54,000, 47,000, 35,000, 31,000, and 28,000. All mastigoneme protein components are glycoproteins as judged by periodic acid-Schiff staining. The mastigoneme preparation contained three major protein bands. Two of them were revealed as doublets and migrated with an average velocity corresponding to 83,000 delatons, the other major protein band migrated with a velocity corresponding to 54,000 daltons. A heavy carbohydrate band is seen near the bromphenol blue tracking dye. The axoneme preparation showed one major protein band having an apparent molecular weight of about 54,000 and some proteins having high molecular weights which remained on top of the polyacrylamide gel.

摘要

本文描述了对植物鞭毛虫丹麦赭纤虫鞭毛膜的分离与纯化。该方法简单、温和、快速,且能得到纯净的膜制剂。此外,该方法还能从单一鞭毛制剂中分离出纯净的轴丝和茸鞭的制剂。通过电子显微镜和丙烯酰胺凝胶电泳对每个组分进行了研究。通过相差显微镜和电子显微镜判断,分离得到的鞭毛制剂几乎不含其他细胞器。纯化后的膜制剂由直径为500至1500埃的小囊泡组成,具有约80埃厚的三层结构。通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳对分离得到的膜进行分析,显示出五条主要蛋白带、五条次要蛋白带以及一些留在原点的蛋白。这五条主要蛋白组分的表观分子量分别为54,000、47,000、35,000、31,000和28,000。通过高碘酸-希夫染色判断,所有茸鞭蛋白组分均为糖蛋白。茸鞭制剂包含三条主要蛋白带。其中两条显示为双重带,迁移平均速度对应83,000道尔顿,另一条主要蛋白带迁移速度对应54,000道尔顿。在溴酚蓝示踪染料附近可见一条浓重的碳水化合物带。轴丝制剂显示出一条表观分子量约为54,000的主要蛋白带以及一些高分子量蛋白,这些蛋白留在聚丙烯酰胺凝胶的顶部。

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