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通过生化和免疫学方法纯化脑微管蛋白酪氨酸连接酶

Purification of brain tubulin-tyrosine ligase by biochemical and immunological methods.

作者信息

Schröder H C, Wehland J, Weber K

出版信息

J Cell Biol. 1985 Jan;100(1):276-81. doi: 10.1083/jcb.100.1.276.

Abstract

Tubulin-tyrosine ligase (TTL), the enzyme responsible for the reversible addition of a tyrosine residue at the carboxyl end of alpha-tubulin, has been purified from porcine brain using a purification scheme based on standard biochemical procedures. The enzyme preparation was nearly homogeneous (purity greater than 95%), was free of tubulin, and could be stored in the presence of glycerol for several months without loss in activity. To develop a more convenient purification of TTL, we have isolated mouse hybridoma cells secreting antibodies to TTL. These monoclonal antibodies recognize TTL not only in brain tissue but also in the liver of various mammals. Monoclonal antibodies isolated from ascites fluid allowed a rapid purification of TTL from a crude brain extract. TTL stayed bound to the immunoaffinity column in 1.5 M NaCl and was eluted with 3 M MgCl2. Highly active TTL was recovered nearly quantitatively at greater than 95% purity and could be stabilized in the presence of glycerol. Glycerol gradient centrifugation, SDS gel electrophoresis and immunoblots identified TTL as a monomeric protein with an apparent polypeptide molecular weight of about 40,000. A one to one complex of TTL with alpha beta-tubulin was observed by gradient centrifugation.

摘要

微管蛋白酪氨酸连接酶(TTL)是一种负责在α-微管蛋白羧基末端可逆添加酪氨酸残基的酶,已使用基于标准生化程序的纯化方案从猪脑中纯化出来。该酶制剂几乎是纯的(纯度大于95%),不含微管蛋白,并且可以在甘油存在下储存数月而活性不失。为了开发更简便的TTL纯化方法,我们分离了分泌针对TTL抗体的小鼠杂交瘤细胞。这些单克隆抗体不仅能识别脑组织中的TTL,还能识别各种哺乳动物肝脏中的TTL。从腹水液中分离的单克隆抗体可使TTL从粗脑提取物中快速纯化。TTL在1.5 M NaCl中与免疫亲和柱结合,并在3 M MgCl2中洗脱。以大于95%的纯度几乎定量地回收了高活性的TTL,并且可以在甘油存在下稳定保存。甘油梯度离心、SDS凝胶电泳和免疫印迹鉴定TTL为一种表观多肽分子量约为40,000的单体蛋白。通过梯度离心观察到TTL与αβ-微管蛋白形成一对一的复合物。

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