Amir-Zaltsman Y, Ezra E, Scherson T, Zutra A, Littauer U Z, Salomon Y
EMBO J. 1982;1(2):181-6. doi: 10.1002/j.1460-2075.1982.tb01144.x.
Incubation of purified rat brain tubulin with cholera toxin and radiolabeled [32P] or [8-3H]NAD results in the labeling of both alpha and beta subunits as revealed on sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). Treatment of these protein bands with snake venom phosphodiesterase resulted in quantitative release of labeled 5'-AMP, respectively labeled with the corresponding isotope. Two-dimensional separation by isoelectric focusing and SDS-PAGE of labeled and native tubulin revealed that labeling occurs at least in four different isotubulins. The isoelectric point of the labeled isotubulins was slightly lower than that of native purified tubulin. This shift in mobility is probably due to additional negative charges involved with the incorporation of ADP-ribosyl residues into the tubulin subunits. SDS-PAGE of peptides derived from [32P]ADP-ribosylated alpha and beta tubulin subunits by Staphylococcus aureus protease cleavage showed a peptide pattern identical with that of native tubulin. Microtubule-associated proteins (MAP1 and MAP2) of high molecular weight were also shown to undergo ADP-ribosylation. Incubation of permeated rat neuroblastoma cells in the presence of [32P]NAD and cholera toxin results in the labeling of only a few cell proteins of which tubulin is one of the major substrates.
用霍乱毒素以及放射性标记的[32P]或[8-3H]NAD培育纯化的大鼠脑微管蛋白,经十二烷基硫酸钠聚丙烯酰胺凝胶电泳(SDS-PAGE)显示,α和β亚基均被标记。用蛇毒磷酸二酯酶处理这些蛋白条带,分别导致标记的5'-AMP以相应同位素定量释放。对标记的和天然的微管蛋白进行等电聚焦和SDS-PAGE二维分离显示,标记至少发生在四种不同的同型微管蛋白中。标记的同型微管蛋白的等电点略低于天然纯化的微管蛋白。迁移率的这种变化可能是由于在微管蛋白亚基中掺入ADP-核糖基残基而产生了额外的负电荷。金黄色葡萄球菌蛋白酶裂解[32P]ADP-核糖基化的α和β微管蛋白亚基产生的肽段经SDS-PAGE显示,其肽谱与天然微管蛋白相同。高分子量的微管相关蛋白(MAP1和MAP2)也显示会发生ADP-核糖基化。在[32P]NAD和霍乱毒素存在的情况下培育通透的大鼠神经母细胞瘤细胞,结果显示只有少数细胞蛋白被标记,其中微管蛋白是主要底物之一。
