Blanchard C Z, Hales B J
Louisiana State University, Baton Rouge 70803-1804, USA.
Biochemistry. 1996 Jan 16;35(2):472-8. doi: 10.1021/bi951429j.
When Q-Sepharose was used in the purification of the V nitrogenase proteins from Azotobacter vinelandii, an increase in resolution was observed that resulted in a separation of the nitrogenase component 1 protein (Av1') into two forms, labeled Av1'A and Av1'B. Even though both forms possessed the same enzymatic behavior, Av1'A exhibited a lower specific activity and migrated during gel filtration with an apparent lower molecular weight than Av1'B. Furthermore, SDS-polyacrylamide gel electrophoresis showed different relative compositions of the two major subunits of both forms, with Av1'A possessing a trimer (alpha beta 2) pattern compared to the more typical tetramer (alpha 2 beta 2) pattern found for Av1'B. Metal analysis indicated a V-to-Fe ratio of 1:19 for Av1'A and 1:15 (or 2:30) for Av1'B, while acid-labile sulfide analysis showed that Av1'A possessed about half as much sulfide as Av1'B. EPR spectroscopy revealed that both proteins retained the S = 3/2 and S = 1/2 signals observed in earlier isolations, with an additional S = 1/2 signal present in the spectrum of protein A. These results suggest that Av1'A is an incomplete form of the VFe protein, containing only one cofactor and one P cluster with an additional [Fe4-S4]-like cluster. The presence of a V storage protein in A. vinelandii was also investigated. Although no V storage protein was found, two V-binding proteins were observed.
当使用Q-琼脂糖从棕色固氮菌中纯化V型固氮酶蛋白时,分辨率有所提高,导致固氮酶组分1蛋白(Av1')分离为两种形式,分别标记为Av1'A和Av1'B。尽管两种形式具有相同的酶促行为,但Av1'A的比活性较低,在凝胶过滤过程中的迁移分子量明显低于Av1'B。此外,SDS-聚丙烯酰胺凝胶电泳显示两种形式的两个主要亚基的相对组成不同,Av1'A具有三聚体(αβ2)模式,而Av1'B则具有更典型的四聚体(α2β2)模式。金属分析表明,Av1'A的V与Fe的比例为1:19,Av1'B为1:15(或2:30),而酸不稳定硫化物分析表明,Av1'A的硫化物含量约为Av1'B的一半。电子顺磁共振光谱显示,两种蛋白质都保留了早期分离中观察到的S = 3/2和S = 1/2信号,蛋白质A的光谱中还存在一个额外的S = 1/2信号。这些结果表明,Av1'A是VFe蛋白的一种不完整形式,仅包含一个辅因子和一个P簇以及一个额外的[Fe4-S4]样簇。还研究了棕色固氮菌中V储存蛋白的存在情况。虽然未发现V储存蛋白,但观察到两种V结合蛋白。
