Walker J E, Fearnley I M, Gay N J, Gibson B W, Northrop F D, Powell S J, Runswick M J, Saraste M, Tybulewicz V L
J Mol Biol. 1985 Aug 20;184(4):677-701. doi: 10.1016/0022-2836(85)90313-4.
The enzyme complex F1-ATPase has been isolated from bovine heart mitochondria by gel filtration of the enzyme released by chloroform from sub-mitochondrial particles. The five individual subunits alpha, beta, gamma, delta and epsilon that comprise the complex have been purified from it, and their amino acid sequences determined almost entirely by direct protein sequence analysis. A single overlap in the gamma-subunit was obtained by DNA sequence analysis of a complementary DNA clone isolated from a bovine cDNA library using a mixture of 32 oligonucleotides as the hybridization probe. The alpha, beta, gamma, delta and epsilon subunits contain 509, 480, 272, 146 and 50 amino acids, respectively. Two half cystine residues are present in the alpha-subunit and one in each of the gamma- and epsilon-chains; they are absent from the beta- and delta-subunits. The stoichiometry of subunits in the complex is estimated to be alpha 3 beta 3 gamma 1 delta 1 epsilon 1 and the molecular weight of the complex is 371,135. Mild trypsinolysis of the F1-ATPase complex, which has little effect on the hydrolytic activity of the enzyme, releases peptides from the N-terminal regions of the alpha- and beta-chains only; the C-terminal regions are unaffected. Sequence analysis of the released peptides demonstrates that the N terminals of the alpha- and beta-chains are ragged. In 65% of alpha-chains, the terminus is pyrrolidone carboxylic acid; in the remainder this residue is absent and the chains commence at residue 2, i.e. lysine. In the beta-subunit a minority of chains (16%) have N-terminal glutamine, or its deamidation product, glutamic acid (6%), or the cyclized derivative, pyrrolidone carboxylic acid (5%). A further 28% commence at residue 2, alanine, and 45% at residue 3, serine. The delta-chains also are heterogeneous; in 50% of chains the N-terminal alanine residue is absent. The sequences of the alpha- and beta-chains show that they are weakly homologous, as they are in bacterial F1-ATPases. The sequence of the bovine delta-subunit of F1-ATPase shows that it is the counterpart of the bacterial epsilon-subunit. The bovine epsilon-subunit is not related to any known bacterial or chloroplast H+-ATPase subunit, nor to any other known sequence. The counterpart of the bacterial delta-subunit is bovine oligomycin sensitivity conferral protein, which helps to bind F1 to the inner mitochondrial membrane.(ABSTRACT TRUNCATED AT 400 WORDS)
通过对氯仿从亚线粒体颗粒中释放的酶进行凝胶过滤,已从牛心线粒体中分离出F1 - ATP酶复合体。构成该复合体的五个亚基α、β、γ、δ和ε已从中纯化出来,并且几乎完全通过直接蛋白质序列分析确定了它们的氨基酸序列。使用32种寡核苷酸混合物作为杂交探针,从牛cDNA文库中分离出一个互补DNA克隆,通过对其进行DNA序列分析,获得了γ亚基中的一个单一重叠序列。α、β、γ、δ和ε亚基分别包含509、480、272、146和50个氨基酸。α亚基中有两个半胱氨酸残基,γ链和ε链中各有一个;β亚基和δ亚基中没有。该复合体中亚基的化学计量估计为α3β3γ1δ1ε1,复合体的分子量为371,135。对F1 - ATP酶复合体进行温和的胰蛋白酶消化,对该酶的水解活性影响很小,仅从α链和β链的N端区域释放出肽段;C端区域未受影响。对释放肽段的序列分析表明,α链和β链的N端参差不齐。在65%的α链中,末端是吡咯烷酮羧酸;其余的α链中没有这个残基,这些链从第2个残基即赖氨酸开始。在β亚基中,少数链(16%)的N端是谷氨酰胺,或其脱酰胺产物谷氨酸(6%),或环化衍生物吡咯烷酮羧酸(5%)。另外28%从第2个残基丙氨酸开始,45%从第3个残基丝氨酸开始。δ链也具有异质性;在50%的链中,N端丙氨酸残基不存在。α链和β链的序列表明它们具有弱同源性,细菌F1 - ATP酶中的情况也是如此。牛F1 - ATP酶δ亚基的序列表明它相当于细菌的ε亚基。牛ε亚基与任何已知的细菌或叶绿体H⁺ - ATP酶亚基均无关联,也与任何其他已知序列无关。细菌δ亚基的对应物是牛寡霉素敏感性赋予蛋白,它有助于将F1结合到线粒体内膜上。(摘要截短至400字)
