Williams N, Hullihen J, Pedersen P L
Biochemistry. 1987 Jan 13;26(1):162-9. doi: 10.1021/bi00375a023.
F1-ATPase of rat liver was examined for its capacity to interact with both metal ions and nucleotides and for the effect of covalent ATPase inhibitors on these interactions. As isolated, rat liver F1 contains about 2 mol of Mg2+/mol of F1, 1 mol of which can be removed or exchanged. The remaining mole of Mg2+ per mole of F1 remains very tightly associated with F1 and is recovered in the alpha gamma fraction after cold denaturation. Rat liver F1 also contains as isolated a nearly equivalent amount of nucleotide (approximately 1.7 mol/mol of F1) which is readily removed by incubation at room temperature followed by column centrifugation. The "2 Mg2+ enzyme" binds almost 3 mol of 5'-adenylyl imidodiphosphate (AMP-PNP)/mol of F1 in the presence or absence of added divalent cation. When divalent cation is present as Co2+, an equivalent activator to Mg2+ in the ATPase reaction, 1 mol of F1 binds 3 mol of both AMP-PNP and Co2+. under these conditions, the very tight Mg2+ site remains loaded, the exchangeable Mg2+ site is replaced with AMP-PNPCo, and two additional AMP-PNPCo sites are filled. At this point, ADP can be loaded onto the enzyme as a fourth nucleotide at a site separate and distinct from the AMP-PNP sites. Significantly, rat liver F1 contains only a single readily detectable ADP binding site in the presence or absence of divalent cation.(ABSTRACT TRUNCATED AT 250 WORDS)
对大鼠肝脏的F1 - ATP酶进行了研究,考察其与金属离子和核苷酸相互作用的能力,以及共价ATP酶抑制剂对这些相互作用的影响。刚分离出来时,大鼠肝脏F1每摩尔含有约2摩尔Mg2 +,其中1摩尔可以被去除或交换。每摩尔F1剩余的1摩尔Mg2 +与F1紧密结合,在冷变性后可在αγ组分中回收。刚分离出来的大鼠肝脏F1还含有几乎等量的核苷酸(约每摩尔F1含1.7摩尔),通过室温孵育然后柱离心可轻易去除。“2Mg2 +酶”在添加或不添加二价阳离子的情况下,每摩尔F1能结合近3摩尔的5'-腺苷酰亚胺二磷酸(AMP - PNP)。当二价阳离子为Co2 +(ATP酶反应中与Mg2 +等效的激活剂)时,1摩尔F1能结合3摩尔的AMP - PNP和Co2 +。在这些条件下,紧密结合的Mg2 +位点保持被占据状态,可交换的Mg2 +位点被AMP - PNP - Co取代,另外两个AMP - PNP - Co位点被填满。此时,ADP可以作为第四个核苷酸加载到酶上,位于与AMP - PNP位点分开且不同的位点。值得注意的是,无论有无二价阳离子,大鼠肝脏F1仅含有一个易于检测到的ADP结合位点。(摘要截短至250字)
