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紧密结合的ADP和ATP与叶绿体ATP合酶的调控及催化作用的关系。

Relationship of tightly bound ADP and ATP to control and catalysis by chloroplast ATP synthase.

作者信息

Zhou J M, Xue Z X, Du Z Y, Melese T, Boyer P D

机构信息

Department of Chemistry and Biochemistry, University of California, Los Angeles 90024-1570.

出版信息

Biochemistry. 1988 Jul 12;27(14):5129-35. doi: 10.1021/bi00414a027.

DOI:10.1021/bi00414a027
PMID:2901855
Abstract

Whether the tightly bound ADP that can cause a pronounced inhibition of ATP hydrolysis by the chloroplast ATP synthase and F1 ATPase (CF1) is bound at catalytic sites or at noncatalytic regulatory sites or both has been uncertain. We have used photolabeling by 2-azido-ATP and 2-azido-ADP to ascertain the location, with Mg2+ activation, of tightly bound ADP (a) that inhibits the hydrolysis of ATP by chloroplast ATP synthase, (b) that can result in an inhibited form of CF1 that slowly regains activity during ATP hydrolysis, and (c) that arises when low concentrations of ADP markedly inhibit the hydrolysis of GTP by CF1. The data show that in all instances the inhibition is associated with ADP binding without inorganic phosphate (Pi) at catalytic sites. After photophosphorylation of ADP or 2-azido-ADP with [32P]Pi, similar amounts of the corresponding triphosphates are present on washed thylakoid membranes. Trials with appropriately labeled substrates show that a small portion of the tightly bound 2-azido-ATP gives rise to covalent labeling with an ATP moiety at noncatalytic sites but that most of the bound 2-azido-ATP gives rise to covalent labeling by an ADP moiety at a catalytic site. We also report the occurrence of a 1-2-min delay in the onset of the Mg2+-induced inhibition after addition of CF1 to solutions containing Mg2+ and ATP, and that this delay is not associated with the filling of noncatalytic sites. A rapid burst of Pi formation is followed by a much lower, constant steady-state rate.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

紧密结合的ADP可显著抑制叶绿体ATP合酶和F1 ATP酶(CF1)的ATP水解,其是结合在催化位点、非催化调节位点还是两者都有,一直不确定。我们利用2-叠氮基-ATP和2-叠氮基-ADP进行光标记,以确定在Mg2+激活下紧密结合的ADP的位置,这种ADP:(a)抑制叶绿体ATP合酶的ATP水解;(b)可导致CF1的一种受抑制形式,其在ATP水解过程中缓慢恢复活性;(c)在低浓度ADP显著抑制CF1的GTP水解时出现。数据表明,在所有情况下,抑制作用都与催化位点上无无机磷酸(Pi)时ADP的结合有关。用[32P]Pi对ADP或2-叠氮基-ADP进行光磷酸化后,洗涤过的类囊体膜上存在相似量的相应三磷酸酯。用适当标记的底物进行的试验表明,一小部分紧密结合的2-叠氮基-ATP在非催化位点与ATP部分发生共价标记,但大部分结合的2-叠氮基-ATP在催化位点与ADP部分发生共价标记。我们还报告了在向含有Mg2+和ATP的溶液中添加CF1后,Mg2+诱导的抑制作用开始出现时有1-2分钟的延迟,且这种延迟与非催化位点的填充无关。Pi形成的快速爆发之后是一个低得多的恒定稳态速率。(摘要截短于250字)

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