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头部基团之间的间隔对驱动蛋白半位点 ADP 释放及动力学持续性的调控

Modulation of kinesin half-site ADP release and kinetic processivity by a spacer between the head groups.

作者信息

Hackney David D, Stock Maryanne F, Moore Jodi, Patterson Reid A

机构信息

Department of Biological Sciences, Carnegie Mellon University, 4400 Fifth Avenue, Pittsburgh, Pennsylvania 15213, USA. ddh+@andrew.cmu.edu

出版信息

Biochemistry. 2003 Oct 21;42(41):12011-8. doi: 10.1021/bi0349118.

Abstract

A series of modifications of the junction of the neck linker and neck coil of dimeric Drosophila kinesin were constructed to determine the influence of head orientation and spacing on the ATPase kinetics. Ala(345) is the first residue in the coiled-coil of the neck, and its replacement with glycine or proline produces no significant change in the k(cat) or K(0.5(MT)) values for activation of their ATPase by microtubules (MTs) or in their k(bi(ratio)) value for the average number of ATP molecules hydrolyzed during a processive encounter with a MT. Addition or deletion of a single amino acid at the junction produces only modest changes with less than a 2-fold reduction in kinetic processivity. Insertion of a spacer of 6 or 12 additional amino acids at the neck linker junction increases the K(0.5(MT)) value by 3-4-fold with a corresponding decrease in kinetic processivity. The sliding velocities of all the mutant constructs under multimotor conditions are within 30% of the wild-type value. All the constructs with single residue changes exhibit half-site ADP release on binding to MTs. The constructs with long insertion, however, rapidly release both ADP molecules per dimer on binding to a MT, indicating that the steric constraints that prevent release of ADP from the tethered head of wild-type kinesin have been relieved by the long insertions. The constructs with long inserts have decreased kinetic processivity and dissociate from the MT during ATP hydrolysis 3-fold faster than wild-type.

摘要

构建了一系列对二聚体果蝇驱动蛋白颈部连接子和颈部螺旋连接处的修饰,以确定头部方向和间距对ATP酶动力学的影响。丙氨酸(345)是颈部卷曲螺旋中的第一个残基,用甘氨酸或脯氨酸取代它,在微管(MT)激活其ATP酶的催化常数(k(cat))或半最大激活浓度(K(0.5(MT)))值,或在与MT进行持续相遇过程中水解的ATP分子平均数的双分子速率常数(k(bi(ratio)))值方面,均未产生显著变化。在连接处添加或删除单个氨基酸只会产生适度变化,动力学持续能力降低不到2倍。在颈部连接子连接处插入6个或12个额外氨基酸的间隔物会使K(0.5(MT))值增加3至4倍,同时动力学持续能力相应降低。在多马达条件下,所有突变体构建体的滑动速度都在野生型值的30%以内。所有单残基变化的构建体在与MT结合时均表现出半位点ADP释放。然而,具有长插入的构建体在与MT结合时,每个二聚体迅速释放两个ADP分子,这表明阻止野生型驱动蛋白束缚头部释放ADP的空间位阻已因长插入而得到缓解。具有长插入的构建体动力学持续能力降低,在ATP水解过程中从MT上解离的速度比野生型快3倍。

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