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Altering the speed of a DNA packaging motor from bacteriophage T4
被引:6
|作者:
Lin, Siying
[1
]
Alam, Tanfis I.
[1
]
Kottadiel, Vishal I.
[1
]
VanGessel, Carl J.
[1
]
Tang, Wei-Chun
[1
]
Chemla, Yann R.
[2
]
Rao, Venigalla B.
[1
]
机构:
[1] Catholic Univ Amer, Dept Biol, Washington, DC 20064 USA
[2] Univ Illinois, Ctr Biophys & Quantitat Biol, Dept Phys, Urbana, IL USA
基金:
美国国家科学基金会;
美国国家卫生研究院;
关键词:
SINGLE-MOLECULE;
EVOLUTIONARY RELATIONSHIPS;
SMALL TERMINASE;
ATPASE;
TRANSLOCATION;
MECHANISMS;
COORDINATION;
PROCESSIVITY;
PROTEINS;
DYNAMICS;
D O I:
10.1093/nar/gkx809
中图分类号:
Q5 [生物化学];
Q7 [分子生物学];
学科分类号:
071010 ;
081704 ;
摘要:
The speed at which a molecular motor operates is critically important for the survival of a virus or an organism but very little is known about the underlying mechanisms. Tailed bacteriophage T4 employs one of the fastest and most powerful packaging motors, a pentamer of gp17 that translocates DNA at a rate of up to similar to 2000-bp/s. We hypothesize, guided by structural and genetic analyses, that a unique hydrophobic environment in the catalytic space of gp17-adenosine triphosphatase (ATPase) determines the rate at which the 'lytic water' molecule is activated and OH-nucleophile is generated, in turn determining the speed of the motor. We tested this hypothesis by identifying two hydrophobic amino acids, M195 and F259, in the catalytic space of gp17-ATPase that are in a position to modulate motor speed. Combinatorial mutagenesis demonstrated that hydrophobic substitutions were tolerated but polar or charged substitutions resulted in null or cold-sensitive/small-plaque phenotypes. Quantitative biochemical and single-molecule analyses showed that the mutant motors exhibited 1.8-to 2.5-fold lower rate of ATP hydrolysis, 2.5-to 4.5-fold lower DNA packaging velocity, and required an activator protein, gp16 for rapid firing of ATPases. These studies uncover a speed control mechanism that might allow selection of motors with optimal performance for organisms' survival.
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页码:11437 / 11448
页数:12
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