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Biomolecular applications of single-molecule measurements : Kinetics and dynamics of a single enzyme reaction
被引:5
|作者:
Paige, MF
[1
]
Fromm, DP
[1
]
Moerner, WE
[1
]
机构:
[1] Stanford Univ, Dept Chem, Stanford, CA 94305 USA
来源:
METHODS FOR ULTRASENSITIVE DETECTION II
|
2002年
/
4634卷
关键词:
single-molecule;
enzyme;
fluorescence;
kinetics;
microscopy;
immobilization;
D O I:
10.1117/12.463828
中图分类号:
TM [电工技术];
TN [电子技术、通信技术];
学科分类号:
0808 ;
0809 ;
摘要:
In this work we describe preliminary experiments in which we have used ultra-sensitive fluorescence microscopy to observe the dynamics of individual enzyme molecules acting upon a substrate. The enzyme, P-galactosidase from E.coli, is specifically immobilized onto a glass substrate while maintaining its functionality. The immobilized protein degrades a fluorogenic substrate to produce a fluorescent product, whose generation can be observed in real time. Individual copies of beta-galactosidase can be observed for many minutes, allowing the measurement of a large number of successive substrate turnover events. A rudimentary analysis of these turnovers using autocorrelation functions is presented, and a strong heterogeneity in reaction rates between different molecules is observed. In addition, the challenges inherent in successful surface immobilization of proteins for single-molecule experiments are discussed.
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页码:92 / 103
页数:12
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