Single-molecule imaging of fluorescent proteins

被引:14
|
作者
Douglass, Adam D. [1 ]
Vale, Ronald D. [1 ]
机构
[1] Univ Calif San Francisco, Howard Hughes Med Inst, Dept Cellular & Mol Pharmacol, San Francisco, CA 94107 USA
来源
关键词
D O I
10.1016/S0091-679X(08)85006-6
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Single molecule imaging techniques overcome the averaging effects inherent in ensemble measurements and. enable characterization of the enormous heterogeneity that exists in biomolecular systems. Though long the domain of a few highly specialized labs, optical imaging of single molecules in living cells is becoming a widely accessible technique. The development of commercially available microscopes, robust analysis tools, and sensitive, low-noise detectors has contributed to this dissemination, as has the ever-growing array of fluorescent proteins. The relative ease with which genetically-tagged proteins can be created and introduced into a cell has largely eliminated more cumbersome and less precise means of particle labeling. A number of special considerations apply when using genetically encoded fluorophores for single molecule experiments, however. We discuss the means by which fluorescent proteins can be transfected into living cells to obtain the low particle densities required for single molecule imaging, and consider the limitations that are placed on single molecule analysis by the fluorophore's photo-physical properties. We also discuss the types of morphology and subcellular localization that make certain preparations more amenable to single particle imaging than others. Last, we discuss some common pitfalls involved in analyzing single molecule datasets, and consider some of the unique information that can be obtained using these techniques.
引用
收藏
页码:113 / 125
页数:13
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