Measuring fast gene dynamics in single cells with time-lapse luminescence microscopy

被引:18
|
作者
Mazo-Vargas, Anyimilehidi [1 ,2 ,3 ]
Park, Heungwon [1 ,2 ,3 ,4 ]
Aydin, Mert [1 ,2 ,3 ]
Buchler, Nicolas E. [1 ,2 ,3 ,4 ]
机构
[1] Duke Univ, Inst Genome Sci & Policy, Durham, NC 27710 USA
[2] Duke Univ, Duke Ctr Syst Biol, Durham, NC 27710 USA
[3] Duke Univ, Dept Biol, Durham, NC 27710 USA
[4] Duke Univ, Dept Phys, Durham, NC 27710 USA
基金
美国国家卫生研究院;
关键词
GREEN FLUORESCENT PROTEIN; FIREFLY LUCIFERASE; SACCHAROMYCES-CEREVISIAE; IMAGE-ANALYSIS; BUDDING YEAST; BIOLUMINESCENCE; EXPRESSION; CYCLE; SYSTEM; MUTAGENESIS;
D O I
10.1091/mbc.E14-07-1187
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Time-lapse fluorescence microscopy is an important tool for measuring in vivo gene dynamics in single cells. However, fluorescent proteins are limited by slow chromophore maturation times and the cellular autofluorescence or phototoxicity that arises from light excitation. An alternative is luciferase, an enzyme that emits photons and is active upon folding. The photon flux per luciferase is significantly lower than that for fluorescent proteins. Thus time-lapse luminescence microscopy has been successfully used to track gene dynamics only in larger organisms and for slower processes, for which more total photons can be collected in one exposure. Here we tested green, yellow, and red beetle luciferases and optimized substrate conditions for in vivo luminescence. By combining time-lapse luminescence microscopy with a microfluidic device, we tracked the dynamics of cell cycle genes in single yeast with subminute exposure times over many generations. Our method was faster and in cells with much smaller volumes than previous work. Fluorescence of an optimized reporter (Venus) lagged luminescence by 15-20 min, which is consistent with its known rate of chromophore maturation in yeast. Our work demonstrates that luciferases are better than fluorescent proteins at faithfully tracking the underlying gene expression.
引用
收藏
页码:3699 / 3708
页数:10
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