Advantages of substituting bioluminescence for fluorescence in a resonance energy transfer-based periplasmic binding protein biosensor

被引:18
|
作者
Dacres, Helen [1 ]
Michie, Michelle [1 ]
Anderson, Alisha [1 ]
Trowell, Stephen C. [1 ]
机构
[1] CSIRO Food Futures Natl Res Flagship & Ecosyst Sc, Canberra, ACT 2601, Australia
来源
关键词
RLuc2; RLuc8; Maltose binding proteins; Beer analysis; Conformational change; MALTOSE-BINDING; RENILLA LUCIFERASE; RECEPTOR; DESIGN; TRANSPORT; LIGAND; CELLS; MBP;
D O I
10.1016/j.bios.2012.09.004
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
A genetically encoded maltose biosensor was constructed, comprising maltose binding protein (MBP) flanked by a green fluorescent protein (GFP(2)) at the N-terminus and a Renilla luciferase variant (RLuc2) at the C-terminus. This Bioluminescence resonance energy transfer(2) (BRET2) system showed a 30% increase in the BEET ratio upon maltose binding, compared with a 10% increase with an equivalent fluorescence resonance energy transfer (FRET) biosensor. BRET2 provides a better matched Forster distance to the known separation of the N and C termini of MBP than FRET. The sensor responded to maltose and maltotriose and the response was completely abolished by introduction of a single point mutation in the BRET2 tagged MBP protein. The half maximal effective concentration (EC50) was 0.37 mu M for maltose and the response was linear over almost three log units ranging from 10 nM to 3.16 mu M maltose for the BRET2 system compared to an EC50 of 2.3 mu M and a linear response ranging from 0.3 mu M to 21.1 mu M for the equivalent FRET-based biosensor. The biosensor's estimate of maltose in beer matched that of a commercial enzyme-linked assay but was quicker and more precise, demonstrating its applicability to real-world samples. A similar BRET2-based transduction scheme approach would likely be applicable to other binding proteins that have a "venus-fly-trap" mechanism. (C) 2012 Elsevier B.V. All rights reserved.
引用
收藏
页码:459 / 464
页数:6
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