Design and study of the efflux function of the EGFP fused MexAB-OprM membrane transporter in Pseudomonas aeruginosa using fluorescence spectroscopy

Ding, Feng; Lee, Kerry J.; Vahedi-Faridi, A.; Yoneyama, Hiroshi; Osgood, C.; Xu, Xiao

doi:10.1039/c4an00108g

Cited by 9 publications

(19 citation statements)

References 56 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Thus, the PBS buffer (but not cell culture medium) was used to suspend the bacterial cells for the study of accumulation kinetics of pump substrates over time, as those reported previously. 14, 15, 24, 25, 33, 35, 37 Note that the cells would grow in the culture medium, and the number of the cells would change over time, making the study of the accumulation rates of single NPs in the cells over time impossible. Our studies demonstrate that the bacterial cells remain alive and retain their efflux functions in the PBS buffer, as shown in Figs.…”

Section: Methodsmentioning

confidence: 99%

See 1 more Smart Citation

Single nanoparticle plasmonic spectroscopy for study of the efflux function of multidrug ABC membrane transporters of single live cells

et al. 2016

Self Cite

View full text Add to dashboard Cite

ATP-binding cassette (ABC) membrane transporters exist in all living organisms and play key roles in a wide range of cellular and physiological functions. The ABC transporters can selectively extrude a wide variety of structurally and functionally unrelated substrates, leading to multidrug resistance. Despite extensive study, their efflux molecular mechanisms remain elusive. In this study, we synthesized and characterized purified silver nanoparticles (Ag NPs) (97 ± 13 nm in diameter), and used them as photostable optical imaging probes to study efflux kinetics of ABC membrane transporters (BmrA) of single live cells (B. subtillis). The NPs with concentrations up to 3.7 pM were stable (non-aggregated) in a PBS buffer and biocompatible with the cells. We found a high dependence of accumulation of the intracellular NPs in single live cells (WT, Ct-BmrA-EGFP, ΔbmrA) upon the cellular expression level of BmrA and NP concentration (0.93, 1.85 and 3.7 pM), showing the highest accumulation of intracellular NPs in ΔbmrA (deletion of BmrA) and the lowest ones in Ct-BmrA-EGFP (over-expression of BmrA). Interestingly, the accumulation of intracellular NPs in ΔbmrA increases nearly proportionally with the NP concentration, while those in WT and Ct-BrmA-EGFP do not. This suggests that the NPs enter the cells via passive diffusion driven by concentration gradients and are extruded out of cells by BmrA transporters, similar to conventional pump substrates (antibiotics). This study shows that such large substrates (84-100 nm NPs) can enter into the live cells and be extruded out of the cells by BmrA, and the NPs can serve as nm-sized optical imaging probes to study the size-dependent efflux kinetics of membrane transporters in single live cells in real time.

show abstract

Section: Methodsmentioning

confidence: 99%

“…9-15 These conventional methods enable one to study ensemble accumulation kinetics of bulk cells. We have also demonstrated that thin-layer total-internal reflection fluorescence microscopy and spectroscopy can be used to measure efflux kinetics of single membrane transporters of single live cells in real-time.…”

Section: Introductionmentioning

confidence: 99%

Single nanoparticle plasmonic spectroscopy for study of the efflux function of multidrug ABC membrane transporters of single live cells

et al. 2016

Self Cite

View full text Add to dashboard Cite

show abstract

Section: Methodsmentioning

confidence: 99%

“…14–15, 18–19, 29, 61 The previous studies have showed that the bacterial cells in the PBS buffer retain their efflux function over hours. 14–15, 18–19, 29, 61 Notably, the bacterial cells suspended in the PBS buffer retain their cellular growth stage and cellular function over hours, and their number remains the same over time. 14–15, 18–19, 29, 61 Therefore, in order to use the same growth stage and number of the cells over the duration of each experiment (2 h), it is essential to study the accumulation rates of the NPs in the cells that are suspended in the PBS buffer, but not in the cell culture medium which would lead to the cell growth and creation of the cells with various growth stages and functions.…”

Section: Methodsmentioning

confidence: 99%

Single Nanoparticle Plasmonic Spectroscopy for Study of Charge-Dependent Efflux Function of Multidrug ABC Transporters of Single Live Bacillus subtilis Cells

et al. 2016

Self Cite

View full text Add to dashboard Cite

Multidrug membrane transporters can selectively extrude a wide variety of structurally and functionally unrelated substrates, and they are responsible for ineffective treatment of a wide range of diseases (e.g., infection and cancer). Their underlying molecular mechanisms remain elusive. In this study, we functionalized Ag NPs (11 nm in diameter) with two biocompatible peptides (CALNNK, CALNNE) to prepare positively and negatively charged Ag-peptide NPs (Ag-CALNNK NPs+ζ, Ag-CALNNE NPs−4ζ), respectively. We used them as photostable plasmonic imaging probes to study charge-dependent efflux kinetics of BmrA (ABC) membrane transporter of single live Bacillus (B.) subtilis cells. Two strains of the cells, normal expression of BmrA (WT) or devoid of BmrA (ΔBmrA), were used to study the charge-dependent efflux kinetics of single NPs upon the expression of BmrA. The NPs (1.4 nM) were stable (non-aggregated) in a PBS buffer and biocompatible to the cells. We found the high dependent accumulation of the intracellular NPs in both WT and ΔBmrA upon the charge and concentration of NPs. Notably, the accumulation rates of the positively charged NPs in single live WT cells are nearly identical to those in ΔBmrA cells, showing independence upon the expression of BmrA. In contrast, the accumulation rates of the negatively charged NPs in WT are much lower than in ΔBmrA, showing high dependence upon the expression of BmrA and suggesting that BmrA extrude the negatively charged NPs, but not positively charged NPs, out of the WT. The accumulation of positively charged NPs in both WT and ΔBmrA increases nearly proportionally to the NP concentration. The accumulation of negatively charged NPs in ΔBmrA, but not in WT, also increases nearly proportionally to the NP concentration. These results suggest that both negatively and positively charged NPs enter the cells via passive diffusion driven by concentration gradients across the cellular membrane, and BmrA can only extrude the negatively charged NPs out of the WT. This study shows that single NP plasmon spectroscopy can serve as a powerful tool to identify single plasmonic NPs and to probe the charge-dependent efflux kinetics and function of single membrane transporters in single live cells in real time.

show abstract

“… 61 − 66 Some literature has also reported the changes in the biological property of the sample after fluorescence labeling. 67 , 68 Similarly, the radio ligand binding assay 69 produces toxic radioactive wastes which are extremely harmful to in vivo studies. Although the above-mentioned techniques are useful to screen the binding specificity of signaling molecules such as drugs and neurotransmitters, they suffer from some serious limitations.…”

Section: Introductionmentioning

confidence: 99%

Raman Spectroscopic Analysis of Signaling Molecules–Dopamine Receptors Interactions in Living Cells

Silwal

2018

ACS Omega

View full text Add to dashboard Cite

The selective interaction of signaling compounds including neurotransmitters and drugs with the dopamine receptors (DARs) is extremely important for the treatment of neurodegenerative diseases. Here, we report a method to probe the selective interactions of signaling compounds with D1 and D2 DARs in living cells using the combined approach of theoretical calculation and surface-enhanced Raman spectroscopy (SERS). When signaling compounds such as DA, amphetamine, methamphetamine, and methylenedioxypyrovalerone interact with D1 dopamine receptors (DRD1), the intracellular cyclic adenosine monophosphate (cAMP) level is increased. However, the intracellular level of cAMP is decreased when D2 dopamine receptors (DRD2) interact with the abovementioned signaling compounds. In our experiments, we have internalized the silica-coated silver nanoparticles (AgNP@SiO2) in living cells to adsorb biologically generated cAMP which was probed by using SERS. Besides adsorptions of cAMP, AgNP@SiO2 has a crucial role for the enhancement of Raman cross section of the samples. We observed the characteristic SERS peaks of cAMP when DRD1-overexpressed cells interact with the signaling compounds; these peaks were not observed for other cells including DRD2-overexpressed and DRD1–DRD2-coexpressed cells. Our experimental approach is successful to probe the intracellular cAMP and characterize the selectivity of signaling compounds to different types of DARs. Furthermore, our experimental approach is highly capable for in vivo studies because it can probe intracellular cAMP using a low input power of incident laser without significant cell damage. Our experimental results and density functional theory calculations showed that 780 and 1503 cm–1 are signature Raman peaks of cAMP. The SERS peak at 780 cm–1 is associated with C–O, C–C, and C–N stretching and symmetric and asymmetric bending of two O–H bonds of cAMP, whereas the SERS peak at 1503 cm–1 is contributed by the O9–H3 bending mode.

show abstract

Design and study of the efflux function of the EGFP fused MexAB-OprM membrane transporter in Pseudomonas aeruginosa using fluorescence spectroscopy

Cited by 9 publications

References 56 publications

Single nanoparticle plasmonic spectroscopy for study of the efflux function of multidrug ABC membrane transporters of single live cells

Single nanoparticle plasmonic spectroscopy for study of the efflux function of multidrug ABC membrane transporters of single live cells

Single Nanoparticle Plasmonic Spectroscopy for Study of Charge-Dependent Efflux Function of Multidrug ABC Transporters of Single Live Bacillus subtilis Cells

Raman Spectroscopic Analysis of Signaling Molecules–Dopamine Receptors Interactions in Living Cells

Contact Info

Product

Resources

About