Respiration from activity of respiratory chain: redoxsensor green

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• Page authors: PRIMO
• Responsible curator: Hagen Buck-Wiese

RedoxSensor Green (RSG) is a cell-permeant, fluorogenic dye whose reduction is coupled to electron transport system (ETS) activity inside cells. Upon entering the cell, RSG is reduced by ETS enzymes to a highly fluorescent product that is retained intracellularly, and the resulting per-cell fluorescence intensity is proportional to respiration rate. Individual cells can then be analysed by flow cytometry or epifluorescence microscopy, enabling single-cell or population-level resolution of respiratory activity^[1].

Conversion from RSG fluorescence to absolute oxygen consumption requires calibration against a parallel Winkler or optode-based bulk respiration measurement from the same sample. The assay is performed in discrete mode on natural seawater samples with no pre-concentration step.

The method provides a single point measurement in space. Incubations are short (minutes to one hour), minimizing the time cells spend outside their natural environment. Single-cell resolution means that community-level heterogeneity in respiratory activity can be characterized.

Per-cell RSG fluorescence intensity, calibrated against bulk O₂ consumption, yields single-cell respiration rates in attomol O₂ cell^-1 h^-1. Community-level rates (µmol O₂ L^-1 h^-1) are obtained by multiplying single-cell rates by cell abundance. The distribution of per-cell rates across the population reveals the proportion of highly active vs. low-activity cells.

Units are amol O₂ cell^-1 h^-1 at the single-cell level, or µmol O₂ L^-1 h^-1 for community-level estimates. The currency is oxygen.

Typical samples are < 1 L in volume.

RSG fluorescence is assumed to be proportional to respiratory rate across the range of physiological states encountered in the environment. In practice, cell membrane permeability — which governs RSG uptake — varies with the physiological state of individual cells, potentially biasing estimates in cells with compromised membranes or altered membrane potential. It is not established whether all active cells in a natural community incorporate RSG equally. The calibration step (linking fluorescence to O₂ consumption via Winkler) introduces uncertainty from the assumption that the calibration applies across the diversity of cell types and physiological states in the sample.

• Kalyuzhnaya et al. (2008) Real-time detection of actively metabolizing microbes by redox sensing as applied to methylotroph populations in Lake Washington ^[1]

• Munson-McGee et al. (2022) Decoupling of respiration rates and abundance in marine prokaryoplankton ^[2]

• Community respiration (µmol O₂ L^-1 h^-1) = mean RSG fluorescence per cell × cell abundance × calibration factor (from parallel Winkler measurement).