Search Thermo Fisher Scientific
Search Thermo Fisher Scientific
There are two major prerequisites for measuring intracellular ion concentrations using fluorescent indicators:
This technical note focuses on these prerequisites. Further information on the practical aspects of ion measurements using fluorescent indicators can be found in several reviews.
Cell loading methods can be divided into two groups. Bulk loading procedures are applicable to large populations of cells and include:
Procedures such as microinjection and infusion from whole-cell patch pipettes must be carried out one cell at a time. Reviews of some of these techniques have been published; see also Techniques for loading molecules into the cytoplasm—Table 14.1 (Choosing a Tracer—Section 14.1).
The noninvasive and technically straightforward AM ester technique is by far the most popular method for loading fluorescent ion indicators (Figure 1). The carboxylate groups of indicators for Ca2+ and other cations and the phenolic hydroxyl groups of pH indicators are derivatized as acetoxymethyl or acetate esters, respectively, rendering the indicator permeant to membranes and insensitive to ions. Once inside the cell, these derivatized indicators are hydrolyzed by ubiquitous intracellular esterases, releasing the ion-sensitive polyanionic indicator.
In practice, a 1–10 mM stock solution of the ester probe in anhydrous dimethylsulfoxide (DMSO) is prepared and divided into appropriately sized aliquots that can be stored desiccated at –20°C. This procedure will curtail the spontaneous ester hydrolysis that can occur in moist environments. Before loading, the DMSO stock solution should be diluted at least 1:200 in serum-free culture medium to a final concentration of about 1–10 µM. The nonionic and nondenaturing detergent Pluronic F-127 or the related PowerLoad reagent (P3000MP, P6866, P6867, P10020; Chelators, Calibration Buffers, Ionophores and Cell-Loading Reagents—Section 19.8) are frequently added to help disperse the indicator in the loading medium. After incubation at 20–37°C for 15–60 minutes, the cells should be washed two to three times with fresh serum-free culture medium (serum may contain esterase activity). The loading medium should also be free of amino acids or buffers containing primary or secondary amines because aliphatic amines may cleave the AM esters and prevent loading. The overall loading efficiency is typically 10–40%, depending on the molecular structure of the indicator, the type of cells and the incubation conditions.
Figure 1. Schematic diagram of the processes involved in loading cells using membrane-permeant acetoxymethyl (AM) ester derivatives of fluorescent indicators, in this case fura-2. Note the generation of potentially toxic by-products (formaldehyde and acetic acid).
The dissociation constant (Kd) is the key conversion parameter linking fluorescence signals to ion concentrations, assuming that the indicator is operating as an equilibrium sensor. This conventional assumption requires that the concentration of the indicator is close to the Kd value. Because intracellular indicator concentrations can easily reach 10–100 µM, even if the externally applied concentration is only 1–10 µM, this assumption is not always valid. For pH indicators, Kd is conventionally expressed as its negative log (pKa). The concentration range over which an indicator produces an observable response is approximately 0.1 × Kd to 10 × Kd. For ratiometric measurements, the response range also depends on wavelength-dependent parameters. For BAPTA-based Ca2+ indicators in particular, the Kd is very sensitive to a number of environmental factors, including temperature, pH, ionic strength and interactions of the indicator with proteins. Examination of published data shows that values of Kd determined in situ within cells can be up to fivefold higher than values determined in vitro (Comparison of in vitro and in situ Kd values for various Ca2+ indicators—Table 19.2), underscoring the importance of performing calibrations to determine the Kd directly in the system under study.
Calibration procedures basically consist of recording fluorescence signals corresponding to a series of precisely manipulated ion concentrations. The resulting sigmoidal titration curve is either linearized by means of a Hill plot or analyzed directly by nonlinear regression to yield Kd. For in vitro calibrations of Ca2+ indicators, EGTA buffering is widely used to produce defined Ca2+ concentrations that can be calculated from the Kd of the Ca2+-EGTA complex. This technique is used in the Calcium Calibration Buffer Kits (Chelators, Calibration Buffers, Ionophores and Cell-Loading Reagents—Section 19.8). In situ calibrations of intracellular indicators generally utilize an ionophore to equilibrate the controlled external ion concentration with the ion concentration within the cell. Commonly used ionophores include:
Indicators that show an excitation or emission spectral shift upon ion binding can be calibrated using a ratio of the fluorescence intensities measured at two different wavelengths, resulting in the cancellation of artifactual variations in the fluorescence signal that might otherwise be misinterpreted as changes in ion concentration (Figure 2). Note that background levels must be subtracted from the component fluorescence intensities before calculation of the ratio. Examples of indicators exhibiting ion-dependent spectral shifts include the Ca2+ indicators fura-2 (Figure 3) and indo-1 (Fluorescent Ca2+ Indicators Excited with UV Light—Section 19.2), and the pH indicators BCECF and SNARF-1 (Probes Useful at Near-Neutral pH—Section 20.2). The ratio of two intensities with opposite ion-sensitive responses (for example, 340 nm/380 nm in Figure 3) gives the largest possible dynamic range of ratio signals for a particular indicator. Alternatively, the ratio of an ion-sensitive intensity to an ion-insensitive intensity (measured at a spectral isosbestic point, e.g., 360 nm in Figure 3) can be used (Figure 2). Ratiometric measurements reduce or eliminate variations of several determining factors in the measured fluorescence intensity, including indicator concentration, excitation path length, excitation intensity and detection efficiency. Artifacts that are eliminated include photobleaching and leakage of the indicator, variable cell thickness, and nonuniform indicator distribution within cells (due to compartmentalization) or among populations of cells (due to loading efficacy variations).
Figure 2. Simulated data demonstrating the practical importance of ratiometric fluorescence techniques. This figure represents an ion indicator that exhibits a fluorescence intensity increase in response to ion binding at wavelength λ1 and a corresponding decrease at λ3. Fluorescence measured at an isosbestic point (λ2) is independent of ion concentration. The intracellular indicator concentration diminishes rapidly due to photobleaching, leakage (assuming the extracellular indicator is not detectable) or some other process. The change of intracellular ion concentration due to a stimulus applied at the time indicated by the arrow is unambiguously identified by recording the fluorescence intensity ratios λ1/λ3 or λ1/λ2. |
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