Open Access
1 July 2010 Fluorescence imaging of membrane dynamics in living cells
Author Affiliations +
Abstract
Methods of wide-field fluorescence microscopy for measuring membrane dynamics of living cells are described, including spectral imaging as well as anisotropy imaging of the membrane marker 6-dodecanoyl-2-dimethylamino naphthalene (laurdan). Plasma membranes are selected by illumination with an evanescent electromagnetic field and distinguished from intracellular membranes assessed by whole-cell illumination. While fluorescence spectra of laurdan appeared red-shifted with decreasing membrane stiffness, fluorescence anisotropy and rotational correlation times were reduced with increasing membrane fluidity. Membrane stiffness was found to increase with decreasing temperature and increasing amounts of cholesterol and was always higher for the plasma membrane than for intracellular membranes. These effects may have some clinical relevance in the research of drug resistance or cell aging.

1.

Introduction

Membrane dynamics—including mechanical stiffness and exchange of lipid molecules (membrane fluidity)—has a large impact on cell function and may be an important factor for pathogenesis of, e.g., cancer1 or Alzheimer’s disease.2 An essential component of lipid bilayers is cholesterol, which determines its fluidity and rigidity. Membrane dynamics has so far been deduced from measurements of fluorescence polarization3 or fluorescence recovery after photobleaching (FRAP)4 using specific membrane markers. In addition, polarity-sensitive probes, e.g., 6-dodecanoyl-2-dimethylamino naphthalene (laurdan), whose electronic excitation energy is different in polar and nonpolar environments,5, 6 proved to be useful for membrane studies. Once incorporated into cell membranes, the fluorescence spectrum of laurdan shows a shift toward longer wavelengths when the laurdan molecules come into contact with adjacent water molecules of the cytoplasm, e.g., when membrane stiffness decreases or when a phase transition from the tightly packed gel phase to the liquid crystalline phase of membrane lipids occurs. Fluorescence maxima around 440nm and 490nm have been observed, so far, and the generalized polarization

Eq. 1

GP=(I440I490)(I440+I490),
has been defined as a parameter of membrane stiffness,7 with I440 corresponding to the fluorescence intensity at 440nm and I490 to that at 490nm .

In addition to fluorescence spectra, measurements of fluorescence anisotropy r can give valuable information about membrane dynamics according to

Eq. 2

r=(II)(I+2I),
with I and I corresponding to the fluorescence intensities with an electrical field vector parallel and perpendicular to the plane of incidence. The faster a molecule rotates between optical excitation and fluorescence, the lower is the expected value r . This value can be determined from steady state as well as from time-resolved fluorescence measurements. In the latter case, r(t) decays exponentially after short laser pulse excitation according to

Eq. 3

r(t)=(r0r)etτr+r,
with the initial value r0 , the limiting value r (observed at times that are long in comparison with the fluorescence lifetime and expressing that the rotational motion of a fluorophore may be hindered in one direction), and the rotational correlation time τr which is a direct measure of membrane viscosity.3

While conventional wide-field microscopy permits simultaneous measurements of different cell membranes—including the plasma membrane and various intracellular membranes—the plasma membrane can be examined selectively upon total internal reflection (TIR) of a laser beam8, 9 propagating through a medium of refractive index n1 (e.g., glass substrate) and meeting a second medium of refractive index n2<n1 (e.g., cell). Despite being totally reflected at all angles of incidence Θ that are greater than a critical angle Θc=arcsin (n2n1) , the incident beam establishes an evanescent electromagnetic field that penetrates into the second medium and decays exponentially with the distance z from the interface. According to the relation

Eq. 4

d=(λ4π)(n12sin2Θn22)12,
penetration depths d between about 60nm and more than 300nm are attained depending on the wavelength λ and the angle of incidence Θ .

The present paper reports on fluorescence microscopy of human U373-MG glioblastoma cells incubated with laurdan and presents spectral images and fluorescence anisotropy images upon variation of temperature as well as of the intracellular amount of cholesterol. Changes of cholesterol in cell membranes may affect protein interactions,10 e.g., in pathogenesis of Alzheimer’s disease,11, 12 and may have some influence on drug resistance13 as well as on cell aging.14 Plasma membranes illuminated selectively by TIR illumination are distinguished from intracellular membranes assessed by epi-illumination of whole cells.

2.

Materials and Methods

2.1.

Materials

U373-MG human glioblastoma cells were obtained from the European Collection of Cell Cultures (ECACC No. 89081403). Cells were routinely grown in RPMI 1640 medium supplemented with 10% fetal calf serum and antibiotics at 37°C and 5% CO2 . The hydrophobic membrane marker 6-dodecanoyl-2-dimethylamino naphthalene (laurdan) was obtained from Molecular Probes (Göttingen, Germany) and prepared as a 2mM Stock solution in ethanol. Water-soluble cholesterol and methyl- β -cyclodextrine (MβCD) were obtained from Sigma (Munich, Germany). After seeding of 150cellsmm2 , cells were grown on microscope object slides for 48h prior to rinsing with Earl’s balanced salt solution (EBSS) and incubation with laurdan (8μM) or coincubation with laurdan (8μM) and MβCD (4mM) or coincubation with laurdan (8μM) and a MβCD :cholesterol complex (0.63mM:0.1mM) diluted in culture medium without serum. Cholesterol depletion after application of MβCD as well as cholesterol enrichment after application of a MβCD :cholesterol complex are well documented in the literature.15 After incubation for 60min in each case, the intracellular amount of cholesterol was either reduced to about 50% (MβCD) or enriched to about 200% ( MβCD :cholesterol complex), as determined with an Amplex Red Cholesterol Assay Kit (Molecular Probes) and visualized by coupling of cholesterol to the antibiotic filipin (Sigma). After rinsing with EBSS, cells were measured in an open aluminum chamber at variable temperatures ranging from 16°Cto40°C using a 63×0.90 water immersion objective lens. This custom-made chamber (filled with a layer of 2to3mm EBSS) contained a Peltier element for heating or cooling, as well as a calibrated thermocouple for temperature measurements in close vicinity to the measured part of the samples.

2.2.

Experimental Setup

As depicted in Fig. 1 , a diode laser with high repetition pulses (LDH 400 with driver PDL 800-B, Picoquant, Berlin, Germany; wavelength: 391nm ; pulse energy: 12pJ ; pulse duration: 55ps ; repetition rate: 40MHz ; average power: 0.5mW ) was adapted to a fluorescence microscope (Axioplan 1, Carl Zeiss, Jena, Germany) using either a multimode fiber for epi-illumination of whole cells or a single-mode fiber-optic system (kineFlex-p-3-S-395, Point Source, Southampton, UK) together with a custom-made condenser unit16 for illumination of the plasma membrane and adjacent cellular sites under total internal reflection (TIR). Commonly, an angle of incidence Θ=67±0.5deg was used, permitting a penetration depth of the evanescent wave of about 120±20nm , if refractive indices n1=1.515 (glass substrate) and n2=1.37 (cytoplasm) are assumed. For anisotropy measurements, the electrical field vector was always polarized perpendicular to the plane of incidence. Fluorescence images were recorded by an electron multiplying (EM)–CCD camera with Peltier cooling and a sensitivity below 1016Wpixel (DV887DC, ANDOR Technology, Belfast, UK)17 in combination with appropriate spectral filters (bandpass filters for 454±20nm and 497±20nm used sequentially for spectral imaging or long-pass filter for λ420nm used for anisotropy imaging). For anisotropy imaging, two polarized fluorescence images (with an electrical field vector parallel and perpendicular to the plane of incidence) were generated by a polarization beamsplitter and detected simultaneously on different segments of the EM-CCD camera (Dual View, Optical Insights, Tucson, Arizona). Slight differences of sensitivity within the two detection paths were corrected by determination of the so-called G factor, i.e., the factor of fluorescence intensities measured within the two paths when in both cases the polarization of emission and excitation light was parallel. For additional measurements of fluorescence spectra, a custom-made polychromator together with an image-intensifying detection unit (IMD 4562, Hamamatsu Photonics, Ichino-Cho, Japan) was fixed on top of the microscope,18 whereas for measurements of the rotational correlation time, fluorescence decay kinetics was recorded with a time-gated image-intensifying camera (Picostar HR 12; LaVision, Göttingen, Germany) at a temporal resolution of 200ps (Ref. 19).

Fig. 1

Fluorescence microscope for spectral imaging or anisotropy imaging on TIR or epi-illumination. In some cases, the EM-CCD camera was replaced by a polychromator with an image-intensified detector or a time-gated image-intensifying camera.

046017_1_053004jbo1.jpg

3.

Results

3.1.

Spectral Imaging

The fluorescence spectrum of U373-MG glioblastoma cells incubated with laurdan is depicted in Fig. 2 together with the molecular structure of laurdan. All spectra are related to single cells either without further treatment (lower curve) or on enrichment of cholesterol (to about 200% of its natural amount; middle curve) or on cholesterol depletion (to about 50% of its natural amount; upper curve). While absolute fluorescence intensities varied from cell to cell up to a factor of about 2, the intensity ratio of the fluorescence bands around 440nm and 490nm increased with the amount of cholesterol. This finding can be described by an increase of the generalized polarization (GP) with increasing membrane stiffness according to Eq. 1.

Fig. 2

Fluorescence spectra of single U373-MG glioblastoma cells incubated with laurdan ( 8μM , 1h ) at a natural amount of cholesterol (lower curve) or on cholesterol enrichment (to 200%; middle curve) or cholesterol depletion (to 50%, upper curve) at T=24°C (whole cell illumination at λ=391nm ); molecular structure of laurdan.

046017_1_053004jbo2.jpg

GP values determined from fluorescence images recorded within both spectral bands are depicted in Fig. 3 as a function of the intracellular amount of cholesterol on illumination of whole cells [(a): epi-illumination] and plasma membranes [(c): TIR illumination]. Corresponding images of fluorescence intensity [(b), (d), recorded at λ420nm ] as well as a color scale for the GP values have been added. This figure proves the increasing GP values with increasing amounts of cholesterol and shows that GPs are always higher for the plasma membranes than for inner parts of the cells. This holds for all temperatures in the range 16°CT40°C , although GP decreases continuously with increasing temperature (data not shown).

Fig. 3

GP images [(a), (c); calculated according to Eq. 1] and corresponding fluorescence intensities [(b), (d); recorded at λ420nm ] of U373-MG glioblastoma cells incubated with laurdan as a function of intracellular cholesterol amount for whole cells [(a), (b): epi-illumination] and plasma membranes [(c), (d): TIR illumination] at T=24°C (image size: 140μm×140μm each); scale of GP values.

046017_1_053004jbo3.jpg

3.2.

Fluorescence Anisotropy Imaging

Polarized measurements of laurdan fluorescence in U373-MG glioblastoma cells always showed higher fluorescence intensity within the plane of the incident electrical field vector than perpendicular to this plane. In addition, time-resolved measurements after picosecond laser pulse excitation showed a fluorescence decrease with a lifetime around 5ns (Ref. 19) for both polarizations as well as some delayed increase for the polarization perpendicular to the plane of incidence.

Images of steady state anisotropy determined according to Eq. 2 are depicted in Fig. 4 for whole-cell illumination and in Fig. 5 for TIR illumination as a function of temperature and intracellular amount of cholesterol. These figures clearly show increasing anisotropies with increasing amounts of cholesterol and decreasing temperatures. In addition, anisotropy values are always higher for the plasma membranes (visualized as cell edges on epi-illumination and cell surfaces on TIR illumination) than for inner parts of the cells including the nuclear membrane. A similar result is obtained if instead of the fluorescence anisotropy r , the rotational correlation time τr is determined from fluorescence decay kinetics, as depicted in Fig. 6 . Again, τr decreases with temperature and increases with the amount of cholesterol (not shown) due to decreasing membrane viscosity in the first case and increasing viscosity in the second case. Obviously, the most pronounced change of τr occurs in the temperature range between 24°C and 32°C .

Fig. 4

Fluorescence anisotropy images of U373-MG glioblastoma cells incubated with laurdan as a function of temperature and intracellular cholesterol amount on whole-cell illumination (image size: 70μm×140μm each).

046017_1_053004jbo4.jpg

Fig. 5

Fluorescence anisotropy images of U373-MG glioblastoma cells incubated with laurdan as a function of temperature and intracellular cholesterol amount on TIR illumination (image size: 70μm×140μm each).

046017_1_053004jbo5.jpg

Fig. 6

Temperature dependence of the rotational correlation time of U373-MG glioblastoma cells incubated with laurdan on TIR (black bars: plasma membrane) and epi-illumination (gray bars: whole cell); median values±median absolute deviations (MADs) of 20 single-cell measurements in each case.

046017_1_053004jbo6.jpg

4.

Discussion

Several parameters characterizing membrane dynamics of living cells have been reported. While the generalized polarization (GP) of laurdan characterizes mechanical stiffness, the fluorescence anisotropy r and the rotational correlation time τr seem to characterize membrane viscosity or (inverse to viscosity) membrane fluidity. Obviously, similar information can be deduced from r and τr . GP on one hand and r as well as τr on the other hand show a pronounced decrease with temperature and an increase with the intracellular amount of cholesterol. This proves an inverse behavior of mechanical stiffness and fluidity of cell membranes. Experiments of staining cholesterol with fluorescent filipin showed that on cholesterol depletion with methyl- β -cyclodextrine (MβCD) , this depletion occurred primarily from inner parts of the cells, whereas comparably high cholesterol amounts were maintained in the plasma membranes.20 This explains their higher stiffness and lower fluidity in comparison with intracellular membranes.

A decrease of membrane stiffness with increasing temperature has been well documented for artificial membranes,5, 6, 7 but only in a few cases for living cells.21 While in artificial membranes, this decrease occurred in a small temperature interval (typically, around 40°C ), it occurred more gradually in a temperature range between about 15°C and 40°C for living cells. This is in good agreement with our own experiments and may be explained by the fact that several different membranes are expected to interfere.

It is of long-term interest to know how cholesterol may affect intermolecular interactions in cell membranes and whether it might favor or prevent pathogenesis of pathological processes. Just recently, we could show that enrichment as well as depletion of cholesterol could prevent interaction of amyloid precursor protein (APP) and β -secretase,12 which favors the production of amyloid peptide in the pathogenesis of Alzheimer’s disease. In addition, an influence of cholesterol on cell aging is well described in the literature14 and verified by our own experiments (not shown): Aging cells of subcultures 38–42 (i.e., cells split 38–42 times) were stiffer than cells of the subcultures 18–24 generally used for our experiments.

While fluorescence spectra5, 6, 7, 21, 22 and anisotropy22 measurements of laurdan have been well documented in the literature, only few imaging data of living cells are available so far.23, 24 Therefore, it was a main purpose of this paper to present spectral and anisotropy images of single cells and to compare laurdan fluorescence arising from plasma membranes with that arising from whole cells (and dominated by intracellular membranes). Switching of the illumination mode between total internal reflection (TIR) and epi-illumination is performed easily by two different illumination paths and a sliding mirror, as depicted in Fig. 1. TIR illumination with a hemispherical or hemicylindrical glass prism (Fig. 1) has further advantages in comparison with commercial TIR devices using high aperture objective lenses: easy variation of the penetration depth of the evanescent electromagnetic field by variation of the angle of incidence, and use of any kind of objective lens, even of rather low numerical aperture. This is essential for selection of larger object fields and for maintaining the polarization of light in fluorescence anisotropy measurements.

Imaging experiments profit to a large extent from the availability of highly sensitive EM-CCD cameras with excellent signal-to-noise ratio. Microscopic resolution in spectral and anisotropy imaging, however, is commonly limited by the Abbé criterion to about 200nm but can be improved to a few nanometers in the axial direction by variable-angle TIR microscopy.16 So, microdomains of different membrane stiffness or fluidity can be visualized down to diameters around 200nm , whereas cholesterol-enriched lipid rafts of only a few nanometers in size cannot be resolved.25 The excellent axial resolution, however, permits us to measure cholesterol-dependent cellular adhesions on a substrate in a nanometer scale, and loosening of those adhesions on depletion of cholesterol—finally leading to detachment of whole cells—has previously been well documented.26

Acknowledgments

The authors thank C. Hintze (Hochschule Aalen) for cell cultivation as well as P. Kruse and E. Winkler (ILM Ulm) for their support in quantitative measurements of cholesterol. Research was funded by the Bundesministerium für Bildung und Forschung (BMBF) and the Land Baden-Württemberg.

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©(2010) Society of Photo-Optical Instrumentation Engineers (SPIE)
Petra Weber, Michael Wagner, and Herbert Schneckenburger "Fluorescence imaging of membrane dynamics in living cells," Journal of Biomedical Optics 15(4), 046017 (1 July 2010). https://doi.org/10.1117/1.3470446
Published: 1 July 2010
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KEYWORDS
Luminescence

Plasma

Fluorescence anisotropy

Anisotropy

Polarization

Cameras

Microscopy

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