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Cell Calcium. Author manuscript; available in PMC Jul 1, 2010.
Published in final edited form as:
PMCID: PMC2703684
NIHMSID: NIHMS110934
Store-operated Ca2+ influx and subplasmalemmal mitochondria
Marek K. Korzeniowski,a Gergö Szanda,b Tamas Balla,a and András Spätbc*
a Section on Molecular Signal Transduction, Program on Developmental Neuroscience, NICHD, NIH, Bethesda, MD, USA
b Dept. of Physiology, Semmelweis University, Budapest, Hungary
c Laboratory of Neurobiochemistry and Molecular Physiology, Hungarian Academy of Sciences, Budapest, Hungary
* Corresponding author: Phone: +36 20 825 4026. Fax: +36 1 266 7480., E-mail address: spat/at/puskin.sote.hu (A. Spät)
Calcium depletion of the endoplasmic reticulum (ER) induces oligomerisation, puncta formation and translocation of the ER Ca2+ sensor proteins, STIM1 and −2 into plasma membrane (PM)-adjacent regions of the ER, where they activate the Orai1, −2 or −3 proteins present in the opposing PM. These proteins form ion channels through which store-operated Ca2+ influx (SOC) occurs. Calcium ions exert negative feed-back on SOC. Here we examined whether subplasmalemmal mitochondria, which reduce this feed-back by Ca2+ uptake, are located within or out of the high-Ca2+ microdomains (HCMDs) formed between the ER and plasmalemmal Orai1 channels. For this purpose, COS-7 cells were co-transfected with Orai1, STIM1 labelled with YFP or mRFP and the mitochondrially targeted Ca2+ sensitive fluorescent protein inverse Pericam. Depletion of ER Ca2+ with ATP + thapsigargin (in Ca2+-free medium) induced the appearance of STIM1 puncta in the ≤100 nm wide subplasmalemmal space, as examined with TIRF. Mitochondria were located either in the gaps between STIM1-tagged puncta or in remote, STIM1-free regions. After addition of Ca2+ mitochondrial Ca2+ concentration increased irrespective of the mitochondrion-STIM1 distance. These observations indicate that mitochondria are exposed to Ca2+ diffused laterally from the HCMDs formed between the PM and the subplasmalemmal ER.
Keywords: mitochondria, calcium, store-operated calcium entry, STIM1
Inositol 1,4,5-trisphosphate-induced Ca2+ depletion of the ER induces Ca2+ influx from the extracellular space, a process originally termed as ‘capacitative Ca2+ influx’ [1]. This form of Ca2+ entry, presently more often referred to as store-operated Ca2+ influx (SOC) can also be induced by thapsigargin (Tg) [2] and other inhibitors of SERCA, the Ca. ATPase of the ER. The molecular basis of SOC has recently been unveiled by the discovery of two sets of proteins: STIM1 and −2, the Ca2+-sensor membrane proteins of the ER [35] and Orai1, −2 and −3, plasma membrane (PM) proteins forming Ca2+-selective channels [68]. Although additional channels may also be regulated by STIM proteins and contribute to SOC [911], STIM1 and Orai1 are necessary and sufficient components of the SOC mechanism in most cell types, including COS-7 cells examined in the present study. Upon depletion of ER luminal Ca2+, STIM1 undergoes sequential oligomerisation with ensuing formation of clusters and translocation into PM-adjacent regions within the ER [3,5,1214]. The STIM1 clusters in the ER induce multimerization of the plasmalemmal Orai1 molecules where the two molecules colocalise [1417] allowing a dramatic increase in SOC [18,19].
The role of mitochondria in the control of SOC has been suggested by several observations. Since elevation of cytosolic [Ca2+] ([Ca2+]c) exerts negative feed-back on SOC [20], Ca2+ sequestration by mitochondria will reduce this inhibition [2123]. This action of mitochondria requires an energized state but does not involve changes in intracellular ATP, indicating that it may be accounted for by Ca2+ uptake [24]. Indeed, SOC is more active in the vicinity of than far from subplasmalemmal mitochondria [25]. Also, sustained activity of SOC channels may require the translocation of mitochondria into subplasmalemmal regions [26].
Mitochondrial Ca2+ uptake occurs via the Ruthenium Red-sensitive Ca2+ uniporter, a highly selective inwardly rectifying channel that displays low affinity for Ca2+ [27]. However, mitochondrial Ca2+ sequestration does occur despite the low Ca2+ affinity of the uniporter during stimulation with a Ca2+ mobilising agonist. This is because of the rapidly forming but short-lived high-Ca2+ microdomains (HCMDs) between the mouth of IP3 receptor-channels and closely apposed mitochondria [28,29]. Mitochondrial Ca2+ uptake during voltage-operated Ca2+ influx has also been accounted for by the formation of HCMDs between the cytosolic mouth of the plasmalemmal channel and the apposing mitochondria [3033]. However, the formation of such HCMDs may not be an absolute requirement for mitochondrial Ca2+ uptake during SOC. Observations in glomerulosa, luteal, HeLa and H295R cells suggest that SOC may be followed by mitochondrial Ca2+ uptake without the need for HCMD [3438]. Therefore we examined whether subplasmalemmal mitochondria are in a location where SOC-induced HCMDs may be formed.
Cells
COS-7 cells were cultured on glass coverslips and transfected for 24 h with 0.5–0.5 μg plasmid DNA of Orai1 and mRFP-STIM1 and 1 μg mitochondrially-targeted inverse Pericam (i-Pericam) [39] per dish (~ 105 cells), using Lipofectamine 2000. Orai1 and STIM1 plasmids transcription was driven by the thymidine kinase (TK) promoter of the herpes simplex virus as described [14].
Confocal laser scanning microscopy
Confocal analysis was performed at 35°C in a modified Krebs-Ringer buffer containing (in mM): 120 NaCl, 4.7 KCl, 1.2 CaCl2, 0.7 MgSO4, 10 glucose, 10 sodium Hepes, pH 7.4, using a Zeiss LSM 510-META scanning confocal microscope and a 63x/1.4 objective. The optical slice was set at 1.5 μm. Data were acquired in multitrack mode with scanning in the frame mode using the 488 and 543 nm lasers and BP 505–545 and LP560 emission filters for YFP or mt-i-Pericam and Rhod-2 or mRFP, respectively.
Total internal reflection fluorescent microscopy (TIRF)
TIRF analysis was performed at room temperature in an Olympus through the lens dual launch TIRF microscope system equipped with a Hammamatsu EM-CCD camera and a PlanApo 60x/1.45 objective. 488 or 568 nm lasers and 535/40 and 645/75 emission filters were used for the mt-i-Pericam and mRFP, respectively. The Openlab Software (Improvision) was used for data acquisition, and the pictures were exported as TIFF files for processing with the Metamorph software (Molecular Devices). In some cases, the microscopic images were deconvoluted using a plugin (Iterative Deconvolve 3D) of ImageJ 1.37a.
Statistics
Statistical data are expressed as means ± S.E.M. For the evaluation of co-localisation of STIM1 puncta and subplasmalemmal mitochondria Pearson’s coefficient [40] was calculated after thresholding, applying a plugin of ImageJ 1.37a which excludes zero-zero pixels (Intensity Correlation Analysis). For curve fitting in Fig. 3 the spline/Lowess function of the Prism software was applied. Initial rate of Ca2+ -induced decrease in i-Pericam fluorescence in mitochondria close to or far from STIM1-labelled ER was compared with ANOVA.
Fig. 3
Fig. 3
TIRF analysis (performed at room temperature) of COS-7 cells expressing mRFP-STIM1, untagged Orai1 and inverse-Pericam-targeted to the mitochondrial matrix. (A) This recording (representative for 5 cells) was started after treatment of cells with ATP (more ...)
In order to enhance the active sites of SOC in COS-7 cells, Orai-1 and fluorescent protein-tagged STIM1 proteins were co-expressed. To achieve only moderate levels of expression, these constructs were driven by the thymidine kinase (TK) promoter [14]. The ER Ca2+ store was rapidly depleted by the addition of 50 μM ATP and 200 nM Tg to stimulate the endogenous metabotropic P2Y receptors and inhibit the SERCA Ca2+ pump, respectively. Ca2+ responses of the transfected cells in the cytosol and mitochondria were followed by confocal microscopy in regions of interest (ROIs) over the nucleus and over mitochondria, respectively, using the Ca2+ sensitive fluorescent dye Rhod-2. The rate and extent of the translocation of STIM1 towards the cell periphery was estimated off-line by measuring YFP fluorescence in ROIs over the perinuclear ER and puncta-rich periphery, respectively. As shown in Fig. 1, addition of ATP + Tg in the presence of external Ca2+, induced a rapid increase in [Ca2+]c that was associated with a moderate rise in mitochondrial [Ca2+] ([Ca2+]m). This reflected the rapid Ca2+ release from the ER. However, a second phase of the Ca2+ response was observed with a slight delay, which was much more pronounced in the mitochondria than in the cytosol (note the different scales of cytosolic and mitochondrial Rhod-2 signals on the y axes in Fig. 1B !). The onset of this secondary Ca2+ rise coincided with the translocation of STIM1 from the ER to the cell periphery and was, therefore, attributed to massive Ca2+ influx via the expressed Orai1 channels. Based on these data it may be assumed that mitochondria are capable of a significant sequestration of the inflowing Ca2+ and to some extent may protect the cytosol from very large [Ca2+]i increases.
Fig. 1
Fig. 1
Confocal image of a Rhod-2 loaded COS-7 cell transfected with TK-YFP-STIM1 and untagged Orai1. (A) Upper row: control, lower row: 5 min after the addition 50 μM ATP and 200 nM Tg in normal Ca2+ containing medium. Note the large increase in Rhod-2 (more ...)
In subsequent experiments the effects of Ca2+ depletion of the ER and increased Ca2+ influx on [Ca2+]m were studied with confocal- and TIRF microscopy, in order to determine whether the mitochondrial responses were dependent on the localization of the mitochondrion relative to that of STIM1. For this, cells were cotransfected with mRFP-STIM1 and a mitochondrially targeted inverse Pericam (i-Pericam) (Fig. 2). i-Pericam is a Ca2+ sensitive protein displaying high fluorescence intensity at low [Ca2+]m [39]. The application of i-Pericam was preferred over that of Rhod-2 because of its better suitability to detect mitochondria at low [Ca2+]m which was critical in subsequent TIRF experiments. In the resting state, mRFP-STIM1 showed its usual ER localization with some association with microtubules as described in several previous studies [41,42]. The mitochondria could easily be detected due to their high fluorescence at to low [Ca2+]m. Ca2+ depletion of the ER was induced with ATP + Tg in a Ca2+-free medium (containing 100 μM EGTA). Within 2 minutes of drug application, mRFP fluorescence became highly punctated indicating the formation of STIM1 clusters and enrichment in close proximity to the PM (Fig. 2A). Ca2+ influx was then initiated by the addition of 2 mM Ca2+ to the medium so that the effect of Ca2+ influx could be studied without Ca2+ release from the ER Ca2+ stores. Within 10 s after the addition of Ca2+, i-Pericam fluorescence rapidly decreased reflecting the SOC-evoked increase in [Ca2+]m (Fig. 2B). These experiments showed that i-Pericam is capable of reporting the rapid Ca2+ rise in the mitochondria associated with Ca2+ influx.
Fig. 2
Fig. 2
Confocal image of a COS-7 cell expressing mRFP-STIM1, untagged Orai1 and inverse-Pericam-targeted to the mitochondrial matrix. (A) Upper row: control, middle row: 2 min after stimulation with 50 μM ATP and 200 nM Tg in Ca2+-free medium (note the (more ...)
Next, the position of the mitochondria relative to the STIM1 puncta within the ≤100 nm wide subplasmalemmal space was examined with TIRF microscopy. After ER Ca2+ depletion by the addition of ATP + Tg (in a Ca2+-free medium containing 100 μM EGTA), mRFP-STIM1 puncta were detectable at the vicinity of the PM, and a few mitochondria showing i-Pericam fluorescence could also be located in this space. Importantly, the PM-close mitochondria showed no preferential localization close to the STIM1 puncta, but were found either in between the STIM1 patches or further away, in STIM1-free regions (Fig. 3A). Very few mitochondria could be detected contacting or at least partially overlapping with red fluorescing (mRFP) pixels. This was clearly demonstrable in pixel intensity profiles where pixels with high intensities in both green and red channels were very rarely detected. Colocalisation was also statistically estimated. Pearson’s coefficient which may change between +1 (colocalisation) and −1 (exclusion), was −0.750 ± 0.105 (means ± S.E.M.) in the original images and −0.912 ± 0.026 after deconvolution (n=5), confirming the lack of colocalisation of mRFP and i-Pericam.
Since Ca2+ influx probably saturates i-Pericam [39] the amplitude of mitochondrial Ca2+ response could not be accurately measured. Therefore we compared the initial rate of the fall of dye fluorescence (expressed as ΔF/Fo per second where Fo is F before adding Ca2+) in mitochondria far from ER (i.e. more than 10 pixels distance between the two organelles) and those close to ER. There was no statistical difference in the rates estimated for 12 far and 12 close mitochondria (selected in 3 cells) (p = 0.125). Similarly, no difference was observed when fluorescence intensities were expressed as per cent of max-min values (Fig. 3B). (These experiments were performed at room temperature to allow detection of small differences, therefore the Ca2+ response of mitochondria was somewhat slower than observed at 35 C.)
The relationship between mRFP-STIM1 and i-Pericam in ER-Ca2+-depleted cells was further evaluated with scatter plots. In Ca2+ depleted cells high i-Pericam fluorescence values (requiring good i-Pericam expression and low [Ca2+]m) were found in the low range of STIM1 fluorescence. Following readdition of Ca2+ the green fluorescence intensities of these pixels was drastically reduced, indicating that these pixels corresponded to functioning mitochondria capable of Ca2+ uptake (Fig. 4). The prominent fall of i-Pericam fluorescence across the spectrum of pixels with red fluorescence upon the induction of Ca2+ also confirmed the conclusion that mitochondria show equally good Ca2+ responses whether located in between STIM1 puncta or in remote, STIM1-free regions.
Fig. 4
Fig. 4
Scatter plot showing the fluorescence intensity of mitochondrially targeted i-Pericam (Y axis) as a function of the fluorescence intensity of STIM1-mRFP (X axis) in the cell shown in Fig. 3. Left panel: 9 min after Ca2+ depletion induced with ATP + Tg, (more ...)
Collectively, these results did not indicate the existence of preferential spatial positioning of mitochondria close to the STIM1/Orai1 formed Ca2+ entry sites. HCMDs is spatially and temporally defined local elevations of [Ca2+]c around the mouth of a Ca2+ release channel or a plasmalemmal Ca2+ channel. Its formation is allowed by a low diffusion rate of Ca2+ (due to immobile cytosolic Ca2+ buffers) and facilitated by a physical barrier for diffusion, the subplasmalemmal ER sites containing STIM1 puncta in our case. This way SOC-related HCMDs theoretically could be formed between Orai1 clusters and the apposing ER membrane rich in STIM1 puncta. Given the limited distance between the STIM1-labelled ER membrane and the Orai1 in the apposing PM, which was estimated to be in the range of 10–25 nm [14,43], this space is too narrow to accommodate a mitochondrion. Therefore, mitochondria may be exposed to Ca2+ diffusing only laterally from the HCMDs during SOC. This means that subplasmalemmal mitochondria are exposed to Ca2+ at concentrations probably exceeding that of the global cytosolic [Ca2+] increase. The nearer they are to the HCMDs formed around the orifice of Orai channels the higher [Ca2+] they are exposed to, but at least in non-excitable cells, even this local [Ca2+] may not attain the high values found in HCMDs close to the ER Ca2+ release sites. Whereas the estimated subplasmalemmal [Ca2+] values ranged between 20 and 300 μM in various excitable cells [4447] subplasmalemmal [Ca2+] amounted to only ~1.6 μM in the non-excitable endothelial cells [25]. Therefore in non-excitable cells the cell-type specific threshold of mitochondrial Ca2+ uptake (cf. [48]) rather than the position relative to the SOC site may determine to what an extent mitochondria can modify subplasmalemmal [Ca2+]c during SOC.
Acknowledgments
Mt-inverse Pericam was kindly gifted by Prof. A. Miyawaki (Saitama, Japan). The confocal imaging was performed at the Microscopy & Imaging Core of the National Institute of Child Health and Human Development, NIH with the kind assistance of Drs. Vincent Schram and James T. Russell. This research was supported in part by the Intramural Research Program of the National Institute of Child Health and Human Development of the National Institutes of Health.
Footnotes
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