Department of Human Genetics, University of California, Los Angeles, CA 90095, USA
* Author for correspondence (e-mail: edellangelica{at}mednet.ucla.edu)
Accepted 12 August 2005
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Summary |
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Key words: Lysosomes, Endosomes, Microtubules, Time-lapse microscopy, Hermansky-Pudlak syndrome
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Introduction |
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The perinuclear steady-state distribution of lysosomes has been shown to reflect a balance between long-range vectorial movement towards the plus and minus ends of microtubules as well as short-range movement on actin filaments (Matteoni and Kreiss, 1987; Taunton et al., 2000
; Cordonnier et al., 2001
). Molecular motors implicated in the movement of lysosomes (and probably of late endosomes) include dynein and its associated dynactin complex (for movement towards the minus end of microtubules), kinesin superfamily members such as KIF2ß and KIF1Bß3 (for microtubule-dependent movement towards the cell periphery) and myosin I
(for movement on actin filaments) (Burkhardt et al., 1997
; Harada et al., 1998
; Santama et al., 1998
; Valetti et al., 1999
; Cordonnier et al., 2001
; Matsushita et al., 2004
). Other factors include: Rab7 and its effector, Rab7-interacting lysosomal protein, which regulate attachment of late endocytic organelles to dynactin/dynein (Jordens et al., 2001
); and MLN64, which regulates attachment of these organelles to actin filaments (Hölttä-Vuori et al., 2005
). Interference with the function of these proteins, either by loss-of-function or overexpression approaches, has been reported to modify the steady-state distribution of late endosomes and lysosomes, as inferred from fluorescence microscopic analyses (Burkhardt et al., 1997
; Harada et al., 1998
; Santama et al., 1998
; Valetti et al., 1999
; Bucci et al., 2000
; Cantalupo et al., 2001
; Cordonnier et al., 2001
; Matsushita et al., 2004
; Hölttä-Vuori et al., 2005
).
We (Nazarian et al., 2003) and others (Chiang et al., 2003
; Martina et al., 2003
) have described a stable protein complex, named BLOC-3 (for `biogenesis of lysosome-related organelles complex 3), which is expressed ubiquitously and contains the products of the HPS1 and HPS4 genes mutated in Hermansky-Pudlak syndrome (HPS) types 1 and 4, respectively. HPS is a group of autosomal recessive disorders involving defects in lysosome-related organelles (reviewed by Di Pietro and Dell'Angelica, 2005
). Common to all forms of HPS are albinism and bleeding diathesis, resulting from abnormalities in melanosomes and platelet dense granules, respectively. Patients suffering from HPS-1 and HPS-4 are at risk of developing progressive pulmonary fibrosis, which might arise from defects in another lysosome-related organelle, the lamellar body of type II lung epithelial cells. A mild form of ceroid lipofuscinosis has also been described for HPS type 1 patients, suggesting that lysosomal degradative function might be compromised (reviewed by Gunay-Aygun et al., 2004
). The murine orthologs of human HPS1 and HPS4 are mutated in the pale ear and light ear strains, respectively, which serve as bona fide models of the disease (Li et al., 2004
). Using immortalized fibroblasts derived from the skin of these mutant mice, we observed relatively reduced percentages of cells displaying pronounced perinuclear distribution at steady-state of markers of late endosomes (lysobisphosphatidic acid), lysosomes (internalized dextran), or both (Lamp1). Colocalization experiments indicated that the observed differences were unlikely to be owing to protein missorting, suggesting that BLOC-3 might regulate the movement/distribution of late endosomes and lysosomes (Nazarian et al., 2003
).
In this work, we sought to develop a quantitative method to estimate the extent of organelle clustering at the perinuclear region of the cell, which has so far relied on intrinsically subjective approaches. We applied this method to the analysis of Lamp1-positive organelles in mutant fibroblasts deficient in BLOC-3 as well as in BLOC-1 or BLOC-2, another two protein complexes associated with HPS (Di Pietro and Dell'Angelica, 2005). We also performed time-lapse microscopic experiments on live cells expressing human LAMP1 fused to green fluorescence protein (GFP), to test the hypothesis that BLOC-3 plays a role in the regulation of the movement of late endocytic organelles. During the course of these experiments, we observed that high levels of LAMP1-GFP overexpression can elicit organelle aggregation, and examined the possible mechanism of this phenomenon.
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Materials and Methods |
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DNA constructs
To generate an expression plasmid encoding the LAMP1-GFP fusion protein, the complete open-reading frame of human LAMP1 (GenBank accession number XM_052636) and portions of the 5' and 3' untranslated regions were amplified by reverse-transcriptase PCR from total RNA purified from MEG-01 cells using the TRIzol reagent. The product was purified and used as template for nested PCR using primers designed to append an EcoRI site upstream of the Kozak sequence and to replace the translation termination site by a segment encoding the linker sequence GSTGSTGSTGA (single-letter amino acid code) followed by a SalI site. The nested PCR product was gel purified and cloned in the EcoRI-SalI sites of the pEGFP-N3 vector (BD Biosciences Clontech). A variant construct expressing LAMP1-mGFP, in which the leucine residue at position 221 of the GFP domain was replaced by lysine to avoid anti-parallel dimerization (Zacharias et al., 2002), was generated by site-directed mutagenesis using the QuickChange XL kit (Stratagene). Constructs were verified by DNA sequencing.
Cell culture, transfection and dextran internalization
The generation and culture conditions of immortalized fibroblast lines derived from the skin of wild-type (C57BL/6J), pale ear (B6.C3Fe-Hps1ep/J), pallid (B6.Cg-Pldnpa/J) and cocoa (B6.B10-Hps3coa/J) mice were described previously (Nazarian et al., 2003; Di Pietro et al., 2004
). Transient transfection using FuGENE 6 and labeling of lysosomes through internalization of Texas-Red-conjugated dextran were performed as described (Nazarian et al., 2003
).
For stable transfection, murine fibroblasts were grown at 37°C in complete DMEM [Dulbecco's modified Eagle medium supplemented with 20% (v/v) fetal bovine serum, 2 mM glutamine, 0.1 mg/ml streptomycin and 100 units/ml penicillin] to 60-70% confluency, and subsequently transfected with the LAMP1-GFP-encoding plasmid using FuGENE 6 in serum-free DMEM. The medium was changed to complete DMEM 5 hours after transfection, and to complete DMEM containing 2 g/l G418 one day later. Cells displaying resistance to G418 and expressing LAMP1-GFP (as judged by fluorescence microscopy) were cloned by limiting dilution and, in the cases of one line derived from wild-type fibroblasts and one line derived from pale ear fibroblasts, by preparative cell sorting on a BD FACSVantage SE flow cytometer (Becton Dickinson).
Fluorescence microscopy of fixed cells
Immunofluorescence staining of fixed/permeabilized cells was carried out as described (Dell'Angelica et al., 1997). The samples were examined on a Zeiss Axioskop 2 microscope equipped with an Orca-ER digital camera (Carl Zeiss) or, for analyses requiring high optical resolution (e.g. colocalization experiments), on a Leica TCS SP multiphoton confocal microscope (Leica).
Determination of perinuclear clustering index
Fixed/permeabilized fibroblasts from wild-type, pallid, cocoa and pale ear mice (three independent cell lines per strain) were stained using rat monoclonal antibody 1D4B against endogenous murine Lamp1, followed by Cy3-conjugated secondary antibody against rat IgG. Digital images (1344x1024 pixels, 8 bits per pixel) of randomly selected cells were acquired on a Zeiss Axioskop 2 microscope equipped with an Orca-ER digital camera, using a 40x objective and appropriate filters. Two images were acquired for each selected microscopic field; one was obtained under conditions optimized to prevent signal saturation, and the other was overexposed to facilitate delimitation of the cell perimeter. The images were saved as TIFF files using coded file names, to ensure that the person(s) involved in subsequent image analysis could readily recognize which two files corresponded to the optimal and overexposed versions of each image but could not establish the identity of the cell line. Images were imported into NIH Image 1.62, using the Stacks option to align each pair of optimal and overexposed images. For each cell in the image, the perimeter of the whole cell (C) and that of the nucleus (N) were drawn by an operator (see, for example, Fig. 1A,B). Although drawing of these two perimeters was based on the overexposed version of the image, all calculations were performed using the optimal version. Additional areas, including the nucleus and part of the perinuclear region of the cell (nucleus + perinuclear, or NP), were delimited according to the following rules: (1) it must completely include the area delimited as the nucleus; (2) it must not extend outside the cell; and (3) its shape should maximize inclusion of Lamp1 staining signal (for example, see Fig. 1C). For each delimited region, its size (S, in pixels) and mean fluorescence intensity (F, in arbitrary units) were measured, and multiplication of these two values allowed calculation of the total fluorescence signal of the region. To calculate the uncorrected mean fluorescence intensity of the perinuclear (or cytoplasmic) regions, the total fluorescence signal of the N region was subtracted from that of the NP region (or of the C region), and the resulting value was divided by the size of NP (or of C) minus the size of N. A background mean fluorescence intensity, FB, was measured from areas delimited at random places outside the cells and subtracted from the uncorrected mean fluorescence intensity values of the perinuclear and cytoplasmic regions. Hence, the perinuclear/cytoplasmic Lamp1 staining ratio (R) was calculated using the following equation:
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Time-lapse fluorescence microscopy
Fibroblasts were grown on glass-bottomed culture dishes (Mattek). Initial analyses of the dynamics of late endosomes and lysosomes were carried out using wild-type and mutant fibroblast lines stably expressing LAMP1-GFP, and subsequent experiments were performed using fibroblasts that had been transiently transfected to express LAMP1-GFP or LAMP1-mGFP. In all cases, cells expressing low levels of the fusion protein, as judged by GFP fluorescence, were selected for imaging. To prepare cell samples for the analysis of lysosome dynamics, cells were first incubated for 8 hours in complete DMEM containing 0.5 g/l BODIPY-FL-conjugated dextran, transferred to glass-bottomed culture dishes, and incubated for another 12 hours in complete DMEM lacking dextran, at 37°C in a tissue culture incubator.
For acquisition of time-lapse fluorescence images, the medium was changed to complete DMEM lacking Phenol Red and containing 25 mM Hepes buffer (pH 7.4), and the glass-bottomed culture dishes were placed on the heating stage of a Leica DM-IRBE inverted microscope equipped with a 100x objective and Orca-ER digital camera, and controlled by SlideBook software (Intelligent Imaging Innovations, Denver, CO). The temperature of the sample was set to 35°C. In typical experiments, images were acquired every 2 seconds for 98 seconds, and pixel size was equivalent to 0.39x0.39 µm. In some experiments, cells were pre-incubated for at least 90 minutes in the presence of 30 µM nocodazole to disrupt microtubules.
For quantitative analysis of time-lapse experiments, 30 fluorescent organelles per cell were selected at random among those that were not in overcrowded regions of the initial frame image, and their positions determined in each subsequent frame by manual tracking. Because several organelles changed their shape during movement, their position was calculated as the center of mass of the fluorescence signal. The two-dimensional displacement between consecutive frames was calculated from the changes in X and Y position coordinates, using Pitagora's equation (changes in Z position were considered negligible due to the flat extended shape of the cells). For each organelle, the following values were calculated as defined: maximum speed (in µm/second) was defined as the highest value of speed (displacement divided by time) obtained between two consecutive frames; effective distance (in µm) was defined as the maximum distance between any two positions of the trajectory during the 98-second period; average speed on microtubules (in µm/second) was defined as the arithmetic average of all speed values between consecutive frames that were equal or larger than 0.78 µm/second; percentage of time at speed 0.78 µm/second was defined as the percentage of the 2-second intervals between frames in which the displacement was equal or larger than 1.56 µm; number of events with speed increasing to
0.78 µm/second was defined as the number of times within 98 seconds in which a 2-second interval with speed <0.78 µm/second was followed by another interval with speed
0.78 µm/second; and duration of events with speed
0.78 µm/second (in seconds) was defined as the arithmetic average of the duration of series of consecutive 2-second intervals with speed
0.78 µm/second.
Statistical analyses
Statistical analysis of the PCI data was performed using one-way ANOVA followed by a posteriori Tukey's test, considering each average value per cell line (out of 20 randomly selected cells) an independent observation. For the analysis of data derived from time-lapse microscopic experiments, each median value per cell (out of 30 randomly selected organelles) was considered an independent observation. Ten cells were analyzed per cell line, and three (for LAMP1-GFP) or two (for LAMP1-mGFP) independent cell lines were analyzed per murine strain (wild-type or pale ear). The maximum speed, effective distance and average speed on microtubules data were analyzed using an ANOVA model upon logarithmic transformation (to make the assumption of Gaussian distributions appropriate). For the analysis of the percentage of time at speed 0.78 µm/second and the number of events with speed increasing to
0.78 µm/second data, the odds of obtaining zero as the median value per cell were compared using Fisher's exact test. The duration of events with speed
0.78 µm/second data was analyzed using both Kolmogorov-Smirnov test and Fisher's exact test.
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Results |
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We focused our analysis on late endosomes and lysosomes labeled with endogenously expressed Lamp1, which we previously reported to be relatively less concentrated in the perinuclear region of BLOC-3-deficient fibroblasts as inferred from reduced percentages of cells displaying pronounced perinuclear accumulation (Nazarian et al., 2003). Our approach consisted of estimating the concentration gradient of Lamp1 staining from determinations of the perinuclear/cytoplasmic staining ratio as a function of the relative size of the perinuclear region. We obtained digital images of Lamp1-stained cells under conditions in which the whole cell was included (i.e. low magnification and no optical sectioning) and the fluorescence signal intensities were within the dynamic range of the digital camera. To avoid bias in our analysis, the cells were randomly picked for imaging, and the resulting images were processed following a `blinded' approach in which the operator was unaware of the sample identity.
Our attempts to develop an algorithm for fully automatic analysis of the images were hampered by the high variability in size and shape, not only of whole cells but also of their perinuclear regions. As an alternative, we chose to have an operator delimiting by hand (with the aid of a computer mouse) the whole cell (Fig. 1A), the nucleus (Fig. 1B) and a third area including the nucleus and part of the perinuclear region (Fig. 1C). Whereas definition of the first two regions was straightforward, the third was more problematic because we could not fit satisfactorily any simple geometrical shape to the NP region of most cells. Instead, the operator was allowed to delimit areas of any shape, with the main restriction that inclusion of Lamp1 staining should be maximized (e.g. see Fig. 1C). From each area we measured its size and mean fluorescence intensity, and using Equation 1 we calculated the perinuclear/cytoplasmic ratio of Lamp1 staining. As expected, this value was highly dependent on the relative size of the NP region area and approached unity as the size of this area approached that of the whole cell (Fig. 1D). Similar calculations performed for several cells led us to restrict our analysis to relative area sizes in the 0.15-0.25 range, in which the relationship between perinuclear/cytoplasmic staining ratio and relative area size could be fitted reasonably by a linear function (Fig. 1D, gray area). We defined the perinuclear clustering index (PCI) as the slope of the fitted linear function, multiplied by 1 to render positive values. Importantly, we found that the role of the operator in deciding the shape of the NP region area was not a major source of error, as the operator-to-operator variability in the analysis of the same set of cells (11%) was lower than the cell-to-cell variability within a fibroblast line (76%).
Using this quantitative approach, we re-examined the effect of BLOC-3 deficiency on perinuclear clustering of Lamp1-positive organelles in murine skin fibroblasts (Nazarian et al., 2003) and extended our analysis to fibroblasts deficient in BLOC-1 or -2, which are another two protein complexes of unknown molecular function but implicated in the pathogenesis of HPS. We used immortalized lines of skin fibroblasts derived from a wild-type strain and from the pallid, cocoa and pale ear strains deficient in BLOC-1, -2 and -3, respectively. We analyzed three independent cell lines (derived from different animals) per strain; for each cell line, we calculated the PCI as the average of the values obtained for 20 randomly selected cells. The results are shown in Fig. 1E. Consistent with our previous study (Nazarian et al., 2003
), the PCI of Lamp1 staining was significantly reduced in cells deficient in BLOC-3. By contrast, the PCI was not significantly affected in cells deficient in BLOC-1 or -2. Hence, normal perinuclear clustering of Lamp1-positive organelles in fibroblasts requires BLOC-3 function but seems not to depend on BLOC-1 or -2.
The LAMP1-GFP fusion protein localizes to late endocytic organelles at low expression levels but its overexpression causes abnormal organelle aggregation
To characterize further the effects of BLOC-3 deficiency on Lamp1-positive late endosomes and lysosomes, we expressed a construct consisting of the human ortholog of murine Lamp1, LAMP1, fused at its cytoplasmic carboxyl terminus to GFP. We chose to fuse GFP to human LAMP1, and not to the murine protein, because of the availability of a species-specific rat monoclonal antibody, 1D4B, which recognizes mouse Lamp1 and not human LAMP1 and thus allows detection of endogenous Lamp1 in cells expressing the LAMP1-GFP construct. Control experiments using human M1 fibroblasts transfected with the LAMP1-GFP-encoding plasmid corroborated that the monoclonal antibody does not significantly crossreact with LAMP1-GFP, even at the highest expression levels achieved in this study (not shown). Fusion of GFP at the carboxyl terminus of human LAMP1 did not interfere with its subcellular targeting, as judged by extensive colocalization between LAMP1-GFP and endogenous Lamp1 (Fig. 2A-C). As expected, the LAMP1-GFP fusion protein localized to most lysosomes labeled with internalized dextran, as well as to dextran-negative organelles that probably represented late endosomes (Fig. 2D-F). In agreement with a previous study using a GFP-tagged form of the avian Lamp1 homolog, lgp120 (Patterson and Lipincott-Schwartz, 2002), LAMP1-GFP was also targeted to pre-formed lysosomes, as inferred from its partial localization to lysosomes that had been loaded with dextran before transfection with the LAMP1-GFP-encoding plasmid (not shown). At low expression levels, LAMP1-GFP colocalized poorly with the early endosomal marker EEA1 (Fig. 2G-I). The degrees of colocalization of LAMP1-GFP with endogenous Lamp1 (Fig. 2J-L), dextran-loaded lysosomes (Fig. 2M-O) and EEA1 (not shown) in BLOC-3-deficient fibroblasts were similar to those observed in wild-type fibroblasts, implying that the steady-state localization of LAMP1-GFP was not significantly affected by BLOC-3 deficiency.
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High levels of LAMP1-GFP overexpression not only led to accumulation of the chimeric protein at the cell surface and EEA1-positive compartments but, surprisingly, elicited aggregation of late endocytic compartments. Organelle aggregation in LAMP1-GFP-overexpressing cells was inferred from immunostaining of endogenous mouse Lamp1 (Fig. 3A-D) or labeling of lysosomes with fluorescent dextran either before (Fig. 3E,F) or after (not shown) transfection with the LAMP1-GFP-encoding plasmid. At low magnification, the staining appeared as `chunky' (see Fig. 3B,D,F, arrows); however, close examination at high optical resolution by confocal microscopy revealed that the organelles were aggregated but not fused with each other (Fig. 3F, inset, and data not shown). A similar effect was observed upon expression of high levels of LAMP1-GFP in BLOC-3-deficient fibroblasts (Fig. 3I-L), indicating that BLOC-3 function is not required for this phenomenon. Further analyses (not shown) demonstrated that the same effect can be elicited upon overexpression of LAMP1-GFP in other cell lines (e.g. human HeLa and M1 cells) or by overexpression of another Lamp (LAMP3/CD63) tagged with GFP, and that early and recycling endosomes do not seem to be affected as judged by EEA1 and transferrin receptor immunostaining in LAMP1-GFP-overexpressing cells.
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Previous studies have shown that microinjection of divalent antibodies to the cytoplasmic domain of LAMP1 can elicit aggregation of lysosomes (Bakker et al., 1997), and that overexpression of endoplasmic reticulum (ER)-resident membrane proteins fused to GFP at the cytoplasmic domain can induce stacked ER membrane structures resulting from low-affinity, anti-parallel dimerization of the GFP tag (Snapp et al., 2003
). We hypothesized that the aberrant aggregation of late endosomes and lysosomes observed in cells expressing high levels of LAMP1-GFP could be owing to low-affinity binding of LAMP1-GFP from opposing membranes, through dimerization of their GFP tags. To test this hypothesis, we substituted leucine 221 of the GFP domain with lysine, a point mutation known to disrupt the ability of GFP to form anti-parallel dimers (Zacharias et al., 2002
), and examined the ability of the resulting fusion protein variant, LAMP1-mGFP, to elicit aggregation of late endocytic compartments. Wild-type murine fibroblasts were transiently transfected with plasmids encoding LAMP1-GFP or LAMP1-mGFP, and the following day were fixed, permeabilized and subsequently stained for endogenous Lamp1 using Cy3-conjugated secondary antibody. Images of GFP and Cy3 fluorescence were obtained for each of 117 and 134 randomly selected cells expressing LAMP1-GFP and LAMP1-mGFP, respectively, and saved using coded file names. On the basis of GFP fluorescence intensity, we estimated that the expression levels of the two fusion proteins were comparable; in arbitrary units, the median values were 33 and 41, and the ranges were 9-144 and 20-189, for cells expressing LAMP1-GFP and LAMP1-mGFP, respectively. The Cy3 fluorescence images, corresponding to endogenous Lamp1 staining, were scored by two observers who were not aware of the identity of the expressed construct or its expression level. Whereas 16 of the 117 LAMP1-GFP-expressing cells (14%) and 9 of the 11 cells expressing the highest LAMP1-GFP levels (82%) were scored as having `chunky' Lamp1 staining by the two observers, none of the 134 cells expressing LAMP1-mGFP displayed such phenotype (e.g. see Fig. 3G,H). Therefore, the abnormal aggregation of lysosomes and late endosomes caused by LAMP1-GFP overexpression requires the ability of GFP to form dimers.
Dynamics of late endocytic organelles in wild-type and mutant fibroblasts
Time-lapse fluorescence microscopy experiments were performed to test whether BLOC-3 is required for optimal movement of late endocytic compartments. A first set of experiments was carried out using wild-type and pale ear fibroblasts (three independent cell lines per strain) expressing low LAMP1-GFP levels comparable with those of the cells shown in Fig. 2. Subsequent experiments were carried out using cells expressing the non-dimerizing LAMP1-mGFP variant (two independent cell lines per strain) as well as cells in which lysosomes were specifically labeled using BODIPY-FL-conjugated dextran (one cell line per strain). In each case, ten cells per fibroblast line were analyzed by acquiring 50 consecutive GFP fluorescence images at 2-second intervals.
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For quantitative analyses, we randomly selected 30 LAMP1-GFP-labeled organelles per cell, and for each organelle we determined its position at each frame. Examples of two-dimensional projections of the trajectories of selected LAMP1-GFP-positive organelles are depicted in Fig. 4B. For each organelle we calculated the maximum speed and effective distance, the latter defined as the largest distance between any two positions in the trajectory. Fig. 5 shows the distributions of maximum speed (panel A) and effective distance (panel B) corresponding to 900 LAMP1-GFP-positive organelles (30 organelles x 10 cells x 3 cell lines) from wild-type fibroblasts and the same number of organelles from pale ear (BLOC-3-deficient) fibroblasts. Panels A and B of Fig. 5 also show the corresponding distributions of LAMP1-GFP-positive organelles from wild-type cells treated with nocodazole, which allowed us to infer the extent of microtubule-dependent movement as assessed by our system. In particular, movement of LAMP1-GFP-positive organelles in nocodazole-treated wild-type cells only rarely achieved or exceeded an instant speed of 0.78 µm/second (corresponding under our imaging conditions to a displacement of 4 pixels between two consecutive frames; Fig. 5A) and never exceeded an effective distance of 4 µm (Fig. 5B). Interestingly, a relatively larger fraction of organelles from pale ear cells displayed maximum speed values of less than 0.78 µm/second (Fig. 5A) and traveled effective distances of less than 4 µm (Fig. 5B). Similar shifts in maximum speed and effective distance distributions were observed in experiments using wild-type and pale ear cells expressing the LAMP1-mGFP variant construct or labeled with BODIPY-FL-conjugated dextran (not shown).
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We next considered the possibility that the observed differences in the dynamics of late endosomes and lysosomes between normal and BLOC-3-deficient cells could reflect deficiencies in their movement on microtubules. To address this possibility, we took advantage of the observation that LAMP1-positive organelles almost never moved at 0.78 µm/second or faster in nocodazole-treated cells (Fig. 5A). We chose this speed value as a threshold with which to select movement events that most probably occurred on microtubules. For each of the LAMP1-GFP-positive and LAMP1-mGFP-positive organelles analyzed as described above, we calculated the fraction of time traveled at instant speeds matching or exceeding the 0.78 µm/second threshold (Fig. 6A), as well as the average speed of this subset of movement events (referred to as average speed on microtubules; Fig. 5C and data not shown). For statistical analyses, median values per cell were calculated as described above for the other variables. The median values per cell calculated for average speed on microtubules (Fig. 5F) followed normal distributions upon logarithmic transformation and, hence, could be analyzed using an ANOVA model. In this case, however, the effect of BLOC-3 deficiency was statistically not significant (P>0.8). By contrast, a relatively higher fraction of late endocytic compartments within pale ear cells moved less than 2% of the time at the threshold speed or faster, regardless of whether the compartments were labeled with LAMP1-GFP or LAMP1-mGFP variants (Fig. 6A). The data obtained for this variable could not be analyzed using an ANOVA model because a large fraction of the median values per cell were zero, thus making it impossible to achieve a Gaussian distribution, even upon data transformation. For this reason, and because the most salient characteristic of the resulting distributions of median values per cell was the zero value, we applied Fisher's exact test to compare the relative odds of obtaining such value for wild-type and pale ear cells. To maximize statistical power, data obtained using cells expressing LAMP1-GFP or LAMP1-mGFP were pooled. The resulting pale ear/wild-type odds ratio was 3.6, which was statistically significant (P=0.0057). Interestingly, similar differences were observed when organelle movement at instant speeds matching or exceeding the 0.78 µm/second threshold was analyzed taking into account its directionality, i.e. whether such movement was towards (Fig. 6B) or away from (Fig. 6C) the nucleus. Upon calculation of median values per cell, the odds of obtaining zero as a result were significantly higher among pale ear cells, both for movement towards the nucleus (odds ratio
4.3, P=0.0016) and away from the nucleus (odds ratio
3.7, P=0.0038). We also considered whether the observed differences in percentages of time traveling at the threshold speed or faster reflected a reduction in the number of events in which the organelle accelerated to match or exceed the threshold speed, and/or the duration of such events. The distribution of numbers of events with speed increasing to
0.78 µm/second was shifted towards lower values in pale ear cells as compared with wild-type cells (Fig. 7), and the odds of obtaining zero as the median value per cell was significantly higher in pale ear cells (Fisher's exact test, P=0.005). By contrast, the distributions of the duration of such events revealed no statistical differences between wild-type and pale ear cells (not shown). Taken together, these results suggest that lack of BLOC-3 function negatively affects the ability of late endocytic organelles to attach productively to microtubule-dependent motors but does not influence significantly the duration or speed of these movement events.
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Discussion |
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Previous studies on the perinuclear clustering of organelles, including our own (Nazarian et al., 2003), have relied on the subjective judgement of an observer determining whether a given cell displays pronounced perinuclear accumulation or not, followed by comparison of different cell samples based on the percentages of cells determined to display such phenotype (e.g. see Matteoni and Kreiss, 1987
; Poupon et al., 2003
; Matsushita et al., 2004
; Gissen et al., 2005
; Hölttä-Vuori et al., 2005
). Here, we have chosen to estimate the concentration gradient of the staining of an organelle marker around the perinuclear region as the PCI, thus allowing subsequent comparison of cell samples on the basis of their averaged PCI values. It should be emphasized, however, that the PCI is an approximation but not a real measure of such concentration gradient. A second limitation is that subjective judgment is still involved in delimiting the NP region areas necessary for calculation of the PCI. Nevertheless, the fact that the operator-to-operator variability was significantly lower than the cell-to-cell variability implies that such a subjective component should not have a major impact on the results. In any event, the images were analyzed following a `blinded' approach in which the operator was unaware of the sample identity. Another limitation of the method described herein is that it is time-consuming. For these reasons, a fully automatic, image-processing method remains desirable. Finally, the method might not be sensitive enough to detect differences in perinuclear clustering of other organelle markers, or even of Lamp1 staining in cell types different from fibroblasts (e.g. cells that attach poorly to surfaces or with a high nucleus-to-cytoplasm ratio). Hence, its application to other systems may require optimization of experimental and image processing conditions.
Using the PCI approach, we have corroborated our previous observation that BLOC-3 deficiency results in decreased perinuclear clustering of Lamp1-positive, late endocytic organelles, and found no defects in perinuclear clustering of these organelles in mutant cells deficient in BLOC-1 or -2. As in the case of BLOC-3, BLOC-1 and -2 are expressed ubiquitously and mutations in the genes encoding at least some subunits cause HPS in humans and/or mice. However, their molecular function remains obscure (reviewed by Li et al., 2004; Di Pietro and Dell'Angelica, 2005
). Fibroblasts derived from HPS patients bearing mutations in the gene encoding the HPS5 subunit of BLOC-2 have been shown to display exacerbated perinuclear clustering of late endocytic organelles containing LAMP3/CD63, with little or no staining observed in the vicinity of the plasma membrane (Huizing et al., 2004
). By contrast, the same group reported that fibroblasts from patients carrying mutations in the gene encoding the HPS3 subunit of the same complex display normal distribution of LAMP3/CD63 staining (Gunay-Aygun et al., 2004
). Although the PCI determined for three independent cell lines derived from cocoa mice (carrying mutations in the HPS3-encoding gene) seemed to be somewhat higher than the average PCI of wild-type cells (Fig. 1E), the differences were statistically not significant. In addition, we did not see any depletion of Lamp1 staining from the cell periphery of our cell samples. The reasons for the above discrepancies remain unclear.
To test whether BLOC-3 regulates the movement of late endosomes and lysosomes, we have performed time-lapse experiments using live cells expressing LAMP1 fused to either GFP or its non-dimerizing L221K variant, referred herein to as mGFP. At low expression levels, both fusion proteins were targeted correctly to late endocytic organelles, and no significant differences were observed in the dynamics of organelles labeled with LAMP1-GFP versus LAMP1-mGFP. Given the heterogeneity of organelles labeled with LAMP1-GFP or its variant, as well as the intrinsic variability between cells and between cell lines, large sets of time-lapse microscopic data were necessary to test for statistically meaningful differences between control and BLOC-3-deficient cells. For these analyses, we decided to consider each cell, rather than each tracked organelle, as an independent observation. We detected statistically significant differences between control and BLOC-3-deficient fibroblasts in the maximum speed and effective distance traveled by late endocytic organelles, even when the numeric differences were not too dramatic. Because these differences were suggestive of partial defects in organelle movement on microtubules, we defined the speed of 0.78 µm/second as a threshold with which to select those movement events that most probably occurred on microtubules. We realize that by using such a threshold value we may have filtered out movement events that were microtubule dependent but slow; such a limitation must be borne in mind during interpretation of the data. We attempted the alternative approach of performing time-lapse experiments using cells treated with actin-depolymerizing drugs (e.g. Latrunculin A) and assuming that all movement observed under these conditions would be microtubule dependent. However, the relatively large cells used in this study underwent significant changes of shape and partial detachment upon drug treatment, thus precluding acquisition of high-quality images (data not shown). Notwithstanding the potential limitations of using a threshold speed to study microtubule-dependent events, we were able to detect a relative decrease in the frequency of events in which labeled organelles within BLOC-3-deficient cells traveled at instant speeds equal or higher than the threshold. Interestingly, lack of BLOC-3 function affected movement on microtubules (i.e. at the threshold speed or higher) both towards and away from the perinuclear region, suggesting that productive attachment of late endocytic organelles to both dynein/dynactin and kinesins might be compromised. We considered the possibility that the observed differences could simply reflect the existence in BLOC-3-deficient cells of an extra pool of essentially immobile organelles, together with organelles with dynamics identical to those of control cells. However, upon exclusion of organelles that never moved at the threshold speed or faster from the data analysis, the resulting distributions still demonstrated a shift towards reduced frequencies of microtubule-dependent movement events for late endocytic organelles within BLOC-3-deficient cells (data not shown).
By which mechanism does BLOC-3 regulate late endocytic organelle movement? At least three scenarios can be considered. First, BLOC-3 could be directly involved in the attachment of these organelles to microtubule-dependent motors, although our results suggest that, if so, it should mediate attachment to both dynein and kinesin motors. The ability of a protein to regulate bidirectional, microtubule-dependent movement directly has previously been documented for dynactin and MEK/ERK bound to melanosomes (Deacon et al., 2003; Deacon et al., 2005
), although not yet for proteins associated with late endosomes and lysosomes. Given that substantial movement of late endosomes and lysosomes was still observed in pale ear fibroblasts, one must conclude that BLOC-3 function is not essential for organelle attachment to microtubules. Hence, consideration of this first scenario would imply assuming that other cellular proteins can compensate in part for the lack of BLOC-3. Second, BLOC-3 function could be important for detaching late endocytic organelles from actin filaments. In such a scenario, lack of BLOC-3 function would increase the fraction of time spent by late endosomes and lysosomes on actin filaments, thus decreasing the fraction of time in which the organelles would be available for attachment to microtubules. This second scenario would provide a satisfactory explanation for the observations that BLOC-3 deficiency affected microtubule-dependent movement in both directions, and that the observed defects were partial. Third, BLOC-3 could play a rather indirect role, for instance by mediating the intracellular trafficking to late endosomes and lysosomes of a protein that, in turn, would be required for organelle attachment to microtubules and/or detachment from actin filaments. This third scenario, and not the first two, would be compatible with the intracellular localization reported for the HPS1 subunit of BLOC-3, which by immunogold labeling was found to be associated with tubulovesicular membrane profiles in the vicinity of the Golgi complex of lymphoblastoid cells (Oh et al., 2000
). It is worth mentioning that a similar mechanism has been invoked to explain the defective movement of lytic granules, the lysosome-related organelles of cytotoxic T cells, in patients suffering from HPS-2 resulting from mutations in the gene encoding the ß3A subunit of AP-3, a protein complex directly involved in protein trafficking (Clark et al., 2003
).
How can the phenotype of BLOC-3-deficient fibroblasts be reconciled with the clinical manifestations of HPS-1 and -4? As mentioned in the introductory section, the main manifestations of these two forms of HPS are due to defects in cell-type-specific, lysosome-related organelles, namely melanosomes, platelet dense granules and lamellar bodies. Mild ceroid lipofuscinosis has also been described, at least for HPS-1, which could reflect modest defects in lysosomal function due to the observed abnormalities in organelle movement and localization. Conceivably, BLOC-3 could be required for normal movement and distribution of lysosome-related organelles and/or their precursors, and because melanosomes and platelet dense granules (and lamellar bodies?) co-exist with conventional lysosomes, one might even speculate that BLOC-3 could promote spatial segregation of maturing lysosomes and lysosome-related organelles to reduce the chances of heterotypic organelle fusion. Nevertheless, it is clear that future work will be necessary to establish the molecular function of BLOC-3 and its role in the pathogenesis of HPS.
During the course of this study, we noticed that high levels of LAMP1-GFP overexpression induced aberrant aggregation of late endocytic organelles, both in wild-type and BLOC-3-deficient cells. We observed that LAMP1-GFP overexpression was capable of inducing aggregation of pre-existing lysosomes, as inferred from experiments involving loading of lysosomes with fluorescent dextran prior to transfection with the LAMP1-GFP-encoding plasmid (e.g. Fig. 3E,F). We also observed the aggregation phenomenon using different cell types and by overexpressing a construct consisting of human LAMP3/CD63 fused at its cytoplasmic domain to GFP (not shown). Because GFP is capable of low-affinity self-association, we considered the possibility that the observed aggregation of late endocytic organelles could be caused by low-affinity, anti-parallel dimerization of LAMP1-GFP molecules associated with the limiting membranes of opposing organelles. An analogous mechanism has recently been shown to mediate the formation of stacked ER membranes induced by overexpression of an ER-resident membrane protein tagged with GFP at its cytoplasmic domain (Snapp et al., 2003). In agreement with this idea, a point mutation introduced into the GFP domain of LAMP1-GFP to disrupt its ability to dimerize resulted in a variant fusion protein, LAMP1-mGFP, which failed to induce aggregation of late endocytic organelles at the highest expression levels achieved. Consequently, these results raise a note of caution on the interpretation of experiments in which aggregation of late endosomes and lysosomes is induced by overexpression of GFP-fusion proteins, and suggest that non-dimerizing mutant forms of GFP would be more appropriate tools for this type of experiments.
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