Abstract
Efficient phagocytosis of apoptotic cells is crucial for tissue homeostasis and the immune response1,2. Rab5 is known as a key regulator of the early endocytic pathway3 and we have recently shown that Rab5 is also implicated in apoptotic cell engulfment4; however, the precise spatio-temporal dynamics of Rab5 activity remain unknown. Here, using a newly developed fluorescence resonance energy transfer biosensor, we describe a change in Rab5 activity during the engulfment of apoptotic thymocytes. Rab5 activity on phagosome membranes began to increase on disassembly of the actin coat encapsulating phagosomes. Rab5 activation was either continuous or repetitive for up to 10 min, but it ended before the collapse of engulfed apoptotic cells. Expression of a dominant-negative mutant of Rab5 delayed this collapse of apoptotic thymocytes, showing a role for Rab5 in phagosome maturation. Disruption of microtubules with nocodazole inhibited Rab5 activation on the phagosome membrane without perturbing the engulfment of apoptotic cells. Furthermore, we found that Gapex-5 is the guanine nucleotide exchange factor essential for Rab5 activation during the engulfment of apoptotic cells. Gapex-5 was bound to a microtubule-tip-associating protein, EB1, whose depletion inhibited Rab5 activation during phagocytosis. We therefore propose a mechanistic model in which the recruitment of Gapex-5 to phagosomes through the microtubule network induces the transient Rab5 activation.
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Main
To make Rab5 activity visible in living cells, we developed a genetically encoded fluorescence resonance energy transfer (FRET) probe, designated Raichu-Rab5. The probe comprised a modified yellow fluorescent protein (YFP) called Venus, the amino-terminal Rab5-binding domain of EEA1, a modified cyan fluorescent protein (CFP) called SECFP, and Rab5 (Fig. 1a). In this probe design, an increase in Rab5-GTP results in an increase in FRET, which can be represented by the 525 nm/475 nm emission ratio. Characterization of Raichu-Rab5 was conducted similarly to that of other Raichu probes reported previously5,6. In comparison with the wild-type Rab5 probe, Raichu-Rab5-Q79L—which lacks GTPase activity—had an increased FRET efficiency, whereas Raichu-Rab5-S34N—which shows a reduced affinity for guanine nucleotides—had a decreased FRET efficiency, as expected (Supplementary Fig. 1a). The GTP loading of the Rab5 probes correlated well with that of the authentic Rab5 proteins (Supplementary Fig. 1b), and the GTP loadings obtained here were similar to those reported previously7. Next, we examined the sensitivity of Raichu-Rab5 to guanine nucleotide exchange factors (GEFs) and GTPase-activating proteins (GAPs) (Supplementary Fig. 1c). Rab5 GEFs such as Rabex-5, Rin1 and Gapex-5 induced a dose-dependent increase in the FRET efficiency of Raichu-Rab5. In contrast, the expression of Rab5 GAPs such as RabGAP-5 and RN-tre decreased the FRET efficiency in a dose-dependent manner. These results indicate that Raichu-Rab5 is capable of monitoring the balance between GEF and GAP activities towards Rab5.
We then examined the subcellular distribution of Raichu-Rab5. Rab5 localizes at early endosomes and the plasma membrane. Raichu-Rab5 co-localized with authentic Rab5a at endosomal structures in HeLa cells (Supplementary Fig. 2a, top panel). The distribution of Raichu-Rab5 did not overlap with those of Rab7 and Rab11a, which were used as markers for late and recycling endosomes, respectively (Supplementary Fig. 2a, middle and bottom panels). The subcellular distribution of Raichu-Rab5 was very similar to those of early endosomal markers, namely the FYVE domain of EEA1 (ref. 8) and the PX domain of p40phox (also known as NCF4)9 (Supplementary Fig. 2b). Finally, Raichu-Rab5 was found to bind to Rab guanine dissociation inhibitor (RabGDI) as efficiently as authentic Rab5a (data not shown), suggesting that Raichu-Rab5 is also subject to regulation by RabGDI.
By using Raichu-Rab5 we revealed Rab5 activation during the milk-fat-globule epidermal growth factor 8 (MFG-E8)-mediated engulfment of apoptotic cells by Swiss3T3 cells stably expressing integrin αvβ3 (Fig. 1b and Supplementary Video 1). The progress of phagocytosis was monitored by phase-contrast images, in which the completion of engulfment was recognizable by the transition of the engulfed apoptotic cells from phase-bright to phase-dark10. The accumulation of Raichu-Rab5 around the engulfed apoptotic cells, and an increase in FRET, began during the period of phase shift and reached a peak after the completion of engulfment.
During the course of experiments, we noticed that the abundance of cytoplasmic Raichu-Rab5, probably associated with RabGDI, hampered the quantification of FRET at the membrane. We therefore developed a Raichu-Rab5 probe fused to the carboxy terminus of Ki-Ras protein (Raichu-Rab5/PM), which localized at the plasma membrane and on phagocytic vesicles. This alteration did not affect the activation status of Rab5 probe (Supplementary Fig. 3). With this improved Raichu-Rab5 probe, we examined the time course of Rab5 activation more precisely (Figs 1c and 2e, and Supplementary Video 2). We set the zero time point to be the frame immediately before the initiation of the phase shift, which lasted about 3 min on average. Rab5 activation started during this period of phase shift and reached a peak within 4 min on average. Very similar results were obtained in a macrophage cell line, BAM3 (Supplementary Fig. 4). The duration of Rab5 activation varied significantly between different phagosomes. In addition, 37% of phagosomes showed reactivation of Rab5 after the cessation of initial Rab5 activation (Figs 1d and 3c, and Supplementary Video 3). The time course of this Rab5 reactivation also varied between phagosomes: some phagosomes showed a repetitive cycle of activation and inactivation, whereas others showed an abrupt and transient reactivation.
To gain insight into the role of Rab5 activation in phagocytosis, we examined the precise timing of actin assembly, Rab5 recruitment around phagocytic vesicles, and breakdown of apoptotic thymocytes in Swiss 3T3/integrin αvβ3 cells (Fig. 2). As revealed with enhanced green fluorescent protein (EGFP)–actin, actin fibres could be seen around the phagocytic vesicles from -3 to 2 min, showing that Rab5 is activated during actin disassembly (Fig. 2a, d, e). This observation was shown more directly by simultaneous imaging of monomeric red fluorescent protein (mRFP)–actin and Raichu-Rab5 (Supplementary Fig. 5). Next, accumulation of mEGFP–Rab5 on the phagosome membrane was revealed with mRFP as a reference of entirely cytosolic protein11 (Fig. 2b, f). The ratio of mEGFP–Rab5 versus mRFP increased on phagosomes after 3–7 min of internalization, indicating that Rab5 was recruited to phagosomes during this period. This time course of Rab5 accumulation was similar to that of Rab5 activation. Finally, we examined the timing of apoptotic cell breakdown by the use of EGFP-expressing thymocytes. Owing to the acid-labile nature of EGFP, the collapse of apoptotic cells within phagosomes could be monitored by the extinction of fluorescence. With this method, we found that EGFP-expressing thymocyte fluorescence disappeared during the period from 10 to 20 min (Fig. 2c, g). We confirmed, by the use of a pH indicator, that the extinction of EGFP fluorescence was correlated with an increase in intracellular pH level (Supplementary Fig. 6). Thus, Rab5 inactivation preceded the decrease in pH and the breakdown of apoptotic cells. The expression of Rab5-S34N delayed, but did not block, the breakdown of apoptotic thymocytes (Fig. 2h). This indicated that Rab5 activation has a function in phagosome maturation during the engulfment of apoptotic cells, although Rab5-independent pathways may exist. A similar role for Rab5 has been proposed in FcγR-mediated phagocytosis12,13. This is supposed to come from the basic function of Rab5 mediating the fusion of phagosomes with early endosomes14,15. Furthermore, active Rab5 is necessary for the recruitment of Rab7 (ref. 13), which regulates the fusion of phagosomes with late endosomes to initiate the lysis of cell corpses.
In the engulfment process, microtubules were required for Rab5 activation. Treatment with 0.1 μM nocodazole significantly decreased Rab5 activation at the engulfment site (Fig. 3a), indicating that Rab5 activation depends on the integrity of the microtubule network. When microtubules were stabilized with 10 nM paclitaxel, initial Rab5 activation was observed as in the control cells, but repetitive Rab5 activation was inhibited significantly (Fig. 3b, c). Thus, it seems that the repetitive activation of Rab5 as shown in Fig. 1d is due to the dynamic instability of microtubule plus-ends.
To search for the molecular link between microtubule and Rab5 activation during phagocytosis, candidate Rab5 GEFs were depleted by RNA interference, and the resulting phenotypes were examined. The expressions of Rabex-5, Rin1 and Gapex-5 were markedly decreased by transfection of the respective short interfering RNA (siRNAs) in Swiss 3T3/integrin αvβ3 cells (Supplementary Fig. 7a). We then monitored the Rab5 activity during phagocytosis in cells lacking each Rab5 GEF. The depletion of Gapex-5 significantly inhibited Rab5 activation at engulfment sites, whereas neither Rabex-5 depletion nor Rin1 depletion showed any effect on Rab5 activation during phagocytosis (Fig. 3d). Expression of siRNA-resistant Gapex-5 restored the Rab5 activation (Fig. 3d and Supplementary Fig. 7c). The involvement of Gapex-5 in Rab5 activation was corroborated by a significant delay in the duration of EGFP-expressing thymocyte fluorescence in Gapex-5-depleted cells (Fig. 3e). These results demonstrated for the first time that Gapex-5 is an essential regulator for Rab5 activation and phagosome maturation during phagocytosis of apoptotic cells. We assumed that Gapex-5 is delivered to phagosomes by a microtubule-dependent mechanism. This idea could explain the observation that the reduced dynamic instability of microtubules in paclitaxel-treated cells suppressed repetitive Rab5 activation on phagosomes (Fig. 3c). Because Gapex-5 did not show a high affinity for microtubules by itself, we searched for the protein that could link Gapex-5 to microtubule and found that a microtubule-tip-associating protein, EB1 (ref. 16), was associated with Gapex-5 (Supplementary Fig. 8a, c). In agreement with the role predicted for EB1, EB1 knockdown significantly reduced Rab5 activation during phagocytosis (Supplementary Fig. 8b).
The present study shows that Gapex-5-mediated Rab5 activation follows disassembly of the actin coat surrounding phagosomes. Recalling that the Raichu-Rab5 probe monitors the balance of activity between GEFs and GAPs on the membrane, we envisage the following model for the regulation of Rab5 during phagocytosis: first, engulfment of apoptotic cells and accumulation of actin filaments around the nascent phagosome; second, actin disassembly during phagosome membrane closure; third, invasion of microtubules into the cell periphery (this probably happens because the actin filaments behave as physical barriers for microtubule extension17); fourth, delivery of Gapex-5 to phagosomes by EB1 on microtubules; fifth, a subsequent increase in the ratio of GEF activity to GAP activity on the phagosome membrane resulting not only in the activation of local Rab5 but also in the recruitment of Rab5 released from the Rab5–RabGDI complex in the cytosol. There might be a positive feedback mechanism for local amplification of Rab5 signal, as has been proposed for early endosomes3,18. This study shows that live-cell imaging with FRET probes enables us to pinpoint the activation and inactivation of Rab5 and thereby to understand its relationship to the other events of phagocytosis.
Methods Summary
C57BL/6 mice were purchased from Japan SLC. EGFP-transgenic mice19 were a gift from M. Okabe. Swiss3T3 fibroblasts stably expressing integrin αvβ3 were established by infecting cells with a retrovirus carrying mouse integrin αv and β3 cDNAs20 and maintained in DMEM medium supplemented with 10% fetal bovine serum. Retrovirus expressing EGFP–actin, mEGFP–Rab5, mCherry-Rab5-S34N or mCherry-Gapex-5 resistant to Gapex-5 siRNA was additionally inoculated into Swiss3T3/integrin αvβ3 cells. Apoptotic thymocytes were prepared as previously described4. In brief, thymocytes of 4–8-week-old C57BL/6 mice or EGFP-transgenic mice were treated for 5 h with 10 μM dexamethasone at 37 °C to induce apoptosis. Transient transfection of siRNA was used to decrease the level of specific proteins. For time-lapse FRET imaging, Swiss3T3/integrin αvβ3 cells expressing FRET probes were cultured in phenol-red-free DMEM/F12 medium supplemented with 10% fetal bovine serum, and loaded with 4 × 106 apoptotic thymocytes in the presence of 0.1 μg ml-1 MFG-E8. Cells were imaged with an IX81 inverted microscope (Olympus) equipped with a cooled charge-coupled device (CCD) camera (Retiga Exi, QImaging or Cool SNAP-HQ; Roper Scientific), an IX2-ZDC laser-based autofocusing system (Olympus) and an MD-XY30100T-Meta automatically programmable XY stage (Sigma KOKI). The following filters used for the dual-emission imaging studies were obtained from Omega Optical: an XF1071 (440AF21) excitation filter, an XF2034 (455DRLP) dichroic mirror and two emission filters (XF3075 (480AF30) for CFP and XF3079 (535AF26) for YFP). After background subtraction, FRET/CFP ratio images were created with MetaMorph software (Universal Imaging), and the images were used to represent FRET efficiency.
Online Methods
Plasmids
pRaichu-Rab5, derived from the pCAGGS expression vector, encoded a probe, designated Raichu-Rab5, that comprised Venus (the brightest version of YFP)21, the amino-terminal Rab5-binding domain of EEA1 (amino-acid residues 36–218), SECFP (a brighter version of CFP obtained from A. Miyawaki) and Rab5a (a gift from Y. Takai). In both Venus and SECFP, an A206K mutation was introduced to prevent dimerization between fluorescent proteins22. In pRaichu-Rab5/PM, the carboxy-terminal peptide of Rab5, QCCSN, was replaced with that of Ki-Ras, RKMSKDGKKKKKKSKTKCVIM. Mouse Rabex-5 cDNA was cloned from the mouse spleen cDNA library (a gift from N. Mochizuki) and point-mutated to resist siRNA. The cDNA for mCherry was a gift from R. Tsien. mEGFP–Rab5, mCherry-Rab5-S34N (ref. 23) and mCherry-Gapex-5 resistant to Gapex-5 siRNA were subcloned into pCX4bsr (ref. 24). Retroviral vector pCX4bleo-EGFP–actin was provided by M. Okada.
Mice, cells, reagents and antibodies
C57BL/6 mice were purchased from Japan SLC. EGFP-transgenic mice19 were a gift from M. Okabe. Swiss3T3 fibroblasts stably expressing integrin αvβ3 were established by infecting cells with a retrovirus carrying mouse integrin αv and β3 cDNAs20 and were maintained in DMEM medium supplemented with 10% fetal bovine serum. Retrovirus expressing EGFP–actin, mEGFP–Rab5, mCherry-Rab5-S34N or mCherry-Gapex-5 resistant to Gapex-5 siRNA was additionally inoculated into Swiss3T3/integrin αvβ3 cells. For imaging experiments, cells were plated on fibronectin-coated 35-mm glass-base dishes (Asahi Techno Glass).
Preparation of apoptotic thymocytes
Apoptotic thymocytes were prepared as described previously4. In brief, thymocytes of 4–8-week-old C57BL/6 mice or EGFP-transgenic mice were treated with 10 μM dexamethasone at 37 °C for 5 h to induce apoptosis.
RNA interference experiments
Swiss3T3/integrin αvβ3 cells were transfected with the desired siRNAs by using Lipofectamine RNAiMAX (Invitrogen). siRNA sequences for control, mouse Rabex-5, mouse Rin1 and mouse Gapex-5 were 5′-CACCUAAUCCGUGGUUCAA-3′, 5′-UUUAUAGAGACGCGUCAUGAUGUGC-3′, 5′-UUAUACAUUUGCUUCACACCUAAGC-3′ and 5′-GGAGUGUGAUGAAUCGGAUCUUCAA-3′, respectively. After 24 h, the cells were treated with trypsin and plated on glass-base dishes. For FRET imaging, the cells were then transfected with pRaichu-Rab5/PM. Thereafter, the cells were incubated for at least 72 h after siRNA transfection before imaging experiments.
Time-lapse FRET imaging
Swiss3T3/integrin αvβ3 cells expressing FRET probes were cultured in phenol-red-free DMEM/F12 medium supplemented with 10% fetal bovine serum, and loaded with 4 × 106 apoptotic thymocytes in the presence of 0.1 μg ml-1 MFG-E8. Cells were imaged with an IX81 inverted microscope (Olympus) equipped with a cooled CCD camera (Retiga Exi, QImaging or Cool SNAP-HQ; Roper Scientific), an IX2-ZDC laser-based autofocusing system (Olympus) and an MD-XY30100T-Meta automatically programmable XY stage (Sigma KOKI). The following filters used for the dual-emission imaging studies were obtained from Omega Optical: an XF1071 (440AF21) excitation filter, an XF2034 (455DRLP) dichroic mirror, and two emission filters (XF3075 (480AF30) for CFP and XF3079 (535AF26) for YFP). After background subtraction, FRET/CFP ratio images were created with MetaMorph software (Universal Imaging), and the images were used to represent FRET efficiency.
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Acknowledgements
We thank N. Yoshida, N. Fujimoto, A. Nishiyama, K. Fukuhara, Y. Kasakawa for technical assistance; I. Lodhi and A. Saltiel for unpublished information on Gapex-5; Y. Kiyosue for advice on EB1; and members of the Matsuda laboratory for their input. This work was supported by grants from the Ministry of Education, Culture, Sports, Science, and Technology of Japan.
Author Contributions M.K. and M.N. performed the experimental work and data analysis. T.N., S.N. and M.M. wrote the paper. All authors discussed the results and commented on the manuscript.
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Supplementary Information
This file contains Supplementary Methods, Supplementary Video Legends, and Supplementary Figures 1-8 and Legends. (PDF 3758 kb)
Supplementary Video
This file contains Supplementary Movie 1 which shows Rab5 activation during engulfment monitored by Raichu-Rab5. (MPG 4398 kb)
Supplementary Video
This file contains Supplementary Movie 2 which shows Rab5 activation during engulfment monitored by Raichu-Rab5/K-RasCT. (MPG 4398 kb)
Supplementary Video
This file contains Supplementary Movie 3 which shows Repetitive Rab5 activation at the engulfment site . (MPG 4398 kb)
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Kitano, M., Nakaya, M., Nakamura, T. et al. Imaging of Rab5 activity identifies essential regulators for phagosome maturation. Nature 453, 241–245 (2008). https://doi.org/10.1038/nature06857
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DOI: https://doi.org/10.1038/nature06857
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