Mertk Triggers Uptake of Photoreceptor Outer Segments during Phagocytosis by Cultured Retinal Pigment Epithelial Cells

Feng, Wei; Yasumura, Douglas; Matthes, Michael T.; LaVail, Matthew M.; Vollrath, Douglas

doi:10.1074/jbc.m107876200

Cited by 207 publications

(154 citation statements)

References 26 publications

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“…This resulted from either RPE uptake of lone QT or phagocytosis of PPC-graft containing QT. The latter scenario was observed in vitro here (Figure 3f) and in others studies 21,22 and is expected given the RPE's phagocytic roles. 23 …”

Section: Graft Survival and Qt Locationsupporting

confidence: 57%

Bimodal in vivo imaging provides early assessment of stem-cell-based photoreceptor engraftment

Laver

Metcalfe

Szczygiel

et al. 2015

Eye

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Purpose Subretinal transplantation of stem-cell-derived photoreceptor precursor cells (PPCs) is a promising and innovative approach to treating a range of blinding diseases. However, common barriers to efficient preclinical transplantation comes in the form of suboptimal graft architecture, limited graft survival, and immune-rejection, each of which cannot be assessed using conventional in vivo imaging (ie, rodent ophthalmoscopy). With the majority of PPCs reported to die within the first few weeks after transplantation, understanding the mechanisms of graft failure, and ultimately devising preventative methods, currently relies on lengthy end point histology.To address these limitations, we hypothesized that combining two imaging modalities, optical coherence tomography (OCT) and fluorescence confocal scanning laser ophthalmoscopy (fcSLO), could provide a more rapid and comprehensive view of PPC engraftment. Methods Human ESC-derived PPCs were transplanted into 15 retinal dystrophic rats that underwent bimodal imaging at 0, 8, and 15 days posttransplant. Results Bimodal imaging provided serial detection of graft: placement, architecture, and survival; each undetectable under ophthalmoscopy. Bimodal imaging determined graft placement to be either: subretinal (n = 7), choroidal (n = 4), or vitreal (n = 4) indicating neural retinal perforation. Graft architecture was highly variable at the time of transplantation, with notable redistribution over time, while complete, or near complete, graft loss was observed in the majority of recipients after day 8. Of particular importance was detection of vitreal aggregates overlying the graft-possibly an indicator of host-site inflammation and rejection. Conclusion Early real-time feedback of engraftment has the potential to greatly increase efficiency of preclinical trials in cell-based retinal therapeutics.

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Section: Graft Survival and Qt Locationsupporting

confidence: 57%

Bimodal in vivo imaging provides early assessment of stem-cell-based photoreceptor engraftment

Laver

Metcalfe

Szczygiel

et al. 2015

Eye

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“…It is established that binding of POS to RPE cells activates a hierarchy of tyrosine kinases that are essential for phagosome internalization, and that FAK and MerTK play prominent roles in this process (Feng et al, 2002;Finnemann, 2003). Because FAK and anx A2 are substrates for several tyrosine kinases, including Src (Bellagamba et al, 1997), and because we have recently shown that anx A2 is required for the plasma membrane targeting and activation of Src (Hayes and Moss, 2009), we next tested whether anx A2 and c-Src become tyrosine-phosphorylated during POS phagocytosis by ARPE19 cells.…”

Section: Anx A2 Is Recruited To the Forming Phagosomementioning

confidence: 99%

“…Intriguingly, engagement of the ␣v␤5 integrin by its cognate ligand, milk fat globule-EGF8 (MFG-E8), is essential for the circadian synchronization of phagocytosis (Nandrot and Finnemann, 2006;Nandrot et al, 2007), and although phagocytosis of POS occurs in MFG-E8 Ϫ/Ϫ and ␤5 Ϫ/Ϫ mice, in both mutants the daily rhythm is absent. In contrast, focal adhesion kinase (FAK) and MerTK are not required for the initial binding of POS to the apical surface of the RPE, but they are sequentially activated by ␣v␤5 receptors and are essential for phagosome internalization (Feng et al, 2002;Finnemann, 2003).…”

Section: Introductionmentioning

confidence: 99%

“…In these experiments, we observed enrichment of anx A2-GFP on forming but not mature phagosomes ( Figure 2E), which when taken with the data mentioned above strongly suggests that a role for anx A2 in POS phagocytosis is most likely to be at the time of POS engagement and initial internalization. It is established that binding of POS to RPE cells activates a hierarchy of tyrosine kinases that are essential for phagosome internalization, and that FAK and MerTK play prominent roles in this process (Feng et al, 2002;Finnemann, 2003). Because FAK and anx A2 are substrates for several tyrosine kinases, including Src (Bellagamba et al, 1997), and because we have recently shown that anx A2 is required for the plasma membrane targeting and activation of Src (Hayes and Moss, 2009), we next tested whether anx A2 and c-Src become tyrosine-phosphorylated during POS phagocytosis by ARPE19 cells.…”

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confidence: 99%

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Annexin A2 Regulates Phagocytosis of Photoreceptor Outer Segments in the Mouse Retina

Law

Hajjar

et al. 2009

MBoC

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The daily phagocytosis of shed photoreceptor outer segments by pigment epithelial cells is critical for the maintenance of the retina. In a subtractive polymerase chain reaction analysis, we found that functional differentiation of human ARPE19 retinal pigment epithelial (RPE) cells is accompanied by up-regulation of annexin (anx) A2, a major Src substrate and regulator of membrane-cytoskeleton dynamics. Here, we show that anx A2 is recruited to the nascent phagocytic cup in vitro and in vivo and that it fully dissociates once the phagosome is internalized. In ARPE19 cells depleted of anx A2 by using small interfering RNA and in ANX A2 ؊/؊ mice the phagocytosis of outer segments was impaired, and in ANX A2 ؊/؊ mice there was an accumulation of phagocytosed outer segments in the RPE apical processes, indicative of retarded phagosome transport. We show that anx A2 is tyrosine phosphorylated at the onset of phagocytosis and that the synchronized activation of focal adhesion kinase and c-Src is abnormal in ANX A2 ؊/؊ mice. These findings reveal that anx A2 is involved in the circadian regulation of outer segment phagocytosis, and they provide new insight into the protein machinery that regulates phagocytic function in RPE cells. INTRODUCTIONThe retinal pigment epithelium (RPE) performs a range of functions that directly support the retina (Strauss, 2005), including the daily phagocytosis and digestion of shed photoreceptor outer segments (POS). The importance of this activity is exemplified in the dystrophic Royal College of Surgeons rat, which due to a failure in phagocytosis undergoes a progressive and rapid retinal degeneration characterized by accumulation of cellular debris and photoreceptor cell death. The gene responsible for this pathology was identified by positional cloning as the Mer tyrosine kinase (MerTK), a key signaling intermediate that is expressed in RPE cells and plays an essential role in the internalization of bound POS (Chaitin and Hall, 1983;D'Cruz et al., 2000). Recent studies have provided insight into other RPE cell proteins that have distinct roles either in the binding or the internalization of shed POS. For example, the apically expressed ␣v␤5 integrin is required for efficient binding of POS, and RPE cells from ␤5 Ϫ/Ϫ mice show markedly reduced binding of POS in vitro (Nandrot et al., 2004). Intriguingly, engagement of the ␣v␤5 integrin by its cognate ligand, milk fat globule-EGF8 (MFG-E8), is essential for the circadian synchronization of phagocytosis (Nandrot and Finnemann, 2006;Nandrot et al., 2007), and although phagocytosis of POS occurs in MFG-E8 Ϫ/Ϫ and ␤5 Ϫ/Ϫ mice, in both mutants the daily rhythm is absent. In contrast, focal adhesion kinase (FAK) and MerTK are not required for the initial binding of POS to the apical surface of the RPE, but they are sequentially activated by ␣v␤5 receptors and are essential for phagosome internalization (Feng et al., 2002;Finnemann, 2003).Between the pigment epithelium and neuroretina RPE cells extend apical processes into the interphotorecept...

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“…Moreover, we still do not know which RPE proteins serve as substrates for MerTK's kinase activity during RPE phagocytosis. However, both endogenous and overexpressed MerTK reveal a striking redistribution to the sites of internalized POS in in vitro phagocytosis assays suggesting that MerTK receptors may be components of the phagocytic machinery of the RPE (Feng et al, 2002;Finnemann, 2003 residues of MerTK in RPE in culture (Feng et al, 2002;Finnemann, 2003). Although their mutual dependence has not been demonstrated directly, levels of MerTK tyrosine phosphorylation commonly serve to assess the extent of MerTK activity.…”

Section: Role Of Mertk Activation In Rpe Phagocytosismentioning

confidence: 99%

Mertk Activation During RPE Phagocytosis in Vivo Requires αVβ5 Integrin

Finnemann

Nandrot

Retinal Degenerative Diseases

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Mertk Triggers Uptake of Photoreceptor Outer Segments during Phagocytosis by Cultured Retinal Pigment Epithelial Cells

Cited by 207 publications

References 26 publications

Bimodal in vivo imaging provides early assessment of stem-cell-based photoreceptor engraftment

Bimodal in vivo imaging provides early assessment of stem-cell-based photoreceptor engraftment

Annexin A2 Regulates Phagocytosis of Photoreceptor Outer Segments in the Mouse Retina

Mertk Activation During RPE Phagocytosis in Vivo Requires αVβ5 Integrin

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