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Previous Article | Next Article
The Journal of Neuroscience, October 1, 1999, 19(19):8435-8442
Drosophila presenilin Is Required for Neuronal Differentiation and Affects Notch Subcellular Localization and Signaling
Yiquan Guo1, Izhar Livne-Bar1, Lily Zhou1, and Gabrielle L. Boulianne1, 2 1 Program in Developmental Biology, Hospital for Sick Children, Toronto, Ontario, Canada M5G 1X8, and 2 Department of Medical Genetics and Zoology, University of Toronto, Toronto, Ontario, Canada
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Presenilins are a highly conserved family of proteins first identified as causative genes in early onset familial Alzheimer's disease. Recent studies have suggested a role for presenilins in the Notch-signaling pathway, but their specific function within this pathway remains unclear. Here, we have characterized the Drosophila presenilin gene and protein and studied their interaction with Notch in both mutants and transgenics. We find that the Drosophila presenilin protein is proteolytically cleaved and broadly expressed during development with the highest levels in neurons within the larval CNS. We also show that mutations in Drosophila presenilin (Dps) genetically interact with Notch and result in an early pupal-lethal phenotype characterized by defects in eye and wing development and incomplete neuronal differentiation within the larval CNS. Moreover, we find that processing of Notch in the Golgi by the furin protease is unaffected in Dps mutants and that Notch is present and may even accumulate on the plasma membrane of neuroblasts in the larval CNS of Dps mutants. In contrast, overexpression of Dps in transgenics causes Notch to accumulate in the cytoplasm. Taken together, these results indicate that Drosophila presenilin is required for proper neuronal differentiation and may regulate the subcellular localization of Notch proteins within cells, necessary for their accumulation and subsequent signaling capabilities.
Key words: Drosophila; presenilin; Notch; localization; Delta; neurogenesis
INTRODUCTION
Presenilins are a highly conserved, novel family of transmembrane proteins first identified as causative factors in familial Alzheimer's disease (Levy-Lahad et al., 1995
; Rogaev et al., 1995
To investigate the relationship between presenilin and Notch further, we have isolated and characterized mutations in the presenilin gene of Drosophila melanogaster. We find that loss-of-function mutations in Drosophila presenilin (Dps) are early pupal lethal with underdeveloped eye and wing imaginal disks and defects in neuronal differentiation. We also demonstrate that mutations in Dps genetically interact with Notch and Delta and show that Dps affects Notch subcellular localization. Specifically, we find that Notch is present and may even accumulate on the plasma membrane of neuroblasts in the larval CNS of loss-of-function Dps mutants. In agreement with this observation, we find that Dps does not affect the initial processing of Notch that occurs within the Golgi to produce a functional receptor at the plasma membrane. Finally, we also find that Notch accumulates in cells from transgenic flies that overexpress Dps. Taken together these results show that presenilins are required for neuronal differentiation and may play a role in Notch-signaling events by affecting the subcellular distribution and subsequent signaling capability of Notch.
MATERIALS AND METHODS
Fly strains. The deficiencies Df(1)N-8/In(1)dl-49, y1 Hw1 m2 g4, Dl[7]/TM2, and Df(3L)ri-79c/TM3 and the Notch alleles Nnd-3 and NAx-1 were obtained from the Bloomington Stock Center. Dps mutants were generated by imprecise P-element excision as described (Pirrotta, 1986
Immunoblots and immunocytochemistry. Wild-type or mutant Dps protein in immunoblots was detected from extracts derived from second instar larvae, late third instar larvae, or early pupae and from transgenics carrying either a heatshock-Dps transgene or UAS-Dps expressed from a daughterless-GAL4 driver. Immunoblots and immunocytochemistry were performed using affinity-purified Dps-specific antibodies generated to an N-terminal peptide corresponding to amino acids 28-43 of Dps or a C-terminal peptide corresponding to amino acids 520-538. Affinity purification of the antibody was performed using the ImmunoPure Ag/Ab Immunobilization Kit (Pierce, Rockford, IL). Primary antibodies were detected with either HRP-conjugated (immunoblots) or fluorescein- or rhodamine-conjugated secondary antibodies (immunocytochemistry) (Jackson ImmunoResearch, West Grove, PA). Immunoblots to detect Notch protein were performed using the monoclonal antibody C17.9C6 (kindly provided by Dr. S. Artavanis-Tsakonas) that recognizes the intracellular domain of Notch (1:3000). To control for loading, we stained immunoblots with Ponceau S. Double-labeling of imaginal disks and CNS from wild type and Dps mutants was performed using rat ELAV antibody 7E8A10 (Developmental Studies Hybridoma Bank) and mouse CUT antibody (a gift from Dr. K. Blochlinger). The subcellular localization of Notch in Dps mutants was detected in the CNS of second or late third instar larvae by immunocytochemistry using the monoclonal antibody C17.9C6 to the intracellular domain of Notch (kindly provided by Dr. S. Artavanis-Tsakonas) (Fehon et al., 1990
RESULTS
Molecular organization of the Drosophila presenilin gene
We and others have reported previously the cloning of the Drosophila presenilin gene and shown that it encodes a protein with over 50% amino acid identity to its vertebrate counterparts (Boulianne et al., 1997
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Figure 1. Genomic organization and deletion analysis of the Dps locus. The genomic organization of the Dps gene was determined by sequencing genomic DNA obtained from a P1 clone (#DS03069; Berkeley Drosophila Genome Project) and from genomic DNA obtained after plasmid rescue from the P4 insertion line (GenBank accession number, AF093402) as described (Pirrotta, 1986
Dps is proteolytically cleaved and broadly expressed during development
To examine the processing as well as the cellular and subcellular distribution of Dps during development, we raised polyclonal antibodies to the N- and C-terminal domains of Dps. In agreement with previous Northern blot analyses (Boulianne et al., 1997
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Figure 2. Dps is proteolytically cleaved. Immunoblot analysis of second instar larval extracts from wild type (wt) and mutants indicates that Dps is proteolytically cleaved to give rise to a 25 kDa N-terminal fragment (a) and a 35 kDa C-terminal fragment (b) that are absent from the deletion mutants W6 and W11. Full-length protein can only be detected in third instar larval extracts of transgenic flies that overexpress Dps from a heatshock promoter (hs-Dps) or use a daughterless-GAL4 driver (da-Dps) (c). In the absence of GAL4, only the N-terminal fragment is detected with the N-terminal-specific Dps antibody.
Mutational analysis of Dps
To examine the function of Dps, we generated a series of overlapping deletions by imprecise P-element excision of P4, a homozygous viable P-element insertion located ~1 kb 3' of the Dps gene (Fig. 1). In total, we have generated six deletions, three of which remove portions of the Dps coding region (DpsW20, DpsW6, and DpsW11). All of the deletions fail to complement each other, and none produce any detectable Dps protein as determined by Western blot analysis on extracts from mutant larvae (Fig. 2a,b). The largest deletion (DpsW20) deletes the Dps gene as well as portions of the lipoic acid synthase and the 50 S ribosomal protein L15 genes and is embryonic lethal. DpsW11 and DpsW6 that delete Dps and the 50 S ribosomal protein L15 genes are lethal during the second larval instar, and these larvae are small and grow at a much slower rate.
In addition to the deletion mutants in Dps we have also characterized two EMS alleles, Dps30 and Dps46 (kindly provided by L. Pallank and B. Ganetzky), that were originally identified in a lethal screen over the deficiency Df(3L)ri-79c/TM3 that uncovers the Dps locus and has break points at 77B-C;77F-78A. Both EMS lines fail to complement each other as well as the two Dps deletions we tested, DpsW6 and DpsW11. To determine the molecular basis of these mutations, we sequenced both Dps30 and Dps46. To date, we have been unable to identify a mutation within the coding region of Dps30 and are currently searching for alterations in surrounding regulatory sequences. However, we have found a single missense mutation in Dps46, consisting of a proline to leucine substitution at amino acid 507 within the highly conserved C-terminal domain of Dps.
To address the function of Dps during development, we examined the phenotype in flies of the genotype Dps46/DpsW6 or Dps46/DpsW11 that are mutant for Dps but wild-type for lipoic acid synthase and hemizygous for the 50 S ribosomal protein L15 gene. We find that these mutants are early pupal lethal; the third instar larvae form a pupal case, but no adult structures develop. When we examined the phenotype of the mutants during the late third larval instar stage, we found that the mutant larvae have underdeveloped eye (Fig. 3b,e) and wing (Fig. 3c,f) imaginal disks. Although the eye imaginal disk forms, it fails to undergo proper neuronal differentiation (Fig. 3a,d). The wing imaginal disk is also smaller with the most severe defects observed in the region that will give rise to the wing blade (Fig. 3f). Furthermore, Wingless expression, which is normally detected in two domains within the developing disk, is disrupted in Dps mutant disks (Fig. 3c,f). In contrast, both the antennae and leg imaginal disks appeared normal. Both the lethality as well as the wing and eye phenotypes could be rescued using a Dps transgene driven by a heatshock promoter. To determine whether there was any evidence of neuronal differentiation within the eyes and optic lobes of our pupal lethal mutants, we also examined the expression of two neuronal markers, ELAV (Robinow and White, 1988
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Figure 3. Dps mutants fail to undergo proper neuronal differentiation within the optic lobe anlagen and the eye imaginal disk. a, Wild-type CNS and disks derived from late third larval instar and double-immunostained for CUT (green) and ELAV (red). Note the precise laminar array organization of the optic lobe anlagen (OL) and the regular array of neurons within the developing eye imaginal disk (long arrow). At this stage, CUT expression is also abundant in developing antennal disk (short arrow). b, DAPI staining of disks demonstrating the overall morphology of wild-type eye (arrow) and antennae (arrowhead) disks. c, Wild-type wing imaginal disks immunostained for WINGLESS. Note the normal distribution of wingless in the dorsal region of the wing disk in regions that will give rise to the adult notum and hinge (h) and the ventral staining in regions of the wing blade (wb) that will give rise to the wing margin. d, CNS and imaginal disks from Dps46/DpsW11 late third larval instar. Note the general disorganization of the optic lobe anlagen (OL) and the absence of ELAV expression in the eye imaginal disk (long arrow). In contrast, expression of CUT in the antennal disk appears normal (short arrow). e, DAPI staining of disks from Dps46/DpsW11 mutants. Although the antennae disk (arrowhead) appears normal, the eye disk (arrow) is small and disorganized. f, Wing imaginal disks from Dps46/DpsW11. WINGLESS expression appears normal in the dorsal compartment in regions that will give rise to the notum and hinge (h) but is absent from ventral regions that give rise to the wing blade and margin (wb).
Dps genetically interacts with Notch and Delta
A role for presenilins in the Notch-signaling pathway has been suggested previously by studies in both C. elegans (Levitan and Greenwald, 1995
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Figure 4. Dps genetically interacts with Notch and Delta. Dps mutants can modify the phenotype of both Notch and Delta alleles in transheterozygotes. a, Wild type. b, Dps46. c, DpsW11. d, Df(1)N-8. Note the mild notching at the wing tip (arrow). e, Df(1)N-8; Dps46. The Dps mutations (e, f) enhance the notching at the wing tip (arrow). f, Df(1)N-8; DpsW11. g, Nnd-3. Note the thickening of wing vein L3 (arrow). h, Nnd-3; Dps46. The Dps mutations (h, i) enhance the phenotype at the wing veins (thin arrows) and cause notching at the wing tips (thick arrow). i, Nnd-3; DpsW11. j, NAx-1. Note the interruption of wing vein L5 and the absence of L2 (arrows). k, NAx-1; Dps46. Note that the Dps mutation suppresses partially the interruption of L5 and restores L2 (arrows). l, NAx-1; DpsW11. m, Dl[7]. Note the thickening of the wing veins and the slight delta between L4 and L5 (arrows). n, Dl[7]; Dps46. Dps mutants also enhance the wing vein phenotype of Delta mutants in transheterozygotes. Note the enhanced thickening of the wing veins and deltas (thin arrows, thick arrow). o, Dl[7]; DpsW11.
Dps affects the subcellular localization of Notch
To gain insight into the mechanism underlying Dps and Notch interactions, we performed immunocytochemical studies to examine the subcellular distribution of Notch within the larval CNS of Dps mutants. Using an antibody that recognizes the Notch intracellular domain, we find that Notch is expressed at high levels within neuroblasts throughout the proliferative centers in the developing optic lobes and at somewhat lower levels in neuroblasts within the thoracic ganglia of third larval instar CNS as reported previously (Kidd et al., 1989
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Figure 5. Notch staining is increased on the plasma membrane in the third larval instar CNS of Dps mutants. a, c, The distribution of Notch protein in the CNS of wild-type third instar larvae is shown at low (a) and high (c) magnification. Notch is expressed at high levels in the optic lobe anlagen and imaginal disks (a). Within the CNS, Notch protein is detected within the cytoplasm and the plasma membrane (c). b, d, In the CNS of Dps mutants, the overall pattern of Notch expression is affected (b), and the protein levels are reduced in the cytoplasm and increased on the plasma membrane (d). e, f, In contrast, the distribution of HRP on the plasma membrane is unaffected in Dps mutants. In wild type (e), HRP is found on the entire surface of neuroblasts in the CNS, and the same pattern of expression can be observed in Dps mutants (f).
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Figure 6. Notch staining is increased on the plasma membrane in the second larval instar CNS of Dps mutants. a, In wild-type second larval instar CNS, Notch expression is observed throughout the cytoplasm of neuroblasts and at high levels at the plasma membrane in regions of contact between the neuroblast and its progeny (arrow). b, c, In the CNS of Dps mutants, Notch expression is increased on the entire surface of the plasma membrane (thick arrows) and at the regions of contact between cells (thin arrow). d, Processing of Notch to give rise to a functional heterodimeric receptor is unaffected in Dps mutants. Protein extracts were obtained from isolated CNS and imaginal disks from wild-type and Dps homozygous mutant third larval instars. No significant differences were observed in the levels or processing of Notch in Dps mutants compared with that of wild type.
We have also performed the reciprocal experiment to determine whether overexpression of Dps also affected the subcellular distribution of Notch. Specifically, we used the GAL4/UAS system (Brand and Perrimon, 1993
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Figure 7. Notch staining is increased in the cytoplasm of Dps-overexpressing cells. The distribution of Notch and Dps in third instar larval wing disks is shown. a, In wild-type disks, Dps protein is expressed at very low levels. b, Notch is expressed ubiquitously throughout the larval wing disk. c, d, Dps protein can be induced in wing (thin arrow) and haltere (thick arrow) disks using a pnr-GAL4 line to drive expression of UAS-Dps in transgenic lines (c). Notch protein specifically accumulates in cells overexpressing Dps (d). e, f, cut-GAL4 was used to overexpress Dps at the developing wing margin. Note the high levels of Dps protein that accumulate in the cytoplasm of cells at the wing margin (e, arrow). Overexpression of Dps at the margin causes Notch to accumulate within the cytoplasm of these cells (f, arrow). g, h, Overexpression of Dps in a subset of neurons within the developing eye disk (g, arrow) also causes increases in Notch expression within the cytoplasm of these cells (h, arrow).
DISCUSSION
We have used Drosophila melanogaster to study the function of presenilin and to investigate its role in the Notch-signaling pathway. In Drosophila, presenilin is encoded by a single gene whose overall intron-exon structure and splice sites are highly related to that of both the C. elegans and vertebrate presenilins (Boulianne et al., 1997
As found in its vertebrate and C. elegans counterparts, we find that the majority of Dps is proteolytically cleaved and gives rise to a 25 kDa N-terminal fragment and a 35 kDa C-terminal fragment, although full-length Dps can be detected in transgenic flies that overexpress Dps under a variety of promoters. The fact that presenilins are processed in worms, flies, and vertebrates suggests that this is a functionally important event and that the cellular machinery involved in this processing must be highly conserved between species. This is in contrast to previous studies in C. elegans that demonstrated that a naturally occurring mutation (PS1
E9) that deletes exon 9 and removes the cleavage site is capable of rescuing a sel-12 mutant, thereby suggesting that proteolytic processing of presenilins was not essential for function (Levitan et al., 1996
Using immunocytochemical techniques, we find that Dps is broadly expressed during development with higher levels in some tissues, including the larval CNS where the protein accumulates within the cytoplasm of neurons. This is consistent with a recent study showing that Dps is ubiquitously expressed throughout the cytoplasm during development with elevated levels in the larval and pupal optic lobes (Ye and Fortini, 1998
Dps mutations also enhance the wing phenotype of Notch and Delta loss-of-function mutants and suppress the phenotype of a Notch gain-of-function mutation, indicating that the signaling through the Notch receptor is reduced in Dps mutants and that the role of Dps in Notch signaling is not limited to the nervous system. More importantly, Notch is maintained and may even accumulate at the plasma membrane of neuroblasts in flies lacking Dps, whereas overexpression of Dps causes Notch to accumulate within the cytoplasm. Taken together, these data imply either that the cell surface Notch that we observe in Dps mutants is nonfunctional, unable to interact properly with its ligand, or that Dps blocks signal transduction events that occur at the membrane or after Notch is internalized from the membrane. Processing and trafficking of Notch receptors are known to be important for Notch signaling (Blaumueller et al., 1997
-secretase cleavage of amyloid precursor protein (APP), suggests that presenilin may have
In our studies, we find that Notch is uniformly distributed and may even accumulate on the entire plasma membrane of neuroblasts in Dps mutants. This is in contrast to wild-type situations in which Notch specifically accumulates at the interface of ligand-expressing cells during signaling both in cell culture and in vivo. Therefore, presenilin may be affecting targeting of Notch to the appropriate location on the membrane where it can interact with ligand. In the absence of ligand interaction, proteolytic processing of Notch does not occur. Alternatively, Dps could be required for internalization of the receptor-ligand complex and subsequent proteolytic processing because it is not known where within the cell these cleavage events occur. Although presenilin in mammals is thought to reside predominantly in the endoplasmic reticulum (ER) and Golgi, consistent with possible roles in early stages of protein processing, some evidence suggests that it may transiently reach the plasma membrane (Dewji and Singer, 1997
A role for presenilin in protein processing or trafficking has been suggested previously on the basis of its subcellular localization (Kovacks et al., 1996
(40) and A
FOOTNOTES Received April 30, 1999; revised June 15, 1999; accepted June 30, 1999.
Y.G. was supported by a Research Training Award from The Hospital for Sick Children and a fellowship from the Alzheimer's Society of Canada. This work was supported by grants to G.L.B. from the Medical Research Council of Canada, the Alzheimer's Association, and the American Health Assistance Foundation. We thank W. S. Trimble, E. Yeh, and S. E. Egan for useful discussions and critical review of this manuscript. We also thank P. Simpson, K. Blochlinger, K. Kaiser, and P. Deck for providing several of the fly lines used in this study. We especially thank Leo Pallank and Barry Ganetzky for providing us with EMS alleles and S. Artavanis-Tsakonas and K. Blochlinger for generously providing us with antibodies to Notch and Cut, respectively.
Y.G. and I.L.-B. contributed equally to this work.
Correspondence should be addressed to Dr. Gabrielle L. Boulianne, Program in Developmental Biology, Hospital for Sick Children, 555 University Avenue, Toronto, Ontario, Canada M5G 1X8.
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