Distant activation of Notch signaling induces stem cell niche assembly
Authors:
Andriy S. Yatsenko aff001; Halyna R. Shcherbata aff001
Authors place of work:
Institute of Cell Biochemistry, Hannover Medical School, Hannover, Germany
aff001
Published in the journal:
Distant activation of Notch signaling induces stem cell niche assembly. PLoS Genet 17(3): e1009489. doi:10.1371/journal.pgen.1009489
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pgen.1009489
Summary
Here we show that multiple modes of Notch signaling activation specify the complexity of spatial cellular interactions necessary for stem cell niche assembly. In particular, we studied the formation of the germline stem cell niche in Drosophila ovaries, which is a two-step process whereby terminal filaments are formed first. Then, terminal filaments signal to the adjacent cap cell precursors, resulting in Notch signaling activation, which is necessary for the lifelong acquisition of stem cell niche cell fate. The genetic data suggest that in order to initiate the process of stem cell niche assembly, Notch signaling is activated among non-equipotent cells via distant induction, where germline Delta is delivered to somatic cells located several diameters away via cellular projections generated by primordial germ cells. At the same time, to ensure the robustness of niche formation, terminal filament cell fate can also be induced by somatic Delta via cis- or trans-inhibition. This exemplifies a double security mechanism that guarantees that the germline stem cell niche is formed, since it is indispensable for the adjacent germline precursor cells to acquire and maintain stemness necessary for successful reproduction. These findings contribute to our understanding of the formation of stem cell niches in their natural environment, which is important for stem cell biology and regenerative medicine.
Keywords:
Actins – Cell differentiation – Morphogenesis – Notch signaling – Ovaries – Precursor cells – Signal inhibition – Stem cell niche
Introduction
The Notch pathway is an evolutionarily conserved signaling pathway that presents a great assortment of complex behaviors in various developmental situations. During development, cells often express both the Delta ligand and Notch receptor; therefore, they are undecided with regards to Notch signaling status (Fig 1A). This indecisiveness can be resolved randomly over a period of time; for example, when one cell expresses more Notch or Delta due to transcriptional noise, then the adjacent cell accepts the opposite cell fate [1–3]. However, most of the time, in order to generate a stable Notch signaling pattern required for proper tissue organization, Notch signaling is activated via cell-to-cell interactions.
In particular, among a group of equivalent cells, Notch signaling activation induces mutually exclusive cell fates in the adjacent cells in a process called “lateral inhibition”. In this case, the membrane-localized Notch ligand (Delta or Serrate) binds to the Notch receptor on the membrane of the neighboring cell. With the help of mechanical forces, Delta-Notch interaction causes Notch receptor cleavage and translocation of its intracellular domain to the nucleus. There it serves as a transcriptional co-factor that activates expression of Notch-dependent genes, which include repressors of Delta ligand [4–6]. This typical short-range Notch activation via lateral inhibition is seen in multiple tissues of evolutionarily diverse species [7–11]. In addition, it has been shown that in the epithelial cells within imaginal discs, long-range Notch lateral inhibition exists, which is mediated by Delta-promoted planar filopodia. These dynamic filopodia transmit intermittent Delta-Notch signaling, which refines Notch signaling during mechanosensory bristle formation and even can promote tumorigenesis in the mesenchymal cells [12–15].
In contrast to lateral inhibition, which occurs between equipotent cells, Notch signaling is activated via “peripheral induction” between non-equipotent cells. In particular, here we distinguish two types of inductive Notch signaling: if non-equipotent, communicating cells are juxtaposed and Notch signaling is activated in those cells adjacent to the Delta-sending cell, it is called “local induction”; if non-equipotent, communicating cells are distant and a plane of Delta-sending cells signals to one or more layers of Delta-receiving cells, it is called “distant induction” (Fig 1A). Importantly, local induction is sharp, while distant induction could result in graded activation of Notch signaling. In all of the Notch signaling modes described above, Notch signaling activation occurs as a result of trans-interactional communication that happens between the cells, membranes of which are in direct contact or between detached cells with the help of cellular projections. In each mode, amounts of Notch and Delta presented on the interacting membranes are different; therefore, the efficiency of Notch signaling activation depends on cell-cell contact geometry [16].
In addition to trans-activating, Notch and Delta expressed on the same cell surface can form cis-inhibitory complexes, resulting in intrinsic Notch signaling repression [17–20]. Recently, a trans-inhibition mode has been proposed, wherein Delta just binds Notch at cell-to-cell junctional contacts, which, without mechanical pulling force, does not translate into Notch receptor cleavage and activation. This allows larger groups of neighboring cells to express high levels of Delta [21].
In all cases, acquisition of a certain Notch signaling status generates mutually exclusive signaling states between groups of cells that subsequently activate genes coding for factors establishing terminally differentiated cell fates [4,6,14,22].
To study the interplay of Notch signaling activation modes necessary for proper cell fate acquisition and tissue patterning in vivo, we focused on the process of Drosophila ovarian stem cell niche formation as a model system. In the Drosophila ovary, the stem cell niche size directly depends on the strength of Notch signaling: when Delta ligand is overexpressed, it induces enlarged, functional niches, regardless of whether Delta is overexpressed in the germline or soma [23,24]. These data imply that the stem cell niche morphogenesis could be differentially patterned depending on the strength and the source of Delta expression. However, it is undetermined what is the source of Delta and whether the germline communicates with the soma to confer Notch patterning necessary for proper stem cell niche formation.
The onset of Drosophila ovarian morphogenesis is marked by a merger of the primordial germline cells (PGCs) with the somatic gonad precursor cells, which occurs during early embryonic development (Fig 1B). This results in the formation of round, paired gonads in the abdominal region of the embryo, in which germline and somatic cells are intermingled. Both cell types divide mitotically and do not differentiate [25–28]. Only after the second instar larval stage [L2, 72h after egg laying (AEL)], based on their anteroposterior location within the embryo, somatic cells begin to differentiate into round-shaped apical (ACs) and basal cells (BCs), as well as squamous intermingled somatic cells (ICs) that envelop individual PGCs (Fig 1B). At the late third instar larval stage (LL3, 118h AEL), the ovary elongates, as a group of ACs called swarm cells (SCs) begins to migrate posteriorly, probably inducing mechanical forces that allow changes in the shape of the organ [29]. The differentiation of somatic cells progresses, resulting in the appearance of short cylindrical terminal filament cells (TFCs) that form separate terminal filament (TF) stalks (Fig 1B). At the base of each stalk, six ICs change their shape into ellipsoid and acquire a stem cell niche cell fate for life [26,30,31]. These cells are called cap cells (CpCs), and they generate signals necessary for germline stem cell maintenance. Therefore, PGCs that are in direct contact with CpCs become germline stem cells (GSCs), while other PGCs that are enveloped by escort cell precursors (ECs) will differentiate [23,24,32–37]. This concludes the assembly of the functional GSC niche unit, which consists of one TF, CpCs, antrerior ECs, and GSCs and is responsible for GSC self-renewal during the lifetime. Individual GSC niche units are separated by extracellular matrix deposited by a group of posteriorly migrating ACs called sheath cells (SHC), resulting in the formation of individual ovarioles.
Thus, the GSC niche formation is a sequential process in which the TFs are assembled first, followed by specification of CpCs, which act as the niche cells [31,33]. While it is known that Notch signaling activation is essential for the GSC niche cell fate [23,24,33,38,39], it is not clear whether it also plays a role in TF cell specification. To understand the role of Notch signaling in the stem cell niche assembly, we aimed: i) to identify the physiological sources of Delta that chronologically induce Notch signaling in the somatic cell precursors and ii) to distinguish via what modes Notch signaling is activated in the process of acquiring different cell fates by niche cells.
Here we found that the key components of the pathway, Delta and Notch, have dynamic expression patterns, which affects the spatiotemporal pattern of Notch activity. Our data show that the Notch signaling pathway controls both major steps of GSC niche formation (TF assembly and CpC specification), and its activation modes vary significantly depending on the cell type and the sources of the Delta ligand. First, acquisition of a certain Notch signaling status (ON or OFF) is required for proper TF assembly. Depending on the TFC precursor position with regards to the germline, it would have Notch signaling either activated by the germline Delta via trans-interaction or inhibited by the somatic Delta. Importantly, the germline delivers Delta across several cell diameters to the somatic precursor cells plausibly via PGC-generated projections, resulting in the long-range induction of Notch signaling. At the same time, to ensure robustness of ovarian organogenesis, TF cell fate can be also induced by the inhibition of Notch signaling in the somatic TF precursors. Since TF establishment is a pre-requisite for the stem cell niche formation, activating and inhibitory Delta interaction modes offer a double security mechanism which guarantees that these events occur. Later, the Delta ligand expressed by the posterior TF cell activates Notch signaling in the adjacent somatic cells and transforms them into CpCs, which concludes the two-step process of the stem cell niche formation. Notch-induced cell differentiation is accompanied by alteration in size, shape and position of TFCs and CpCs. In summary, our data show that in the process of germline stem cell niche assembly, multiple layers of Notch signaling pathway activation (ON/OFF, low/high) define the accuracy of cell fate choice.
Results
Notch signaling mutants have impaired GSC niche morphogenesis
To study the role of Notch signaling in coordination of stem cell assembly, we analyzed and compared developing ovaries of wild-type and Notch signaling mutants. Conveniently, in the developing ovary, all different cell types can be easily identified using specific markers. Upon differentiation, precursor cells start to express distinctive sets of proteins; for example, TFCs can be marked by expression of the transcription factor, Engrailed (En, Fig 1C), while ICs express another transcription factor, Traffic jam (Tj, Fig 1C), and CpCs express a combination of these two factors (En+Tj, Fig 1C, green+red = yellow). The PGCs can be distinguished based on the presence of proteins that are exclusive for the germline (e.g., Vasa, Fig 1C, blue). Using these multiple markers, we analyzed the organization of the prepupal ovaries, in which niche formation is already completed. We compared the GSC niches of controls and Notch signaling mutants, in particular, we studied Notch (Nts1) temperature-sensitive mutants. Due to lethality, these mutants were kept at the restrictive temperature (25°C) only during the timeframe of the niche formation (late L2—early prepupa). We found that stem cell niche morphogenesis was severely affected in Nts1 mutants—TFs were abnormally shaped, had irregular length and lost their anteroposterior orientation (Fig 1D, arrows). These data suggest that Notch signaling is involved in the process of germline stem cell niche assembly, the TF morphogenesis.
In the developing ovary, the pattern of Notch signaling activation is dynamic
Since the dynamics of Notch signaling in the developing ovary have not been studied before, we analyzed the timing and spatial expression pattern of the key components of Notch signaling–the major Notch signaling ligand, Delta and its receptor, Notch, as well as a Notch activity reporter during different stages of ovarian morphogenesis. It is important to note that depending on the Notch signaling status, the expression pattern and subcellular localization of the Notch receptor and the Delta ligand change. When Notch signaling is activated, membrane-localized Notch interacts with the activated membrane Delta from the other cell (Fig 1A, blue and yellow cells). This generates a pulling force resulting in Notch cleavage and translocation of its intracellular domain to the nucleus [40]. Since endocytosis is essential for Delta activation, activated Delta can be distinguished by its vesicular localization [41]. Nuclear Notch is difficult to detect with antibodies; therefore, Notch signaling activation is depicted as membrane Notch disappearance [42]. However, absence of the signal can also result from the inhibition of Notch expression; therefore, it is more reliable to analyze Notch signaling activation using Notch signaling reporters. At the same time, co-analysis of Notch and Delta expression patterns can be helpful to analyze other Notch signaling modes, such as when Notch signaling is inhibited [18,21]. In these cases, high levels of non-activated Delta are present at the cell membranes. This Delta can bind the Notch receptor in cis- or trans-, but cannot cause its cleavage and activation, leading to Notch signaling inhibition (Fig 1A, light blue cells). Therefore, high Delta and low Notch are co-present on the membranes of the cells in which Notch signaling is inhibited; however, it is impossible to distinguish between extrinsic Delta-trans and intrinsic Delta-cis inhibition. In addition, cells that express relatively high levels of Notch and Delta can be still undecided with respect to their Notch signaling status (Fig 1A, olive cell).
Firstly, to detect active Notch signaling, we used a Notch signaling reporter in which the sequence encoding rat CD2 protein is inserted downstream of the Enhancer of Split [E(spl)mß] promoter, which is activated by Notch signaling [43]. We were intrigued to note that the activation of Notch signaling coincides with the onset of GSC niche morphogenesis. In particular, at the early third instar larval stage (EL3) a small group of ACs adjacent to the germline start to express the Notch signaling reporter (Fig 2A, cyan arrows). Then, at later stages, CpCs adjacent to TFs also have active Notch signaling (Fig 2B–2D, yellow arrows). This suggests that in the stem cell niche precursor cells, Notch signaling plays a role in the terminal cell fate acquisition by both cell types comprising the stem cell niche unit (TFCs and CpCs).
Secondly, we analyzed Delta and Notch protein localization and found that both proteins have highly dynamic spatiotemporal expression patterns (Figs 2 and S1A–S1C). In particular, the Delta ligand is expressed in both the germline and the soma (Fig 2A–2C, lower panel). In the germline, higher levels of Delta are observed at earlier stages, and as ovarian morphogenesis progresses, Delta levels decrease (magenta arrows). We confirmed the specificity of Delta protein expression in PGCs by analysis of mutant ovaries with germline-specific Delta downregulation (S1D and S1E Fig).
Similarly, in the ovarian soma, the Delta expression pattern is dynamic, and Delta levels in general decrease at later stages of development. At EL3 stage, all ACs, including precursors of TFCs, express both Delta ligand and Notch receptor (compare lower panels in Figs 2A and S1A–S1C). Later, the expression of the Notch activity reporter indicates Notch signaling activation in TFCs. However, we noticed that not all TFCs turned “on” Notch signaling (Fig 2B, anterior and posterior TFCs, cyan arrowheads and cyan arrows, respectively). In particular, anterior TFCs express high levels of Delta and do not express the Notch activity reporter, suggesting that Notch signaling could turned “off” in these cells by the somatic Delta. At the same time, posterior TFCs adjacent to the germline lose membrane Delta and Notch and express the Notch activity reporter, suggesting that Notch could turned “on” in these cells by the germline-originated Delta.
The analysis of expression patterns of the Notch receptor and Delta ligand in CpC precursors shows that at early stages of development (EL3), ICs express both proteins (Figs 2A and S1A, yellow arrows), indicating that these cells are in an undecided state. Later, at LL3 and Prepupa, the presence of Delta and Notch at the membranes of ICs is strongly reduced (Figs 2B, 2C, S1B and S1C, yellow arrows). This accords with the onset of Notch signaling activation in a group of ICs adjacent to the TFs, which actually acquire the CpC fate (Figs 2B, 2C and S1A, yellow arrows). Notably, the efficiency of Notch signaling activation in CpCs, as detected by the expression levels of the Notch activity reporter, is lower than in TFCs, indicating that the intensity of Notch signaling is different in these two types of stem cell niche cells.
In summary, the expression pattern analysis demonstrates that the dynamics of Notch signaling in the developing niche cells are spatiotemporally complex and depend on the cell differentiation state. In particular, it is interesting that cells have to switch from the bivalent (Notch and Delta co-expression) to the decided (Notch “off” or Notch “on” and Notch “high” or Notch “low”) state in the course of their differentiation. Next, we wanted to understand how Notch signaling activation is accomplished in these cells during ovarian morphogenesis.
Stem cell niche precursors acquire active Notch signaling status via different mechanisms
TFCs and CpCs derive from different types of somatic precursor cells: TFCs from ACs that are anteriorly located in the ovary; and CpCs from ICs that are medially located and intermingled with PGCs [29,32,33,44]. Upon differentiation, these cells adopt quite distinct shapes: cylindrical TFCs that arrange in the shape of a string (Fig 2E) and ellipsoid CpCs that unite in a shape resembling a flower with six petals (Fig 2F). They also have very different Notch/Delta expression patterns; however, both cell types acquire a certain Notch signaling status as they undergo terminal differentiation (Fig 2C, CD2, cyan and yellow arrows). Since TFCs and CpCs are spatially organized in a different manner and temporally induced to differentiate at different stages, we wanted to understand the sources of Delta signal that specifically control their organization and induce their active Notch status.
We analyzed Notch activity and Delta protein expression in a single TF in greater detail and found that Notch signaling displays a differential activity pattern as visualized by the fluorescent intensity of the Notch activity reporters (S2 Fig). In particular, the TFCs positioned next to the germline showed Notch activation, while cells at the anterior half of the TF showed no Notch activity (S2 Fig). Thus, the response to Delta observed here suggests that for the posterior TFC specification, Notch signaling activation occurs via an inductive mode, in which Delta signal originating from the germline activates Notch signaling via trans-interaction in the adjacent TFC precursors via distant induction (as schematically depicted in Fig 1A).
At the same time, anterior TFCs are positioned >4 cells away from the germline, which makes them less accessible for trans-interactions. Unlike the posterior TFCs, instead of the Notch signaling activity reporter, they express high Delta (Fig 2B and 2C, cyan arrowheads). Thus, the analysis of Notch signaling activation in the TFCs shows that despite the fact that TF cells originate from the same somatic precursor cells (ACs), look identical, and are similarly organized into a filament, they are quite different in terms of Notch signaling activity. We propose that anterior TFCs have Notch signaling inhibited possibly via intrinsic or extrinsic Delta-Notch inhibition, while posterior TFCs have Notch signaling induced via trans-activation as a response to Delta produced by the germline (Fig 2E).
Notably, the most posterior TFC (S2A Fig) has weaker Notch signaling activity due to the fact that the status of this cell (with regards to Notch signaling) is reprogrammed, which happens after the TF is formed and in response to steroid signaling [31]. Actually, this Delta-sending TFC serves as a source of the Delta ligand, which via peripheral induction induces Notch signaling in the adjacent niche cell precursors to convert them into CpCs and to ensure the formation of the stem cell niche (Fig 2F).
Importantly, Notch signaling activity continues to be very dynamic and changes as ovarian organogenesis progresses. After the process of stem cell niche differentiation is finalized, all TFCs and CpCs have Notch signaling activated (Fig 2D), while in the adult germarium, only few TFCs and CpCs have Notch signaling “on” (S3 Fig). During adulthood, CpCs co-express Notch and Delta and according to the rules of lateral inhibition, if at least one cell shifts the balance to express more Notch or Delta, it immediately will initiate the opposite (Delta or Notch) cell status in the adjacent neighbor [7,19,22,45]. Thus, CpCs have a stochastic Notch activity pattern (S3 Fig), suggesting that they per se can be responsible for the maintenance of Notch signaling activity in the adult GSC niche.
Notch signaling plays a role in TF formation
The formation of individual TF stacks precedes CpC specification; however, the role of Notch signaling in TF morphogenesis has not been studied before. TF formation is induced by the rearrangements of anterior cells adjacent to PGCs, which coincides with an acquisition of Notch active status by these cells (as shown above). TF precursor cells cease their division, change shape from spherical to ellipsoid to cylindrical, and increase cell adhesiveness. This attracts the neighboring cells and, in a wave-like fashion, induces cell intercalation into TF stacks [26,44,46–49]. Since the expression analyses demonstrate that Notch signaling is differentially patterned in TF precursors, we hypothesized that the Notch pathway controls the formation of individual TF stacks, which is the first step of GSC niche morphogenesis.
TFs are similar in their organization to the stalk cells in adult ovaries. It has been previously shown that the length of stalks separating individual egg chambers corresponds to the amount of Notch signaling [50,51]. We tested if this is also the case for the TFs by altering Notch and Delta levels. Downregulation of the Notch receptor resulted in TFs containing fewer TFCs with abnormal shapes. Contrarily, overexpressing Delta caused more somatic cells to choose a TF cell fate: in general, individual TFs contained more TFCs (compare Figs 1D and 3B). Also, TFs of Notch mutants appeared to be abnormally shaped and exhibited cell intercalation defects (S4 Fig), which were similar to the Notch mutant phenotypes in stalks of adult ovaries [50,51]. Together, these data support the hypothesis that Notch signaling has a functional role in TF morphogenesis and that the number of cells accepting the TF cell fate is proportional to the extent of Notch signaling activation. However, it is not clear how the Notch signaling pathway is induced in TFC precursors, what is the source of Delta, and whether the germline communicates with the soma in the process of TF formation.
Germline Delta activates Notch signaling in the posterior TFC precursors
Our examination of Notch signaling patterns in the developing TFs and analysis of Notch signaling mutants demonstrates that Notch signaling plays a role in the establishment of the TF cell fate and suggests that this fate can be induced via various Notch signaling modes that act in parallel: (1) germline Delta induces Notch signaling in the posterior TFCs and (2) somatic Delta represses Notch signaling in the anterior TFCs.
Firstly, to investigate the influence of germline Delta on TF formation, we overexpressed Delta specifically in PGCs. We closely examined individual TF organization in the prepupal ovaries and quantified the number of TFCs incorporated into each TF. Normally, there is not much variation in the number of TFCs per TF– 80% of TFs have exactly 8, and the other 20% have 7 or 9 TFCs incorporated into one TF stalk (Fig 3A–3J, green and blue curves, and S1A–S1C Table). This narrow distribution suggests that the process of TF formation is very robust. However, the increased expression of Delta in the germline had a dramatic effect on TF specification (Fig 3B). The number of TFCs per TF ranged from 4 to 14, and the average TFCs/TF number was significantly increased when compared to controls (Fig 3D, purple, and S1A Table). These data show that overexpression of Delta in the germline leads to an increase in TFC specification. This is consistent with previously published data demonstrating that the amount of Delta affects the strength of Notch signaling [23].
Secondly, to show that Delta from the germline plays a role in TF morphogenesis, we downregulated Delta specifically in the germline, which again resulted in a broader distribution in the number of TFCs per TF, where many TFs appeared to have reduced numbers of TFCs/TF (Fig 3C and 3D, magenta, and S1A Table). These data show that hypo-induction of Notch signaling caused by Delta downregulation in the germline decreases the number of somatic precursors adopting a TF cell fate.
Thirdly, to confirm that germline Delta is essential for TFC specification, we analyzed what happens in the absence of germline-produced Delta. In particular, we analyzed TFs in tudor maternal effect mutants that completely lack germline cells. Consistent with a previous study [33], we found that while TFs were formed in the germline-less ovaries, their appearance was dramatically impaired, and the numbers of TFCs per TF were significantly reduced (Fig 3E and 3F, orange, and S1A Table). These data show that germline Delta plays an instructive role, but it is not essential for TF assembly.
Fourthly, to test whether activation of Notch signaling in somatic cells is sufficient to induce TFC fate, we analyzed TFs in ovaries of transgenic animals expressing constitutively active Notch receptor under the control of bab1-Gal4 (see the expression in S1F Fig). Consistent with the previous observation that the activation of Notch signaling coincides with the acquisition of TF cell fate, the expression of constitutively active Notch receptor in TFC precursors (bab1-Gal4>UAS NotchCA) led to the significant increase in TFCs per TF numbers (Fig 3G and 3H, pink, and S1B Table). These data show that ectopic activation of Notch signaling in ACs promotes TFC specification, suggesting that activated Notch is sufficient to induce TFC fate in a cell-autonomous manner.
Fifthly, since induction of Notch signaling via trans-activation requires the presence of the Notch receptor on the membranes of the signal-receiving cells, we quantified the number of TFCs/TF in Notch-deficient ovaries. In Notch (Nts1) temperature-sensitive mutants kept at the restrictive temperature (25°C) only during niche formation (L3), TFs appeared to be shorter with the numbers of TFCs per stalk distributed from 2 to 10 (Fig 3H, red, and S1B Table). This is significantly different from controls, Nts1 mutants kept at the permissive temperature (18°C) that, similarly to the wild type, had 7 to 9 TFC/TF (Fig 3H, dark green, and S1B Table). These data show that the presence of the Notch receptor in TFC precursors is important, but not essential, for TFC specification.
Together, our data on the germline-specific Delta manipulation and analyses of tudor and Notch mutants show that the TFC fate can be induced by two complementing mechanisms. Germline Delta induces TF cell specification via activation of Notch signaling in the posterior TFC precursors. This would require binding to and cleavage of the Notch receptor in the posterior TFC precursors. At the same time, high levels of non-activated somatic Delta inhibit Notch signaling in the anterior TFC precursors. Therefore, TFC precursor-specific deregulation of the Notch receptor or the Delta ligand in these cells should affect TFC specification. We tested this assumption by decreasing Notch receptor and increasing Delta ligand levels in stem cell niche precursors using a bab1-Gal4 driver. We found that Notch downregulation (bab1-Gal4>UAS NotchRNAi) resulted in the appearance of TF stalks in which the numbers of incorporated TFCs was significantly decreased (Fig 3I and 3J, yellow, and S1B Table). These data show that even in the presence of germline Delta, TFC specification was affected when the levels of the Notch receptor were downregulated in TFC precursors (Fig 3I). In contrast, Delta ligand overexpression (bab1-Gal4>UAS Delta, Fig 3J, violet, and S1B Table) resulted in the appearance of TFs which contained significantly more TFCs in comparison to control (bab1-Gal4>GFP, Fig 3J, blue, and S1B Table) and in general a broader distribution of TFC/TF (from 2 to 14). These data show that even if the Notch receptor in soma and the Delta ligand in germline are normally expressed, ectopic Delta expression in the stem cell niche precursors affects their cell fate determination, resulting in abnormally formed TFs.
Together, these studies demonstrate that there are overlapping mechanisms to secure that the precursor cells acquire a certain Notch signaling status necessary for TF cell specification: inhibition of Notch signaling by Delta produced by somatic TFC precursors per se and activation of Notch signaling via distant induction by the germline-produced Delta ligand.
The pattern of Notch signaling activation in TFC precursors is perturbed in Delta germline mutants
To further support the model that there are two mechanisms controlled by Notch signaling that play roles in the establishment of TF stalks, we analyzed the pattern of Notch activation in various mutants with perturbed expression of the Delta ligand and Notch receptor. According to the model, Notch signaling in the four posterior TFCs is activated by germline-derived Delta (Fig 4A); however, when Delta is downregulated in the germline, Notch signaling is not properly activated. Instead of inducing Notch activity in the somatic cells adjacent to the germline in a disc-like pattern, Notch signaling is randomly activated in the more anterior somatic cells in a “salt & pepper” pattern (Fig 4B, nos>DlRNAi). We propose that in the absence of germline Delta, somatic Delta plays a role in Notch signaling activation in the TFC precursors. Our expression analysis shows the Delta ligand as well as the Notch receptor are co-expressed in the TFC precursors, and it has been shown before that in a case when a population of cells co-expresses Notch and Delta, according to the rules of lateral inhibition, at least one cell has to shift the balance to express more Notch or Delta, which immediately will initiate the opposite (Delta or Notch) cell fate in the adjacent neighbor. Even in the Petri dish, cells will spontaneously self-organize into a reiterative “salt & pepper” pattern of Notch signal-receiving and Notch signal-sending cell fates [7,19,22,45]. Therefore, it is possible to activate Notch signaling and induce TF cell fate in some of the Delta-Notch co-expressing anterior somatic cells even without the instructions of the germline Delta.
Moreover, when Delta is upregulated in the germline, more Delta is produced and as a result, the Notch activity reporter is activated in a wider range of TFC precursors (Fig 4C, nos>Dl). However, when Delta is downregulated in ACs, Notch signaling is not only activated in the somatic TFC precursors adjacent to the germline, but in some ACs located more anteriorly that normally express high Delta needed to suppress Notch signaling (Fig 4D, bab1>DlRNAi). It suggests that downregulating Delta expression in the anterior TFC precursors limits the ability of the highly expressed Delta ligand to inhibit Notch signaling.
Also, as expected, when the Notch receptor is downregulated in the Delta-receiving somatic TFC precursors, the E(spl)mβ-CD2 reporter expression is weaker and has less distinct pattern when compared to control (Fig 4E, bab1>NRNAi). At the same time, the expression of the constitutively active Notch receptor in TFC precursors induced Notch signaling in all bab1-expressing TFCs (Fig 4F, bab1>NCA).
Together these data further support the hypothesis that the germline plays an instructive role in the induction of Notch signaling in the posterior TFC precursors via the trans-activation mode and that the somatic Delta inhibits Notch signaling in the anterior TFC precursors.
To strengthen this statement, we analyzed the pattern of Notch activation (1) in the TFs forming next to Delta-deficient PGCs and (2) in mosaic TFs containing wild type and Delta-deficient TFCs. When germline Delta was perturbed, the TFC precursors juxtapositioned to the mutant PGCs had dramatically reduced levels of E(Spl)mß-CD2 expression, supporting the model that germline Delta plays an instructive role in turning Notch signaling “on” in the posterior TFC precursors (Fig 4G and 4H). When the Delta ligand was deleted in the anterior TFCs, it resulted in the activation of Notch signaling in these cells, which normally do not have Notch signaling “on” (Fig 4I), which supports the idea that the somatic Delta in the anterior TFC precursors inhibits Notch signaling via cis- or trans-inhibition. However, when the Delta mutation occurred in TFCs proximal to the germline, no obvious changes in Notch activity pattern were observed (Fig 4I), which is consistent with our hypothesis that the germline Delta induces Notch signaling in these cells. Importantly, regardless of the Delta clone position, the TF cell identity, as evaluated by the cylindrical cell shape and expression of the stem cell niche marker En, was not altered in Delta-deficient cells. These data additionally support the hypothesis that the TF cell fate can be induced by two different Notch signaling modes that act in parallel.
The germline cells deliver Delta on projections to induce TF specification
Together, our sequential analysis of the Notch signaling activation pattern in the developing ovary and our genetic studies strongly suggest that it is the germline Delta expression that initiates stem cell niche formation. As mentioned before, Delta ligand expression was detected in the PGCs just prior to the beginning of TFC specification, and the first TF precursors that have Notch signaling activated and cell shape changed are the ones juxtapositioned to the germline, implying that the germline is the source of Delta that trans-activates Notch signaling in the ACs. For this type of Notch signaling activation, direct contact between the germline and TFC precursors is required. Since Notch signaling was activated several cell diameters away from the germline, we hypothesized that primordial germ cells could form projections that deliver Delta at a distance. We tested this hypothesis using several approaches.
Firstly, to test if cells in the developing ovary have any projections, we expressed membrane-bound GFP (myr::GFP) using the germline-specific nos-Gal4 and somatic niche-specific bab1-Gal4 drivers, which allowed the visualization of contours of the germline and somatic stem cell niche cells. Analysis in live ovaries showed that the PGCs can form ultrafine cellular projections (Fig 5A and 5B, arrows), while in the somatic niche cell these structures were not apparent (Fig 5C).
Secondly, to test if PGCs can form projections long enough to reach TFC precursors positioned 4–5 cells away from the germline, we checked the projection length in PGCs using Life.Act-GFP driven by the germline nos-Gal4 driver. We found that these structures can be up to 12 μm long (Fig 5D), while the length of the TF is ~16–20 μm and the diameter and height of each cylindrical TFC is 9–12 μm and 1.5–3 μm, respectively (Fig 5C). These data demonstrate that the PGC can form cellular extensions which would allow them to communicate with somatic cells located even more than 4 cell diameters away. Supporting this hypothesis, it has been recently shown that adult GSCs can form various cellular projections to fine-tune Dpp signaling [52] and to reach and tightly ensheath CpCs [33].
Thirdly, to detect the presence of Delta on the germline projections, we performed immunohistostaining of the developing ovaries using anti-Delta antibodies (Fig 5G). As shown above, Delta is broadly expressed in the developing ovary (Fig 2A–2C). Upon tissue fixation, the ultrafine projections are largely destroyed (compare Fig 5D and 5E); however, we could distinctly detect the presence of the Delta ligand on the remaining parts of these microscopic structures (Fig 5F). To further test if Delta can decorate the germline cell projections, we expressed GFP-tagged Delta protein using a germline-specific driver (Fig 5G). Analysis of Delta subcellular distribution in the germline cells additionally confirms that the ligand Delta can be present on the germline cell projections. Together, these data demonstrate that PGCs can form cellular projections decorated with Delta that can extend for several cell diameters.
Actin cytoskeleton plays a role in PGC projection formation
To further demonstrate that the cellular projections generated by the germline play a role in ovarian stem cell niche assembly, we performed a pilot genetic screen. We studied mutants for cytoskeleton-maintaining factors, deregulation of which affects the formation of cellular projections. In particular, we focused on factors that have been shown to play a role in the Drosophila germline: i) Actin-related protein 1 (Arp1) which is the short filamentous component of the Dynactin complex that plays an essential role in the activation of the Dynein microtubule motor protein [53]; ii) a Wiskott-Aldrich Syndrome family protein (WASp) member, SCAR, which is an activator of the Arp2/3 complex that promotes actin polymerization and influences cell shape and motility [54]; and iii) a processive actin polymerase Diaphanous (Dia), which nucleates actin filaments de novo, stimulating actin addition at the barbed end and regulates cell shape change and projections [55]. Due to the lethality caused by the loss-of-function of these cell shape regulators, we analyzed their heterozygous mutants (Fig 6). We found that downregulation of any of these factors resulted in the significant alteration of the TFC number per TF. In general, TF had smaller numbers of TFCs, suggesting that actin dynamics affects TF assembly (Fig 6A–6E, blue, yellow, red, and S1C Table). Moreover, the germline-specific downregulation of the actin-binding protein SCAR and the actin-related protein Arp1 caused the appearance of short TFs, in which TFC numbers ranged from 3 to 9, in comparison to 8–9 in controls (Fig 6C–6F, violet, magenta, and S1C Table). This implies that the ability of the cytoskeleton to rearrange, specifically in the germline, plays an important role in TF formation.
It has also been shown that cellular projections generated by both communicating cells are important for proper signaling [56–59]. Therefore, we also perturbed actin cytoskeleton remodeling in the somatic stem cell niche cells using Scar and Arp1 RNAi driven by bab1-Gal4 (Fig 6G and S1C Table). Interestingly, the distribution of TFC numbers per TF was moderately but significantly altered when actin cytoskeleton remodeling was perturbed in the somatic TFC precursors. These data suggest that in the developing ovary, two-way signaling between the germline and soma exists and is communicated via cellular projections.
Finally, to see the significance of actin remodeling on germline projections, we studied their appearance in mutants with germline-specific downregulation of Arp1 (Fig 6H–6I). Comparisons of PGC cell projections marked by Life.Act-GFP of control and actin germline mutants demonstrate that in mutants, the germline projections appear to be noticeably smaller (finer and shorter). These data imply that actin cytoskeleton remodeling is involved in the formation of cellular protrusions in the PGCs and that these protrusions play a role in germline-to-soma communications, establishing the specific signaling pattern necessary for proper cell niche assembly. Combined, these results demonstrate that to induce Notch signaling, the Delta ligand produced by the germline is delivered via actin-mediated cellular projections to the somatic precursor cells positioned several cell diameters away from the Delta source. This is an example of Notch signaling activation among non-equipotent cells via a distant induction mode.
Discussion
Here we show that the formation of the germline stem cell niche in Drosophila depends on the accuracy of spatial patterning within the developing organ, which is controlled by differential activity of Notch signaling (Fig 7). In particular, extrinsic induction (trans-activation) of Notch signaling in TFC precursors by the germline-produced Delta ligand regulates the key step of ovarian morphogenesis, TFC fate acquisition, which leads to the assembly of individual TF stalks. The germline acts as a source of Delta that activates Notch in the adjacent anterior somatic cells; moreover, cellular projections allow refinement of the Notch signaling pattern. They are formed by primordial germ cells and sent several cell diameters to specify TFCs. Additionally, the Notch-Delta interaction between anterior TFC precursors also contribute to TFC specification. Thus, to initiate the germline stem cell niche formation, Notch signaling is patterned by two different mechanisms that act in parallel. Later, TFs also act as Notch-signal sending centers to activate Notch signaling in GSC niche cell precursors, which requires that the status of Notch signaling in one of the posterior TF cells (Transition Cell, dark blue, Fig 7) is reprogrammed from the Notch signal-receiving to Delta-expressing cell [31]. Thus, our data show that during the process of Drosophila ovarian morphogenesis, multiple layers of Notch signaling pathway activation define the specificity of various niche cell fates in the process of the stem cell niche unit assembly.
Apparently, the acquisition of a certain status of Notch signaling (ON/OFF, low/high) is key for niche cells’ terminal differentiation and function as a lifetime support for germline stem cells. Notch signaling is predominantly considered to act as short-range juxtacrine signaling between adjacent cells [11,60]. Here we also see that Notch can be categorized as medium-range signaling used for cell-to-cell communications, where the Delta ligand plays the role of a distant signaling factor. It is produced by a Notch signal-sending cell, and its interaction with the Notch receptor in the nearby and distant cells results in a change in their cell fate. There are several critical steps in posttranslational processing of the Delta ligand necessary for its full activation [61]; however, it is not clear what would affect the activity of Delta as a distant signaling ligand. Recent findings increasingly suggest that cells directly communicate with each other via cellular projections to ensure effectiveness and selectivity of cell-to-cell signaling [62–65]. In particular, they have been shown to be important for BMP signaling communication between Drosophila GSC and their niches [52,66]. Dynamic filopodia in the developing wing disk that are induced by Delta expression allow refinement of the distant Notch signaling pattern [12,13]. Here we demonstrate that the germline-produced Delta can induce a Notch active cell state in the somatic cells that are at least 4 cell diameters away from the Delta source and that the germline cells form extended projections that are decorated with the Delta protein. The Delta ligand is delivered to the membranes of the posterior TFC precursors via these subcellular structures to initiate stem cell niche formation. It would be important to study this process further and identify the type and dynamics of these Delta-positive projections.
Usually, Notch signaling is required to induce different cell fates among equipotent precursor cells. It has also been demonstrated that cells of different origin can communicate via Notch signaling. For example, germline-expressed Delta in the developing oocyte can activate Notch signaling in the adjacent follicular epithelial cells, which induces the mitotic-to-endocycle switch in these cells adjacent to the Delta source [42]. However, it has not been shown before that the distant induction of Notch signaling can occur among non-equipotent cells, where one cell type sends Delta ligand across several cell diameters to cells of another origin, such as the germline and somatic cells in the developing gonad.
Intriguingly, we also found that the TFC fate can be induced via two different Notch signaling modes. The GSC niche unit must be positioned next to the germline to induce GSC fate in a group of primordial germ cells; therefore, it is logical that the germline itself is instructive in this process. However, even in germline-less ovaries, TFs and the niche are established, which supports the idea that there is a second mechanism for the induction of TF cell fate. In particular, somatic anterior cells co-express Delta and Notch, which interact in cis or in trans, leading to Notch inhibition in these cells. Apparently, both Notch activation and Notch inhibition in anterior somatic cells allows them to become TF cells. Similarly, we have recently described that a second mechanism that secures Notch signaling activation also exists to ensure the robustness of stem cell niche assembly [31]. Normally, steroid signaling induces TFC reprogramming into a Delta-sending cell that can induce the perfect hexagonal Notch-signaling pattern in the adjacent CpC precursors via the local induction mechanism (Fig 1A). In addition, Notch signaling can be activated via lateral inhibition, which occurs among the equivalent cell populations. In this case, stem cell niche precursor cells (ICs) are bivalent and co-express both the Delta ligand and Notch receptor. They can acquire Notch active status stochastically, since even without inductive signaling, fluctuations in Delta expression permit one random cell to win and induce Notch signaling in the adjacent cells, which converts them into niche cells and results in the appearance of ectopic niches [31]. Therefore, the niche precursor cell bistability can be resolved by two mechanisms of Notch signaling activation: peripheral local induction and lateral inhibition, which is extrapolated onto the patterning of the adult stem cell niche.
Interestingly, even though posterior TFCs and CpCs both exhibit active Notch signaling, the intensity of Notch activation is different in these cells: TFCs have high, while CpCs have low Notch activity. Recently it has been proposed that the geometry of cell-to-cell contacts influences long- and short-range signaling and diversifies signaling patterns [21]. This work assumes that the kinetics of Notch-Delta signaling depend on junctional contacts, which are different at the projections and at the cell interfaces. In the case of the current study, these would be the contacts between the Delta-positive germline-generated projections and TFC precursors, or between the Delta-sending reprogrammed TFC and CpC precursors. Moreover, our analyses of actin mutants suggest that that the two-way signaling communicated via cellular projections exists between the germline and somatic cells in the developing ovary. It has been shown previously that cellular projections control various processes, from morphogenesis to tumorigenesis, via the distribution of signaling proteins [56,59,67–69]; thus, it is important to study further the activity of cellular projections to understand how Notch signaling activation depends on the projection-mediated dynamics between the germline and the soma.
Together, these data show that multiple modes of Notch signaling activation indicate the complexity of spatial cellular Delta-Notch interactions, resulting in differential Notch signaling activation, tissue patterning, and maintenance. Even though it takes some developmental time, important is that all TFCs and CpCs eventually acquire a certain Notch signaling status. This promotes establishment of a stable pattern and commitment to a fixed fate, which eventually allows the stem cell niche formation. At the same time, during adulthood, GSC niche cells have fluctuating and possibly self-organizing Notch ON/OFF signaling patterns, which is important, since niche cells are essential for a life-long maintenance of GSCs and must be able to sustain their own cell fate and signaling status. Potentially, bioengineering of self-maintaining stem cell niches for in vivo engraftment, maturation and maintenance of stem cells, and also differentiation niches for governance of the efficiency of stem cell progeny differentiation would be of great advantage for regenerative medicine. In addition, a better understanding of stem cell niches in their natural environment may aid the understanding of the development of many diseases.
Materials and methods
Fly strains and genetics
Fly stocks were maintained at 25°C on a standard cornmeal-agar diet in a controlled environment (constant humidity and light-dark cycle) unless otherwise stated. As Control, OregonR crossed to w1118 line was used.
To manipulate Notch signaling, UASp-Dl [23], UAS-NotchCA [23,51], UASt-Dl-RNAi [Bloomington Drosophila Stock Center (BDSC) 36784], UASt-Dl (BDSC 26695), UASt-NRNAi (BDSC 27988) and Nts1 (gift from Frank Hirth) lines were used. To downregulate Notch levels, Nts1 mutants were kept at a semi-restrictive temperature (25°C) through all stages of development. For ectopic expression in the germline or soma, the following driver lines were used: nanos-Gal4 (nos-NGT-Gal4; VP16-nos.UTR-Gal4; BDSC 4442, BDSC 4937) or bab1-Gal4/TM6 [70], BDSC 6803). To mark germline projections, UASp-Life.Act-mGFP (BDSC 58718) and UAS myr::GFP (BDSC 77124) lines were used. To induce Delta loss-of function clones, FRT 82B Dlrev10/TM3, Sb and hs Flp; FRT 82B Ubi-GFP (BDSC 5188) lines were used [71]. To visualize Notch signaling activity, Notch activity reporters E(Spl)mß-CD2 [gift from Wu-Min Deng [43]] and NRE-GFP (BDSC 30727) were used. To visualize Delta, UAS-Dl::GFP lines were used (BDSC 8610 and 8611). To disturb actin cytoskeleton organization, the following mutants were used: Arp1c (BDSC 11424), SCARd37 (BDSC 8754), dia5 (BDSC 9138), Arp1RNAi (BDSC 67932) and SCARRNAi (BDSC 51803) To obtain ovaries without germline, female progeny from homozygous tudor mutant (tudB42, gift from Ruth Lehmann) were analyzed.
Staging of ovaries
For EL3 stage (72 h AEL), larvae that match criteria of L3 size but still feeding were picked. For LL3 stage (~112 h AEL), larvae that started wandering and were out of the food were picked. For prepupal stages (120h AEL), puparia that were still white but had distinct puparium shape and not moving anymore were picked.
Immunohistochemistry
Ovaries were dissected in phosphate-buffered saline (PBS) and fixed while shaking on a nutator for 15 min in PBS containing 4% formaldehyde. Next, they were rinsed with PBT (PBS/0.2%, Triton X-100) four times (15 min, each rinse) and blocked in PBTB (PBT, 0.2% BSA, 5% Normal Goat Serum) for 1 h at room temperature. The tissue was incubated with primary antibodies overnight at 4°C. The next day, they were rinsed with PBT four times (15 min, each rinse) and blocked in PBTB for 1 h at room temperature. The ovaries were then incubated in secondary antibodies overnight at 4°C. The next day, they were rinsed with PBT (4 times, 15 min each rinse) and stained with DAPI (1 mg/ml in PBT) for 10 min. Finally, they were washed with PBT twice (5 min, each wash) and dissected onto slides in 70% glycerol, 3% NPG, 1× PBS [72]. For live analysis of germline projections, ovaries were dissected in PBS, stained with Hoechst and immediately imaged under the confocal microscope.
The following primary antibodies were used: mouse anti-Engrailed (En; 1:20), mouse anti-NICD (1:20) and mouse anti-Delta (Dl, 1:20) from Developmental Studies Hybridoma Bank, rabbit anti-Vasa (1:5000, gift from Herbert Jäckle), mouse anti-CD2 (1:100, Biolegend), guinea pig anti-Traffic Jam (Tj, 1:5000, gift from D. Godt), chicken anti-GFP (1:5000, Abcam). Secondary antibodies: goat anti-rabbit Alexa 488, goat anti-chicken Alexa 488, and goat anti-guinea pig Alexa 647 (1:500, Life Technologies), goat anti-mouse Cy3 IgG1 and goat anti-mouse Alexa 488 (1:250, Jackson ImmunoResearch Laboratory). For visualizing cell nuclei, DAPI (Sigma) and Hoechst (Thermo Fisher) dyes were used. Samples were analyzed using a confocal microscope (Zeiss LSM 700). For making figures, Adobe Photoshop, Adobe Illustrator and Sketches software were used.
Visualization of cellular projections in live ovaries
Transgenic animals expressing membrane GFP—UASp-Life.Act-mGFP (BDSC 58718) or UAS myr::GFP (BDSC 77124) under control of nanos-Gal4 or bab1-Gal4 drivers were generated. To visualize the GFP expression in the germline or in the somatic cells of the stem niche, prepupal ovaries were dissected in Schneider’s medium. To visualize nuclei, 2 μg/ml solution of Hoechst 33258 (bisbenzimide) DNA stain in Schneider’s medium was used. After 5 min of Hoechst staining, live dissected ovaries were placed on a slide with a drop of Halocarbon oil 27 (Sigma Aldrich), covered with a coverslip, and immediately subjected to confocal imaging.
Analysis of the Notch signaling activity in TFs
Prepupal ovaries of transgenic animals containing Notch activity reporters–E(Spl)mß-CD2 or NRE-GFP–were dissected, fixed, and stained with anti-Delta and anti-GFP antibodies, and DAPI. Fluorescent intensity peaks of the Delta receptor and the Notch signaling activity reporter (GFP) in TFCs were produced using ZEN Lite software.
Analyses of the TFC numbers
To analyze the number of TFCs/TF, Z-stack confocal images of the entire ovary at prepupal stage (120h AEL) with 1 μm intervals were captured. TFCs were identified by the disk-shaped morphology and En expression. Firstly, we quantified the number of TFC per TF in controls and different mutants, which varied from 1 to 15. Secondly, the mean and standard deviation of the number of TFC per TF per ovary of control and the mutant was calculated. Thirdly, a Kruskal-Wallis test was performed to test for difference in means between the control and the mutant. Finally, in order to visualize the difference, each mutant was plotted against the control by calculating the probability of the TFC number per TF using the mean and standard deviation derived from the quantified numbers of TFC per TF in controls and mutants.
Supporting information
S1 Fig [a]
In the developing ovary, the expression patterns of the Notch receptor and the Delta ligand are dynamic.
S2 Fig [a]
Notch signaling activation is differentiation stage-dependent.
S3 Fig [a]
Expression of the Notch signaling reporter in adult germarium.
S4 Fig [green]
Notch is involved in the first step of GSC niche assembly, the process of TF formation.
Zdroje
1. Nandagopal N, Santat LA, LeBon L, Sprinzak D, Bronner ME, Elowitz MB. Dynamic Ligand Discrimination in the Notch Signaling Pathway. Cell. 2018;172(4):869–80 e19. Epub 2018/02/06. doi: 10.1016/j.cell.2018.01.002 29398116.
2. Shaya O, Binshtok U, Hersch M, Rivkin D, Weinreb S, Amir-Zilberstein L, et al. Cell-Cell Contact Area Affects Notch Signaling and Notch-Dependent Patterning. Dev Cell. 2017;40(5):505–11 e6. Epub 2017/03/16. doi: 10.1016/j.devcel.2017.02.009 28292428; PubMed Central PMCID: PMC5435110.
3. Sprinzak D, Lakhanpal A, LeBon L, Garcia-Ojalvo J, Elowitz MB. Mutual inactivation of Notch receptors and ligands facilitates developmental patterning. PLoS Comput Biol. 2011;7(6):e1002069. Epub 2011/06/23. doi: 10.1371/journal.pcbi.1002069 21695234; PubMed Central PMCID: PMC3111533.
4. Fiuza UM, Arias AM. Cell and molecular biology of Notch. J Endocrinol. 2007;194(3):459–74. doi: 10.1677/JOE-07-0242 17761886.
5. Le Borgne R, Bardin A, Schweisguth F. The roles of receptor and ligand endocytosis in regulating Notch signaling. Development. 2005;132(8):1751–62. Epub 2005/03/26. 132/8/1751 [pii] doi: 10.1242/dev.01789 15790962.
6. Lai EC. Notch signaling: control of cell communication and cell fate. Development. 2004;131(5):965–73. Epub 2004/02/20. doi: 10.1242/dev.01074 14973298.
7. Petrovic J, Formosa-Jordan P, Luna-Escalante JC, Abello G, Ibanes M, Neves J, et al. Ligand-dependent Notch signaling strength orchestrates lateral induction and lateral inhibition in the developing inner ear. Development. 2014;141(11):2313–24. doi: 10.1242/dev.108100 24821984.
8. Kushwah R, Guezguez B, Lee JB, Hopkins CI, Bhatia M. Pleiotropic roles of Notch signaling in normal, malignant, and developmental hematopoiesis in the human. EMBO Rep. 2014;15(11):1128–38. doi: 10.15252/embr.201438842 25252682; PubMed Central PMCID: PMC4253487.
9. Vanorny DA, Mayo KE. The role of Notch signaling in the mammalian ovary. Reproduction. 2017;153(6):R187–R204. Epub 2017/03/12. doi: 10.1530/REP-16-0689 28283672; PubMed Central PMCID: PMC5512555.
10. Wilkinson HA, Fitzgerald K, Greenwald I. Reciprocal changes in expression of the receptor lin-12 and its ligand lag-2 prior to commitment in a C. elegans cell fate decision. Cell. 1994;79(7):1187–98. Epub 1994/12/30. doi: 10.1016/0092-8674(94)90010-8 8001154.
11. Kovall RA, Gebelein B, Sprinzak D, Kopan R. The Canonical Notch Signaling Pathway: Structural and Biochemical Insights into Shape, Sugar, and Force. Dev Cell. 2017;41(3):228–41. Epub 2017/05/10. doi: 10.1016/j.devcel.2017.04.001 28486129; PubMed Central PMCID: PMC5492985.
12. De Joussineau C, Soule J, Martin M, Anguille C, Montcourrier P, Alexandre D. Delta-promoted filopodia mediate long-range lateral inhibition in Drosophila. Nature. 2003;426(6966):555–9. Epub 2003/12/05. doi: 10.1038/nature02157 14654840.
13. Cohen M, Georgiou M, Stevenson NL, Miodownik M, Baum B. Dynamic filopodia transmit intermittent Delta-Notch signaling to drive pattern refinement during lateral inhibition. Dev Cell. 2010;19(1):78–89. Epub 2010/07/21. doi: 10.1016/j.devcel.2010.06.006 20643352.
14. Hunter GL, Hadjivasiliou Z, Bonin H, He L, Perrimon N, Charras G, et al. Coordinated control of Notch/Delta signalling and cell cycle progression drives lateral inhibition-mediated tissue patterning. Development. 2016;143(13):2305–10. doi: 10.1242/dev.134213 27226324; PubMed Central PMCID: PMC4958321.
15. Boukhatmi H, Martins T, Pillidge Z, Kamenova T, Bray S. Notch Mediates Inter-tissue Communication to Promote Tumorigenesis. Curr Biol. 2020. Epub 2020/04/11. doi: 10.1016/j.cub.2020.02.088 32275875.
16. Khait I, Orsher Y, Golan O, Binshtok U, Gordon-Bar N, Amir-Zilberstein L, et al. Quantitative Analysis of Delta-like 1 Membrane Dynamics Elucidates the Role of Contact Geometry on Notch Signaling. Cell Rep. 2016;14(2):225–33. Epub 2016/01/11. doi: 10.1016/j.celrep.2015.12.040 26748704.
17. del Alamo D, Rouault H, Schweisguth F. Mechanism and significance of cis-inhibition in Notch signalling. Curr Biol. 2011;21(1):R40–7. doi: 10.1016/j.cub.2010.10.034 21215938.
18. Palmer WH, Jia D, Deng WM. Cis-interactions between Notch and its ligands block ligand-independent Notch activity. Elife. 2014;3. doi: 10.7554/eLife.04415 25486593; PubMed Central PMCID: PMC4286723.
19. Sprinzak D, Lakhanpal A, Lebon L, Santat LA, Fontes ME, Anderson GA, et al. Cis-interactions between Notch and Delta generate mutually exclusive signalling states. Nature. 2010;465(7294):86–90. Epub 2010/04/27. doi: 10.1038/nature08959 20418862; PubMed Central PMCID: PMC2886601.
20. Mukherjee T, Kim WS, Mandal L, Banerjee U. Interaction between Notch and Hif-alpha in development and survival of Drosophila blood cells. Science. 2011;332(6034):1210–3. doi: 10.1126/science.1199643 21636775; PubMed Central PMCID: PMC4412745.
21. Hadjivasiliou Z, Hunter GL, Baum B. A new mechanism for spatial pattern formation via lateral and protrusion-mediated lateral signalling. J R Soc Interface. 2016;13(124). Epub 2016/11/04. doi: 10.1098/rsif.2016.0484 27807273; PubMed Central PMCID: PMC5134009.
22. Barad O, Rosin D, Hornstein E, Barkai N. Error minimization in lateral inhibition circuits. Sci Signal. 2010;3(129):ra51. doi: 10.1126/scisignal.2000857 20606215.
23. Ward EJ, Shcherbata HR, Reynolds SH, Fischer KA, Hatfield SD, Ruohola-Baker H. Stem cells signal to the niche through the Notch pathway in the Drosophila ovary. Curr Biol. 2006;16(23):2352–8. Epub 2006/10/31. doi: 10.1016/j.cub.2006.10.022 17070683.
24. Song X, Call GB, Kirilly D, Xie T. Notch signaling controls germline stem cell niche formation in the Drosophila ovary. Development. 2007;134(6):1071–80. doi: 10.1242/dev.003392 17287246.
25. Williamson A, Lehmann R. Germ cell development in Drosophila. Annual review of cell and developmental biology. 1996;12:365–91. Epub 1996/01/01. doi: 10.1146/annurev.cellbio.12.1.365 8970731.
26. Godt D, Laski FA. Mechanisms of cell rearrangement and cell recruitment in Drosophila ovary morphogenesis and the requirement of bric a brac. Development. 1995;121(1):173–87. Epub 1995/01/01. 7867498.
27. Li MA, Alls JD, Avancini RM, Koo K, Godt D. The large Maf factor Traffic Jam controls gonad morphogenesis in Drosophila. Nature cell biology. 2003;5(11):994–1000. Epub 2003/10/28. doi: 10.1038/ncb1058 14578908.
28. Asaoka M, Lin H. Germline stem cells in the Drosophila ovary descend from pole cells in the anterior region of the embryonic gonad. Development. 2004;131(20):5079–89. Epub 2004/10/02. doi: 10.1242/dev.01391 15459101.
29. Gilboa L. Organizing stem cell units in the Drosophila ovary. Curr Opin Genet Dev. 2015;32:31–6. Epub 2015/02/24. doi: 10.1016/j.gde.2015.01.005 25703842.
30. Chen J, Godt D, Gunsalus K, Kiss I, Goldberg M, Laski FA. Cofilin/ADF is required for cell motility during Drosophila ovary development and oogenesis. Nature cell biology. 2001;3(2):204–9. doi: 10.1038/35055120 11175754.
31. Yatsenko AS, Shcherbata HR. Stereotypical architecture of the stem cell niche is spatiotemporally established by miR-125-dependent coordination of Notch and steroid signaling. Development. 2018;145(3). Epub 2018/01/24. doi: 10.1242/dev.159178 29361571; PubMed Central PMCID: PMC5818007.
32. Eliazer S, Buszczak M. Finding a niche: studies from the Drosophila ovary. Stem cell research & therapy. 2011;2(6):45. Epub 2011/11/29. doi: 10.1186/scrt86 22117545; PubMed Central PMCID: PMC3340554.
33. Panchal T, Chen X, Alchits E, Oh Y, Poon J, Kouptsova J, et al. Specification and spatial arrangement of cells in the germline stem cell niche of the Drosophila ovary depend on the Maf transcription factor Traffic jam. PLoS Genet. 2017;13(5):e1006790. Epub 2017/05/26. doi: 10.1371/journal.pgen.1006790 28542174; PubMed Central PMCID: PMC5459507.
34. Spradling AC, Nystul T, Lighthouse D, Morris L, Fox D, Cox R, et al. Stem cells and their niches: integrated units that maintain Drosophila tissues. Cold Spring Harb Symp Quant Biol. 2008;73:49–57. Epub 2008/11/22. sqb.2008.73.023 [pii] doi: 10.1101/sqb.2008.73.023 19022764.
35. Chen D, McKearin DM. A discrete transcriptional silencer in the bam gene determines asymmetric division of the Drosophila germline stem cell. Development. 2003;130(6):1159–70. Epub 2003/02/07. doi: 10.1242/dev.00325 12571107.
36. Xie T, Spradling AC. decapentaplegic is essential for the maintenance and division of germline stem cells in the Drosophila ovary. Cell. 1998;94(2):251–60. Epub 1998/08/08. S0092-8674(00)81424-5 [pii]. doi: 10.1016/s0092-8674(00)81424-5 9695953.
37. Song X, Wong MD, Kawase E, Xi R, Ding BC, McCarthy JJ, et al. Bmp signals from niche cells directly repress transcription of a differentiation-promoting gene, bag of marbles, in germline stem cells in the Drosophila ovary. Development. 2004;131(6):1353–64. Epub 2004/02/20. doi: 10.1242/dev.01026 [pii]. 14973291.
38. Hsu HJ, Drummond-Barbosa D. Insulin signals control the competence of the Drosophila female germline stem cell niche to respond to Notch ligands. Developmental biology. 2011;350(2):290–300. Epub 2010/12/15. doi: 10.1016/j.ydbio.2010.11.032 21145317.
39. Shimizu H, Wilkin MB, Woodcock SA, Bonfini A, Hung Y, Mazaleyrat S, et al. The Drosophila ZO-1 protein Polychaetoid suppresses Deltex-regulated Notch activity to modulate germline stem cell niche formation. Open Biol. 2017;7(4). Epub 2017/04/21. doi: 10.1098/rsob.160322 28424321; PubMed Central PMCID: PMC5413905.
40. Langridge PD, Struhl G. Epsin-Dependent Ligand Endocytosis Activates Notch by Force. Cell. 2017;171(6):1383–96 e12. Epub 2017/12/02. doi: 10.1016/j.cell.2017.10.048 29195077.
41. Trylinski M, Mazouni K, Schweisguth F. Intra-lineage Fate Decisions Involve Activation of Notch Receptors Basal to the Midbody in Drosophila Sensory Organ Precursor Cells. Curr Biol. 2017;27(15):2239–47 e3. Epub 2017/07/25. doi: 10.1016/j.cub.2017.06.030 28736165.
42. Shcherbata HR, Althauser C, Findley SD, Ruohola-Baker H. The mitotic-to-endocycle switch in Drosophila follicle cells is executed by Notch-dependent regulation of G1/S, G2/M and M/G1 cell-cycle transitions. Development. 2004;131(13):3169–81. Epub 2004/06/04. doi: 10.1242/dev.01172 15175253.
43. de Celis JF, Tyler DM, de Celis J, Bray SJ. Notch signalling mediates segmentation of the Drosophila leg. Development. 1998;125(23):4617–26. 9806911.
44. Bolivar J, Pearson J, Lopez-Onieva L, Gonzalez-Reyes A. Genetic dissection of a stem cell niche: the case of the Drosophila ovary. Dev Dyn. 2006;235(11):2969–79. doi: 10.1002/dvdy.20967 17013875.
45. Matsuda M, Koga M, Woltjen K, Nishida E, Ebisuya M. Synthetic lateral inhibition governs cell-type bifurcation with robust ratios. Nat Commun. 2015;6:6195. doi: 10.1038/ncomms7195 25652697.
46. Gancz D, Gilboa L. Insulin and Target of rapamycin signaling orchestrate the development of ovarian niche-stem cell units in Drosophila. Development. 2013;140(20):4145–54. Epub 2013/09/13. doi: 10.1242/dev.093773 24026119.
47. Gancz D, Lengil T, Gilboa L. Coordinated regulation of niche and stem cell precursors by hormonal signaling. PLoS biology. 2011;9(11):e1001202. Epub 2011/12/02. doi: 10.1371/journal.pbio.1001202 22131903; PubMed Central PMCID: PMC3222635.
48. Sarikaya DP, Extavour CG. The Hippo pathway regulates homeostatic growth of stem cell niche precursors in the Drosophila ovary. PLoS Genet. 2015;11(2):e1004962. doi: 10.1371/journal.pgen.1004962 25643260.
49. Hodin J, Riddiford LM. The ecdysone receptor and ultraspiracle regulate the timing and progression of ovarian morphogenesis during Drosophila metamorphosis. Dev Genes Evol. 1998;208(6):304–17. doi: 10.1007/s004270050186 9716721.
50. Assa-Kunik E, Torres IL, Schejter ED, Johnston DS, Shilo BZ. Drosophila follicle cells are patterned by multiple levels of Notch signaling and antagonism between the Notch and JAK/STAT pathways. Development. 2007;134(6):1161–9. Epub 2007/03/03. doi: 10.1242/dev.02800 17332535.
51. Larkin MK, Holder K, Yost C, Giniger E, Ruohola-Baker H. Expression of constitutively active Notch arrests follicle cells at a precursor stage during Drosophila oogenesis and disrupts the anterior-posterior axis of the oocyte. Development. 1996;122(11):3639–50. Epub 1996/11/01. 8951079.
52. Wilcockson SG, Ashe HL. Drosophila Ovarian Germline Stem Cell Cytocensor Projections Dynamically Receive and Attenuate BMP Signaling. Dev Cell. 2019;50(3):296–312 e5. Epub 2019/06/11. doi: 10.1016/j.devcel.2019.05.020 31178401; PubMed Central PMCID: PMC6688100.
53. Nieuwburg R, Nashchekin D, Jakobs M, Carter AP, Khuc Trong P, Goldstein RE, et al. Localised dynactin protects growing microtubules to deliver oskar mRNA to the posterior cortex of the Drosophila oocyte. Elife. 2017;6. Epub 2017/10/17. doi: 10.7554/eLife.27237 29035202; PubMed Central PMCID: PMC5643094.
54. Rodriguez-Mesa E, Abreu-Blanco MT, Rosales-Nieves AE, Parkhurst SM. Developmental expression of Drosophila Wiskott-Aldrich Syndrome family proteins. Dev Dyn. 2012;241(3):608–26. Epub 2012/01/26. doi: 10.1002/dvdy.23742 22275148; PubMed Central PMCID: PMC3288701.
55. Roy S, Huang H, Liu S, Kornberg TB. Cytoneme-mediated contact-dependent transport of the Drosophila decapentaplegic signaling protein. Science. 2014;343(6173):1244624. Epub 2014/01/05. doi: 10.1126/science.1244624 24385607; PubMed Central PMCID: PMC4336149.
56. Ramirez-Weber FA, Kornberg TB. Cytonemes: cellular processes that project to the principal signaling center in Drosophila imaginal discs. Cell. 1999;97(5):599–607. Epub 1999/06/15. doi: 10.1016/s0092-8674(00)80771-0 10367889.
57. Hsiung F, Ramirez-Weber FA, Iwaki DD, Kornberg TB. Dependence of Drosophila wing imaginal disc cytonemes on Decapentaplegic. Nature. 2005;437(7058):560–3. Epub 2005/09/24. doi: 10.1038/nature03951 16177792.
58. Chen W, Huang H, Hatori R, Kornberg TB. Essential basal cytonemes take up Hedgehog in the Drosophila wing imaginal disc. Development. 2017;144(17):3134–44. Epub 2017/07/27. doi: 10.1242/dev.149856 28743798; PubMed Central PMCID: PMC5611956.
59. Fereres S, Hatori R, Hatori M, Kornberg TB. Cytoneme-mediated signaling essential for tumorigenesis. PLoS Genet. 2019;15(9):e1008415. Epub 2019/10/01. doi: 10.1371/journal.pgen.1008415 31568500; PubMed Central PMCID: PMC6786653.
60. Yamamoto S, Schulze KL, Bellen HJ. Introduction to Notch signaling. Methods Mol Biol. 2014;1187:1–14. Epub 2014/07/24. doi: 10.1007/978-1-4939-1139-4_1 25053477.
61. Perez-Mockus G, Schweisguth F. Cell Polarity and Notch Signaling: Linked by the E3 Ubiquitin Ligase Neuralized? Bioessays. 2017;39(11). Epub 2017/09/25. doi: 10.1002/bies.201700128 28940548.
62. Bischoff M, Gradilla AC, Seijo I, Andres G, Rodriguez-Navas C, Gonzalez-Mendez L, et al. Cytonemes are required for the establishment of a normal Hedgehog morphogen gradient in Drosophila epithelia. Nature cell biology. 2013;15(11):1269–81. doi: 10.1038/ncb2856 24121526; PubMed Central PMCID: PMC3840581.
63. Huang H, Kornberg TB. Cells must express components of the planar cell polarity system and extracellular matrix to support cytonemes. Elife. 2016;5. doi: 10.7554/eLife.18979 27591355; PubMed Central PMCID: PMC5030081.
64. Konig A, Shcherbata HR. Soma influences GSC progeny differentiation via the cell adhesion-mediated steroid-let-7-Wingless signaling cascade that regulates chromatin dynamics. Biol Open. 2015;4(3):285–300. Epub 2015/02/11. doi: 10.1242/bio.201410553 25661868; PubMed Central PMCID: PMC4359735.
65. Rojas-Rios P, Guerrero I, Gonzalez-Reyes A. Cytoneme-mediated delivery of hedgehog regulates the expression of bone morphogenetic proteins to maintain germline stem cells in Drosophila. PLoS biology. 2012;10(4):e1001298. Epub 2012/04/18. doi: 10.1371/journal.pbio.1001298 22509132; PubMed Central PMCID: PMC3317903.
66. Inaba M, Buszczak M, Yamashita YM. Nanotubes mediate niche-stem-cell signalling in the Drosophila testis. Nature. 2015;523(7560):329–32. Epub 2015/07/02. doi: 10.1038/nature14602 26131929; PubMed Central PMCID: PMC4586072.
67. Roy S, Hsiung F, Kornberg TB. Specificity of Drosophila cytonemes for distinct signaling pathways. Science. 2011;332(6027):354–8. Epub 2011/04/16. doi: 10.1126/science.1198949 21493861; PubMed Central PMCID: PMC3109072.
68. Kornberg TB. Cytonemes extend their reach. EMBO J. 2013;32(12):1658–9. Epub 2013/05/16. doi: 10.1038/emboj.2013.115 23673359; PubMed Central PMCID: PMC3680737.
69. Kornberg TB. Distributing signaling proteins in space and time: the province of cytonemes. Curr Opin Genet Dev. 2017;45:22–7. Epub 2017/03/01. doi: 10.1016/j.gde.2017.02.010 28242479; PubMed Central PMCID: PMC5502195.
70. Couderc JL, Godt D, Zollman S, Chen J, Li M, Tiong S, et al. The bric a brac locus consists of two paralogous genes encoding BTB/POZ domain proteins and acts as a homeotic and morphogenetic regulator of imaginal development in Drosophila. Development. 2002;129(10):2419–33. Epub 2002/04/26. 11973274.
71. Heitzler P, Simpson P. The choice of cell fate in the epidermis of Drosophila. Cell. 1991;64(6):1083–92. Epub 1991/03/22. doi: 10.1016/0092-8674(91)90263-x 2004417.
72. Konig A, Shcherbata HR. Visualization of adult stem cells within their niches using the Drosophila germline as a model system. Methods Mol Biol. 2013;1035:25–33. Epub 2013/08/21. doi: 10.1007/978-1-62703-508-8_3 23959979.
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